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Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary and its effect on oocyte nuclear maturation in vitro
Accepted Manuscript Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary and its effect on oocyte nuclear maturation in vitro Bruna S.P. Oliveira, Joana A.S. Costa, Elizabete T. Gomes, Diogo M.F. Silva, Sandra M. Torres, Pedro L.J. Monteiro, Jr., Antônio S. Santos Filho, Maria Madalena P. Guerra, Gustavo F. Carneiro, Aurea Wischral, André M. Batista PII:
S0093-691X(17)30398-9
DOI:
10.1016/j.theriogenology.2017.08.013
Reference:
THE 14233
To appear in:
Theriogenology
Received Date: 5 May 2017 Revised Date:
30 July 2017
Accepted Date: 10 August 2017
Please cite this article as: Oliveira BSP, Costa JAS, Gomes ET, Silva DMF, Torres SM, Monteiro Jr. PLJ, Santos Filho AntôS, Guerra MMP, Carneiro GF, Wischral A, Batista AndréM, Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary and its effect on oocyte nuclear maturation in vitro, Theriogenology (2017), doi: 10.1016/j.theriogenology.2017.08.013. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
Revised
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Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary
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and its effect on oocyte nuclear maturation in vitro
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Bruna S. P. Oliveiraa, Joana A. S. Costaa, Elizabete T. Gomesa, Diogo M. F. Silvaa,
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Sandra M. Torresa, Pedro L. J. Monteiro Jrb, Antônio S. Santos Filhoc, Maria Madalena
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P.Guerraa, Gustavo F. Carneirod, Aurea Wischrala, André M. Batistaa,*
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a
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Pernambuco, Brazil.
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Department of Animal Science, University of São Paulo, Piracicaba, SP, Brazil.
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Agronomic Institute of Pernambuco, Arcoverde, PE, Brazil.
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UAG/University Federal Rural of Pernambuco, Garanhuns, PE, Brazil.
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Department of Veterinary Medicine, Federal Rural University of Pernambuco, Recife,
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* Corresponding author: Department of Veterinary Medicine, Rural Federal
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University of Pernambuco, Dom Manoel de Medeiros street, s/n, Dois Irmãos, CEP
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52171-900, Recife, Pernambuco, Brazil. Tel.: +55 81 3320 6414; fax: +55 81 3320
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6057. E-mail address: [email protected]
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ACCEPTED MANUSCRIPT ABSTRACT
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Adiponectin is an adipokine secreted primarily by adipocytes and is involved in the
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control of male and female reproductive functions. Circulating levels of adiponectin are
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inversely correlated with body fat mass, and its biological effects are predominantly
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mediated through two receptors, AdipoR1 and AdipoR2. The aim of the present study
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was to verify the expression of the adiponectin system (adiponectin and its receptors,
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AdipoR1 and AdipoR2) in goat ovary using qPCR and immunohistochemistry analyses
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and further investigate the in vitro effects of recombinant adiponectin (5 µg/mL and 10
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µg/mL) on goat oocyte nuclear maturation. We demonstrated that the mRNA and
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proteins of the adiponectin system are present in goat ovary. Gene and protein
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expression of AdipoR1 and AdipoR2 was detected in follicular cells (oocyte, cumulus,
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granulosa and theca) of small and large antral follicles, while adiponectin mRNA was
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not detected in oocytes from small and large follicles or in large follicle cumulus cells.
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Finally, addition of various concentrations of adiponectin in maturation medium
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affected the number of oocytes that reached metaphase II. In conclusion, in the present
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study, we detected expression of adiponectin and its receptors AdipoR1 and AdipoR2 in
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goat ovarian follicles. Furthermore, we demonstrated that recombinant adiponectin
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increases nuclear maturation of goat oocytes in vitro.
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Keywords: follicle, ovary, goat, adipose tissue, gene expression
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1. Introduction
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Increased livestock productivity has become a major research topic in response
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to increases in the population and consumption [1]. In this context, understanding the
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reproductive physiology of these animals is key to improving reproductive techniques
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and, consequently, increasing productivity. In ruminants, reproductive function can be 2
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influenced at different levels of the hypothalamic-pituitary-gonadal axis by energetic
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alterations related to diet [2], with a well-known relationship between energetic balance
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and reproduction [3]. Adipose tissue, once recognized only for its role as an energy reservoir, has been
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identified as an important modulator of this relationship [4,5]. Now recognized as an
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endocrine organ, adipose tissue releases a wide variety of protein factors called
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adipokines [6]. These adipokines have important effects on various physiological
58
processes, including reproduction [7]. Adiponectin, a 30 kDa, 244 amino acid protein,
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has an N-terminal signal sequence, a species-dependent variable sequence, a collagen
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domain, and a C-terminal globular domain [8,9]. Its secretion is inversely related to
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adipose tissue levels [10], and its circulating levels are two to three times higher in
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females than those in males [11].
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Adiponectin acts through two specific membrane receptors, AdipoR1 and
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AdipoR2 [12]. These receptors are formed by seven transmembrane domains, with an
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intracellular N-terminus and an extracellular C-terminus, and have an opposite
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orientation to that of classical G-proteins-coupled receptors [13,14]. The adiponectin
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system was identified in different organs of the female reproductive system in various
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species. Adiponectin, AdipoR1 and AdipoR2 were observed in ovarian cells of cattle
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[15], chickens [16], mice [17] and swine [18]. AdipoR1 and AdipoR2 were also
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identified in ovarian fish cells [19] and humans [20,21]. Adiponectin protein was also
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visualized in ovine follicular cells [22].
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The literature suggests that adiponectin has a steroidogenic effect on ovarian
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function. In pigs, in vitro studies have shown that adiponectin reduced basal
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testosterone secretion in internal theca cells; in granulosa cells, it increased secretion of
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estradiol and, in combination with insulin, increased secretion of progesterone [23]. In
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progesterone and estradiol [20]. In chickens, adiponectin was also shown to modify the
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progesterone secretion pattern induced by LH, FSH or IGF-1 in granulosa cells [16].
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This adipokine effect was also verified in oocyte maturation in vitro. In pigs,
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adiponectin promoted nuclear maturation of treated oocytes [18]; however this effect
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was not observed in cattle [15,24].
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Regarding caprine species, no reports were found on the adiponectin system and
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its influence on female reproduction. Thus, the objective of this work was first to
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investigate mRNA and protein expression of the adiponectin system (adiponectin,
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AdipoR1 and AdipoR2) in goat ovary and second to study the effects of recombinant
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adiponectin on goat oocyte maturation in vitro.
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2. Materials and methods
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2.1.Tissue collection
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Antral follicles were dissected from the ovaries of adult goats (Capra hircus),
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collected independently of the stage of estrous cycle, obtained from a commercial
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slaughterhouse and transported to the laboratory in saline solution on ice. Isolated
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follicles were classified based on the diameter as small (<3 mm) and large (≥ 3 mm)
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antral follicles.
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Follicles were pooled (10-15 follicles/category) separately into petri dishes in
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phosphate-buffered saline (PBS) and then sectioned under a stereomicroscope (Nikon
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Corporation, Tokyo, Japan). Granulosa cells (GCs) adhering to follicle wall were
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removed by gentle scraping with a scalpel blade. After removal of all cumulus-oocyte
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complexes (COCs) from the petri dish, GCs were recovered by centrifugation at 1200 g
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for 1 min. Then, the theca cell layers (TC) were vortexed for 1 min in 1 ml PBS, 4
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transferred to 1 ml of fresh buffer and centrifuged for 1 min. The GC and TC pellets
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were homogenized in 0.5 ml of TRI® Reagent (Invitrogen, Thermo Fisher Scientific,
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Inc., Carlsbad, CA, USA) and stored at - 80°C until RNA extraction. Cumulus-oocyte complexes were aspirated from small and large antral follicles.
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Cumulus cells were mechanically separated by careful and repeated pipetting until no
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adherent cumulus cells could be observed under the stereomicroscope. Pools of 10-15
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denuded oocytes and cumulus cells of 10-15 COCs, of each category of follicle, were
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collected and immediately subjected to total RNA extraction using TRI® reagent. Six
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samples of each tissue pool were analyzed.
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Cross-contamination of granulosa and theca cells was tested by detection of
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mRNA encoding the cytochrome P450 aromatase (CYP19A1) and 17α-hydroxylase
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(CYP17A1) in each sample by PCR as described by Batista et al. [25]. The presence of
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CYP19A1 amplicons in theca samples or CYP17A1 in granulosa samples indicated
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cross-contamination, and such samples were discarded.
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2.2.Total RNA extraction and cDNA synthesis
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Total RNA was extracted from each cell pool (oocytes, cumulus cells, GCs and
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TCs) using TRI® reagent. Samples were homogenized in 500 µl of TRI® reagent and
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extracted with 100 µl chloroform; after separation of the aqueous phase, RNA was
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precipitated with isopropanol and washed in 70% (v/v) ethanol, and the RNA pellet was
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eluted in MilliQ water. Then, to eliminate possible DNA contamination, all total RNA
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samples were treated with RNase-free DNase (RQ1, Promega, Madison, USA)
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according to the manufacturer's recommended protocol. Total RNA was quantified by
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measuring the absorbance at 260 nm, and RNA purity was determined by the 260/280
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nm absorbance ratio using a NanoVue spectrophotometer (GE Healthcare Life
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Sciences Chicago, Illinois, United States). For complementary DNA (cDNA), 1 µg of total RNA was mixed with 0.5 µg
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random hexamers (Promega, Madison, WI, USA) and 0.5 µg oligo-d(T) primer
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(Promega, Madison, WI, USA). The mixture was then subjected to denaturation at 70°C
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for 5 min and immediately chilled in ice water for 5 min. Subsequently, 13 µL of cDNA
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master mix consisting of 1 µL reverse transcriptase (GoScript™; Promega), 4 µL 5×
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reaction buffer (GoScript™; Promega), 4 µL MgCl2 (25 mM; Promega), 1 µL dNTP
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working stock (0.5mM; Promega), and 3 µL of nuclease-free water was added. The
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samples underwent annealing at 25°C for 5 min, extension at 42°C for 60 min and
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inactivation at 70°C for 15 min.
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2.3.Real-time PCR
Quantitative real-time polymerase chain reaction (qPCR) was performed using a
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Rotor-Gene Q Real-Time PCR System (Qiagen, Hilden, Germany). Primers used were
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designed based on the published sequences for goat adiponectin (GenBank:
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KF452236.1),
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JX573540.1).
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dehydrogenase (GAPDH) and ubiquitin (UBQ) have been previously described [26].
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Primers sequences are shown in Table 1.
(GenBank:
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AdipoR1
Primers
for
the
HQ846828.1)
reference
genes
and
AdipoR2
(GenBank:
glyceraldehyde-3-phosphate
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The qPCR assay was performed in a final reaction volume of 15 µL containing 2
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µL of the standardized sample at a 500 µg/mL concentration, 7.5 µL of qPCR Master
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Mix (GoTaq® qPCR Master Mix; Promega, Madison, USA), 0.5 µL of each forward
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and reverse primer and 4.5 µl nuclease free water. The protocol consisted of one
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activation phase (95°C for 2 min) and one unfolding phase (95°C for 15 sec) followed
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by 40 annealing/extension cycles (60°C for 60 sec). Samples were measured in duplicate with a negative control for each primer
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evaluated. Calculation of the relative expression level of adiponectin, AdipoR1 and
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AdipoR2 genes was conducted based on the comparative cycle threshold method
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(∆∆CT) [27] and normalized using the geometrical means of reference gene expression
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levels: GAPDH and UBQ. Expression of adiponectin, AdipoR1 and AdipoR2 genes was
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calculated by the equation 2−∆∆CT, where ∆CT value was determined by subtracting the
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corresponding geometrical means of reference genes (GAPDH and UBQ) CT value
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from the specific CT of the target. Calculation of ∆∆CT involved using the highest
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sample ∆CT value (i.e., the sample with the lowest target expression) as an arbitrary
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constant to subtract from all other ∆CT sample values.
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2.4.Immunohistochemistry
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Goat ovaries were collected from a commercial abattoir, bisected, and fixed in
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4% paraformaldehyde in PBS for 24 hours. Fixed tissues were subsequently dehydrated,
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diaphanized and included in paraffin. Serial sections (4 µm) were mounted on silanized
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slides (S4651; Sigma, St. Louis, USA), dried overnight at 37°C, deparaffinized in
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xylene and hydrated in decreasing concentrations of ethanol.
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Endogenous peroxidase activity was blocked by tissue incubation in a
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peroxidase blocking reagent (Dako, Carpinteria, USA) for 30 min. Antigen retrieval
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was performed by immersing the sections in citrate buffer (pH 6.0) in a microwave
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oven. Then, non-specific reactions were blocked with normal goat serum (1:10; Dako,
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Glostrup, Denmark) in PBS for 30 min. The rabbit polyclonal antibodies anti-
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adiponectin (N-20-R, sc-17044, Santa Cruz Biotechnology, Santa Cruz, CA, USA), 7
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99184; Santa Cruz Biotechnology) diluted 1:50 in blocking buffer were incubated with
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tissues overnight at 4°C. Antibodies used in this study are recommended for the
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detection of adiponectin and its receptors in most animal species, including rat, human,
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equine, swine, canine and bovine. Sections were then washed in PBS and incubated
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with a peroxidase-conjugated polymer (EnVision ™ + Dual Link System-HRP; Dako,
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Carpinteria, USA) in a humidified chamber at room temperature for 30 min.
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Immunostaining was revealed by incubation at room temperature with 3-3'-
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diaminobenzidine
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counterstained with hematoxylin, photographed and examined by a Leica DM 500 light
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microscope coupled with a Leica ICC50 HD camera and EZ LAS 4.3 software (Leica
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Microsystems Nussloch GmbH, Nussloch, Germany). In the negative controls, the
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primary antibody was omitted from the procedure or primary antibodies were
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preincubated with blocking peptide (sc-17044P, Santa Cruz Biotechnology, Santa Cruz,
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CA, USA) or adiponectin at a ratio of 1:100. No immunoreaction was observed in the
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control preparations.
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sections
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2.5.In vitro maturation (IVM)
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Adult goat ovaries were collected from commercial abattoir and transported to
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the laboratory at 38°C in PBS containing antibiotic/antimycotic solution (Ab/Am, 100
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U/mL penicillin, 100 µg/mL streptomycin and 0.25 µg/mL amphotericin B; Gibco, Life
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Technologies, Grand Island, NY, USA) within two hours of slaughter. COCs were
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obtained by aspiration of antral follicles between 2 and 8 mm in diameter with an 18G
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needle connected to a 10 mL syringe, which was previously filled with 3 mL of
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HEPES-buffered TCM199 and supplemented with Ab/Am solution. The samples were 8
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selected under a stereomicroscope (Nikon Corporation, Tokyo, Japan), and only those
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with at least one layer of compact cumulus cells and homogeneous cytoplasm were
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selected. COCs were washed three times in serum-free maturation medium (TCM-199-
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Bicarbonate, containing 2 mM L-glutamine, 0.3 mM sodium pyruvate and 50 µg/mL
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gentamycin) and randomly distributed on 35 mm petri dishes (Nunc, Roskilde,
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Denmark) containing 25-35 oocytes in 80 µL drops of serum-free maturation medium
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with or without adiponectin (0, 5 or 10 µg/mL) or 10% (v/v) fetal bovine serum (FBS)
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as a positive control, under mineral oil. These adiponectin concentrations were chosen
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based on plasma and follicular fluid levels reported in earlier studies in goats [28, 29],
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and bovine [24]. COCs were cultured for 27 h at 38.5° C in humidified atmosphere of
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5% CO2. Recombinant human adiponectin (rh) (full-length human adiponectin, RD
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172023100) derived from mammalian cells (HEK-293 cells) was purchased from
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BioVendor Laboratory Medicine (Heidelberg, Germany). This experiment was repeated
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seven times (n = 660 oocytes).
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After the maturation period, some oocytes were denuded of cumulus cells by
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careful and repeated pipetting in PBS-PVP. The denuded oocytes were incubated with
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10 µg/mL Hoechst 33342 in PBS-PVP for 30 min at room temperature, washed three
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times in PBS-PVP and mounted on slides with the mounting medium ProLong® Gold
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(Molecular Probes, Life Technologies, Eugene, OR, USA), covered by coverslips
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supported by paraffin columns and sealed with nail polish. Samples were observed
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using a Zeiss Axioplan fluorescence microscope (Carl Zeiss, Inc., Göttingen, Germany).
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Images were acquired using AxioVision software and an AxioCam MRm digital camera
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(Carl Zeiss, Inc., Göttingen, Germany). The oocytes were classified according to the
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nuclear configuration as germinal vesicle (GV; Fig. 1A), germinal vesicle breakdown
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(GVBD; Fig. 1B), metaphase I (MI; Fig. 1C) and metaphase II (MII; Fig. 1D).
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2.6.Statistical analyses
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Categorical data were analyzed using the GLIMMIX Procedure of SAS fitted to
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a binary distribution. However, due the outcome 0 or 100% some analyses were
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performed using Fisher’s exact test using the FREQ procedure of SAS. Data were tested
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for normality of residuals, and data with residuals not normally distributed were
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transformed before analysis. Quantitative PCR data were analyzed using the GLIMMIX
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procedure of SAS fitted to a Gaussian distribution with the fixed effects of cell type and
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follicle size and the random effect of the sample.
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The GLIMMIX procedure (ANOVA) of SAS was used with generalized linear
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model methodology. For the data analyses, a Gaussian distribution was used. The
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variables were analyzed using a mathematical model that included the effects of the
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treatment. The residual method was used to calculate the denominator degrees of
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freedom to approximate the F tests in the mixed models. The relative proportion of the
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oocytes in each nuclear stage of maturation was calculated with the following equation:
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Relative proportion = number of the oocytes in each stage/total of oocytes. The
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statistical comparisons were performed using means adjusted by the least squares mean
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method.
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Differences with P ≤ 0.05 were considered significant, and those with 0.05 < P ≤
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0.10 were considered tendencies. Results are presented as the mean ± standard error of
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the mean (SEM).
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3. Results
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3.1.Analysis of gene expression qPCR revealed adiponectin mRNA in cumulus cells from small follicles and in
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GCs and TCs of both follicular sizes but not in oocytes, regardless of size, or in the
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cumulus cells from large follicles (Figure 2A).
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Adiponectin mRNA levels in small antral follicles were significantly higher (P
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<0.05) in the cumulus cells compared to those in GCs and TCs, and mRNA levels did
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not differ between GCs and TCs. In large antral follicles, adiponectin mRNA levels
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were significantly higher (P <0.05) in granulosa than those in TCs (Figure 2A).
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AdipoR1 and AdipoR2 expression was detected in all evaluated cell types
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(oocytes, cumulus cells, GCs and TCs) of large and small antral follicles. AdipoR1 and
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AdipoR2 showed significant differences (P <0.05) between the cell types derived only
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from large antral follicles. AdipoR1 expression levels were significantly (P < 0.05)
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lower in TCs compared with those in cumulus and GCs but did not differ (P > 0.05)
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compared to oocyte levels (Figure 2B). AdipoR2 mRNA levels in TCs were
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significantly (P < 0.05) lower than those of other cell types (Figure 2C).
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3.2. Protein expression analysis
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Positive immunolocalisation for adiponectin, AdipoR1 and AdipoR2 were found
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in oocyte, cumulus cells and granulosa cells of the follicles at all stages of development
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(Fig. 3). Oocytes from preantral and antral follicles showed intense and uniform
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cytoplasmic staining for the adiponectin (Fig. 3A-C), AdipoR1 (Fig. 3E-G) and
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AdipoR2 (Fig. 3I, J and L) proteins. In addition, theca cells showed moderate
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immunostaining for all proteins (Fig. 3D, H and K). Control tissue samples showed no
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positive staining (Fig. 3X, Y and Z).
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3.3. Adiponectin effects on meiotic progression
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Figure 4 shows the effects of adiponectin on goat oocyte meiotic maturation.
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The proportion of GV or GVBD stage-blocked oocytes (Figure 4A-B) was significantly
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reduced (P <0.05) in the 5 or 10 µg/mL adiponectin-treated groups compared to that of
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the control group. Maturation in the presence of 5 µg/mL adiponectin resulted in higher
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rates of MI compared to those of the group without adiponectin (P <0.05; Figure 4C).
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Additionally, the proportion of oocytes that progressed to MII was significantly higher
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(P <0.05) in the 5 and 10 µg/mL adiponectin-treated groups (Figure 4D) than that in the
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control groups. Groups treated with adiponectin showed similar percentages of MII
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compared to the group cultured with FBS.
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4. Discussion
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This study demonstrated the presence of the adiponectin system in goat follicular
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cells. Although expression and immunolocalization of the adiponectin system has
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already been studied in other species, as well as in different cell types, the gene and
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protein expression of adiponectin and its receptors had not been studied in goats.
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Our results demonstrated that adiponectin was not expressed at detectable levels
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in oocytes of small and large goat antral follicles or cumulus cells from large antral
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follicles. These results differ from those reported by Maillard et al. [15] and Tabandeh
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et al. [30], who found adiponectin expression in oocytes and cumulus cells of bovine
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antral follicles, indicating that there may be species-specific differences in ovarian
294
expression of the adiponectin gene. The lack of adiponectin mRNA in oocytes and cumulus cells from large antral
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follicles is intriguing. However, mRNA samples from several pools of denuded oocytes
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and cumulus cells from large antral follicles were analyzed, and none generated
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amplicons after qPCR. Therefore, it is unlikely to be a methodological problem because
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the reference genes GAPDH and UBQ were easily amplified in these samples, and we
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detected AdipoR1 and AdipoR2 mRNAs in oocytes and cumulus cells.
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Quantitatively, relative adiponectin expression in cumulus cells was significantly
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higher than that in GCs and TCs from small follicles. In large follicles, relative
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expression in GCs was significantly higher compared with that in TCs. These data differ
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from what has been observed in chicken ovaries, in which the expression of adiponectin
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in TCs was 10-30-fold higher than that in GCs [16]. In addition, adiponectin expression
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was also low in GCs of mice [17]. However, Maillard et al. [15] observed good
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adiponectin expression in bovine GCs.
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Receptor expression analysis showed decreased expression of AdipoR1 and
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Adipo2 in TCs of large follicles compared with expression of receptors in GCs. These
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results differ from those found by Tabandeh et al. [30] in cattle, where AdipoR1 and
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AdipoR2 expression was higher in large follicle TCs than that in GCs. Our findings also
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differ from results observed in mice, in which receptor expression in GCs was lower
313
than in TCs [17]. However, similar results were observed in chickens, where AdipoR1
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expression was twice as high in GCs as that in TCs, and AdipoR2 expression was
315
similar in both cell types [16]. This discrepancy suggests a species-specific mode of
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action of the adiponectin system on follicular development.
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immunolocalized in oocytes, cumulus cells, GCs and TCs in ovarian follicles at all
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stages of development. These findings corroborate those obtained in bovines [15], mice
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[17] and humans [21] and further support the physiological relevance of this hormone
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on ovarian function.
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Adiponectin protein was detected in the oocytes by immunohistochemistry,
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although no mRNA was observed, indicating that adiponectin must be produced
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elsewhere and then transported to the oocyte. This is likely because adiponectin is a
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secreted protein, is found in follicular fluid [29], and binds to its receptors on granulosa,
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cumulus and oocyte cells; receptor-bound adiponectin has been shown to be internalized
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in several cell lines [31,32]. The detection of adiponectin appears to be specific because
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preincubation of the antibody with blocking peptide abolished staining.
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Oocyte meiotic maturation and acquisition of developmental competence is an
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essential physiological process for survival of the species. The presence of AdipoR1 and
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AdipoR2 mRNA and protein in both oocytes and cumulus cells suggests that both cell
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types are sensitive to adiponectin and that adiponectin may also affect oocyte
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maturation.
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In the present work, we demonstrated that adiponectin addition (5 or 10 µg/mL)
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during IVM affected goat oocyte meiotic maturation. However, conflicting results have
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been reported in the literature. In cattle, supplementation of IVM medium with
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adiponectin (5 or 10 µg/mL) did not affect bovine oocyte meiotic maturation [15,24]. In
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pigs, however, Chappaz et al. [18] reported that recombinant porcine adiponectin (30
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µg/mL) significantly decreased the proportion of immature oocytes, suggesting that
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adiponectin accelerated porcine oocyte meiotic maturation.
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probably dependent on the species studied or on the culture medium used. The
343
experiment described in the present study was performed with serum-free medium and
344
in the absence of any growth factor or hormone other than adiponectin. However, other
345
studies have usually added gonadotropins or growth factors to the culture media; these
346
additives could have influenced the action of adiponectin or affected its pathways,
347
resulting in different responses. Thus, possible interactions between these additives and
348
the possible pathways by which adiponectin affects oocyte maturation remain unclear
349
and require further investigation.
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In conclusion, this study detected the expression of adiponectin and its receptors,
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AdipoR1 and AdipoR2, in goat ovarian follicles. In addition, adiponectin was shown to
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enhance the progression of goat oocyte nuclear maturation in vitro. The present findings
353
provide evidence for paracrine/autocrine effects of the analyzed hormone. However,
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future studies are needed to elucidate the mechanisms underlying the effect of
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adiponectin on meiotic maturation and to understand the role of the adiponectin system
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in goat fertility.
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Declaration of interest
The authors declare that there is no conflict of interest that could be perceived as
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prejudicing the impartiality of the research reported.
Acknowledgements The authors thank FACEPE (Fundação de Amparo à Ciência e Tecnologia do Estado de Pernambuco) for financial support (APQ-1115-5.05/14).
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2005;26:439–51. doi:10.1210/er.2005-0005. [14] Yamauchi T, Kamon J, Ito Y, Tsuchida A, Yokomizo T, Kita S, et al. Cloning of adiponectin receptors that mediate antidiabetic metabolic effects. Nature
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[16] Chabrolle C, Tosca L, Crochet S, Tesseraud S, Dupont J. Expression of
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adiponectin and its receptors (AdipoR1 and AdipoR2) in chicken ovary: Potential
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role in ovarian steroidogenesis. Domest Anim Endocrinol 2007;33:480–7.
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doi:10.1016/j.domaniend.2006.08.002. [17] Chabrolle C, Tosca L, Dupont J. Regulation of adiponectin and its receptors in rat ovary by human chorionic gonadotrophin treatment and potential involvement
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of adiponectin in granulosa cell steroidogenesis. Reproduction 2007;133:719–31.
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[18] Chappaz E, Albornoz MS, Campos D, Che L, Palin MF, Murphy BD, et al.
Adiponectin enhances in vitro development of swine embryos. Domest Anim
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[19] Nishio SI, Gibert Y, Bernard L, Brunet F, Triqueneaux G, Laudet V. Adiponectin and adiponectin receptor genes are coexpressed during zebrafish embryogenesis
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and regulated by food deprivation. Dev Dyn 2008;237:1682–90.
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[20] Chabrolle C, Tosca L, Ramé C, Lecomte P, Royère D, Dupont J. Adiponectin increases insulin-like growth factor I-induced progesterone and estradiol
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secretion in human granulosa cells. Fertil Steril 2009;92:1988–96.
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Further evidence for a link between obesity and hyperandrogenism in polycystic
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ovary syndrome. PLoS One 2013;8:1–9. doi:10.1371/journal.pone.0080416.
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[22] Ortega HH, Rey F, Velazquez MML, Padmanabhan V. Developmental programming: effect of prenatal steroid excess on intraovarian components of
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insulin signaling pathway and related proteins in sheep. Biol Reprod
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2010;82:1065–75. doi:10.1095/biolreprod.109.082719.
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[23] Kiezun M, Smolinska N, Maleszka A, Dobrzyn K, Szeszko K, Kaminski T. Adiponectin expression in the porcine pituitary during the estrous cycle and its
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effect on LH and FSH secretion. Am J Physiol Endocrinol Metab
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2014;307:E1038-46. doi:10.1152/ajpendo.00299.2014.
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[24] Divar MR, Kafi M, Mohammadi A, Azari M. The In Vitro Effect of Adiponectin on Early Bovine Embryonic Development and Transcriptomic Markers of Oocyte
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Competence. J Fertil Vitr - IVF-Worldwide, Reprod Med Genet Stem Cell Biol
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2016;4:1–7. doi:10.4172/2375-4508.1000172.
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[25] Batista AM, Silva DMF, Rêgo MJBM, Silva FLM, Silva ECB, Beltrão EIC, et al.
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The expression and localization of leptin and its receptor in goat ovarian follicles.
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Anim Reprod Sci 2013;141:142–7. doi:10.1016/j.anireprosci.2013.08.007.
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[26] Frota IM a, Leitão CCF, Costa JJN, Brito IR, van den Hurk R, Silva JR V.
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Stability of housekeeping genes and expression of locally produced growth
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factors and hormone receptors in goat preantral follicles. Zygote 2011;19:71–83.
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doi:10.1017/S0967199410000080.
[27] Livak KJ, Schmittgen TD. Analysis of relative gene expression data using real-
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time quantitative PCR and. Methods 2001;25:402–8.
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doi:10.1006/meth.2001.1262.
[28] Guzel S, Yibar A, Belenli D, Cetin I, Tanriverdi M. The concentrations of
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adipokines in goat milk: relation to plasma levels, inflammatory status, milk
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quality and composition. J Vet Med Sci 2017;79:602-607. doi:10.1292/jvms.16-
460 461
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0061.
[29] Wang Z, Meng C, Ding X, Zhang G, Wang F. Effect of body condition on
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follicle transcriptome in estrous. Peerj Prepr 2016;4:1–34.
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doi:https://doi.org/10.7287/peerj.preprints.2177v1.
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[30] Tabandeh MR, Hosseini A, Saeb M, Kafi M, Saeb S. Changes in the gene expression of adiponectin and adiponectin receptors (AdipoR1 and AdipoR2) in
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ovarian follicular cells of dairy cow at different stages of development.
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Theriogenology 2010;73:659–69. doi:10.1016/j.theriogenology.2009.11.006.
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[31] Ding Q, Wang Z, Chen Y. Endocytosis of adiponectin receptor 1 through a clathrin- and Rab5-dependent pathway 2009;19:317–27.
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doi:10.1038/cr.2008.299.
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[32] Almabouada F, Diaz-ruiz A, Rabanal-ruiz Y, Peinado JR, Vazquez-martinez R,
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Malagon MM. Adiponectin Receptors Form Homomers and Heteromers
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Exhibiting Distinct Ligand Binding and Intracellular Signaling 2013;288:3112–
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25. doi:10.1074/jbc.M112.404624.
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Table Legend
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Table 1. Oligonucleotide primer sequences used to perform qPCR.
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Figure Legends
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Figure 1. Representative images of goat oocytes stained with Hoechst 33342 and
496
evaluated under fluorescence microscopy. Oocytes in germinal vesicle (GV, A),
497
germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
498
D) stages are shown.
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Figure 2. Adiponectin (A); AdipoR1 (B) and AdipoR2 (C) mRNA expression in oocyte
501
– O, cumulus cells – C, granulosa cells – G and theca cells – T isolated from small (< 3
502
mm) and large (≥ 3 mm) goat antral follicles. Different superscripts denote the statistical
503
significance between different cells types isolated from follicles in the same size
504
category (P < 0.05).
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Figure 3. Immunolocalization of adiponectin, AdipoR1 and AdipoR2 in goat ovaries.
507
Positive staining of adiponectin, AdipoR1 and AdipoR2 was observed in oocytes and
508
granulosa cells of primordial (A, E and I), primary (B and I) and secondary follicles (C,
509
F and J). Antral follicles with positive immunostaining of adiponectin, AdipoR1 and
510
AdipoR2 in oocytes, cumulus, theca and granulosa cells (D, G, H, K and L). No staining
511
was observed in the negative control (X, Y and Z). g, granulosa; t, theca, c, cumulus; o,
512
oocytes.
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Figure 4. Effects of recombinant adiponectin (0, 5 or 10 µg/mL) on the progression of
515
meiotic maturation of goat oocytes in vitro matured for 27 h. Germinal vesicle (GV, A),
21
ACCEPTED MANUSCRIPT 516
germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
517
D). The data are expressed as the mean ± SEM. Different superscripts denote the
518
statistical significance among experimental groups within the same stage of meiotic
519
maturation (P < 0.05).
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532 533 534 535 536
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Revised Highlighted
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Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary
542
and its effect on oocyte nuclear maturation in vitro
543
Bruna S. P. Oliveiraa, Joana A. S. Costaa, Elizabete T. Gomesa, Diogo M. F. Silvaa,
544
Sandra M. Torresa, Pedro L. J. Monteiro Jrb, Antônio S. Santos Filhoc, Maria Madalena
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P.Guerraa, Gustavo F. Carneirod, Aurea Wischrala, André M. Batistaa,*
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546 547
a
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Pernambuco, Brazil.
549
b
Department of Animal Science, University of São Paulo, Piracicaba, SP, Brazil.
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C
Agronomic Institute of Pernambuco, Arcoverde, PE, Brazil.
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d
UAG/University Federal Rural of Pernambuco, Garanhuns, PE, Brazil.
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Department of Veterinary Medicine, Federal Rural University of Pernambuco, Recife,
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* Corresponding author: Department of Veterinary Medicine, Rural Federal
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University of Pernambuco, Dom Manoel de Medeiros street, s/n, Dois Irmãos, CEP
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52171-900, Recife, Pernambuco, Brazil. Tel.: +55 81 3320 6414; fax: +55 81 3320
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6057. E-mail address: [email protected]
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ACCEPTED MANUSCRIPT ABSTRACT
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Adiponectin is an adipokine secreted primarily by adipocytes and is involved in the
568
control of male and female reproductive functions. Circulating levels of adiponectin are
569
inversely correlated with body fat mass, and its biological effects are predominantly
570
mediated through two receptors, AdipoR1 and AdipoR2. The aim of the present study
571
was to verify the expression of the adiponectin system (adiponectin and its receptors,
572
AdipoR1 and AdipoR2) in goat ovary using qPCR and immunohistochemistry analyses
573
and further investigate the in vitro effects of recombinant adiponectin (5 µg/mL and 10
574
µg/mL) on goat oocyte nuclear maturation. We demonstrated that the mRNA and
575
proteins of the adiponectin system are present in goat ovary. Gene and protein
576
expression of AdipoR1 and AdipoR2 was detected in follicular cells (oocyte, cumulus,
577
granulosa and theca) of small and large antral follicles, while adiponectin mRNA was
578
not detected in oocytes from small and large follicles or in large follicle cumulus cells.
579
Finally, addition of various concentrations of adiponectin in maturation medium
580
affected the number of oocytes that reached metaphase II. In conclusion, in the present
581
study, we detected expression of adiponectin and its receptors AdipoR1 and AdipoR2 in
582
goat ovarian follicles. Furthermore, we demonstrated that recombinant adiponectin
583
increases nuclear maturation of goat oocytes in vitro.
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Keywords: follicle, ovary, goat, adipose tissue, gene expression
5. Introduction
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Increased livestock productivity has become a major research topic in response
589
to increases in the population and consumption [1]. In this context, understanding the
590
reproductive physiology of these animals is key to improving reproductive techniques 24
ACCEPTED MANUSCRIPT 591
and, consequently, increasing productivity. In ruminants, reproductive function can be
592
influenced at different levels of the hypothalamic-pituitary-gonadal axis by energetic
593
alterations related to diet [2], with a well-known relationship between energetic balance
594
and reproduction [3]. Adipose tissue, once recognized only for its role as an energy reservoir, has been
596
identified as an important modulator of this relationship [4,5]. Now recognized as an
597
endocrine organ, adipose tissue releases a wide variety of protein factors called
598
adipokines [6]. These adipokines have important effects on various physiological
599
processes, including reproduction [7]. Adiponectin, a 30 kDa, 244 amino acid protein,
600
has an N-terminal signal sequence, a species-dependent variable sequence, a collagen
601
domain, and a C-terminal globular domain [8,9]. Its secretion is inversely related to
602
adipose tissue levels [10], and its circulating levels are two to three times higher in
603
females than those in males [11].
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Adiponectin acts through two specific membrane receptors, AdipoR1 and
605
AdipoR2 [12]. These receptors are formed by seven transmembrane domains, with an
606
intracellular N-terminus and an extracellular C-terminus, and have an opposite
607
orientation to that of classical G-proteins-coupled receptors [13,14]. The adiponectin
608
system was identified in different organs of the female reproductive system in various
609
species. Adiponectin, AdipoR1 and AdipoR2 were observed in ovarian cells of cattle
610
[15], chickens [16], mice [17] and swine [18]. AdipoR1 and AdipoR2 were also
611
identified in ovarian fish cells [19] and humans [20,21]. Adiponectin protein was also
612
visualized in ovine follicular cells [22].
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The literature suggests that adiponectin has a steroidogenic effect on ovarian
614
function. In pigs, in vitro studies have shown that adiponectin reduced basal
615
testosterone secretion in internal theca cells; in granulosa cells, it increased secretion of
25
ACCEPTED MANUSCRIPT estradiol and, in combination with insulin, increased secretion of progesterone [23]. In
617
human primary granulosa cells, adiponectin increased IGF-1-induced secretion of
618
progesterone and estradiol [20]. In chickens, adiponectin was also shown to modify the
619
progesterone secretion pattern induced by LH, FSH or IGF-1 in granulosa cells [16].
620
This adipokine effect was also verified in oocyte maturation in vitro. In pigs,
621
adiponectin promoted nuclear maturation of treated oocytes [18]; however this effect
622
was not observed in cattle [15,24].
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Regarding caprine species, no reports were found on the adiponectin system and
624
its influence on female reproduction. Thus, the objective of this work was first to
625
investigate mRNA and protein expression of the adiponectin system (adiponectin,
626
AdipoR1 and AdipoR2) in goat ovary and second to study the effects of recombinant
627
adiponectin on goat oocyte maturation in vitro.
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6. Materials and methods
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6.1.Tissue collection
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Antral follicles were dissected from the ovaries of adult goats (Capra hircus),
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collected independently of the stage of estrous cycle, obtained from a commercial
633
slaughterhouse and transported to the laboratory in saline solution on ice. Isolated
634
follicles were classified based on the diameter as small (<3 mm) and large (≥ 3 mm)
635
antral follicles.
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Follicles were pooled (10-15 follicles/category) separately into petri dishes in
637
phosphate-buffered saline (PBS) and then sectioned under a stereomicroscope (Nikon
638
Corporation, Tokyo, Japan). Granulosa cells (GCs) adhering to follicle wall were
639
removed by gentle scraping with a scalpel blade. After removal of all cumulus-oocyte
640
complexes (COCs) from the petri dish, GCs were recovered by centrifugation at 1200 g 26
ACCEPTED MANUSCRIPT 641
for 1 min. Then, the theca cell layers (TC) were vortexed for 1 min in 1 ml PBS,
642
transferred to 1 ml of fresh buffer and centrifuged for 1 min. The TC and GC pellets
643
were homogenized in 0.5 ml of TRI® Reagent (Invitrogen, Thermo Fisher Scientific,
644
Inc., Carlsbad, CA, USA) and stored at - 80°C until RNA extraction. Cumulus-oocyte complexes were aspirated from small and large antral follicles.
646
Cumulus cells were mechanically separated by careful and repeated pipetting until no
647
adherent cumulus cells could be observed under the stereomicroscope. Pools of 10-15
648
denuded oocytes and cumulus cells of 10-15 COCs, of each category of follicle, were
649
collected and immediately subjected to total RNA extraction using TRI® reagent. Six
650
samples of each tissue pool were analyzed.
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Cross-contamination of granulosa and theca cells was tested by detection of
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mRNA encoding the cytochrome P450 aromatase (CYP19A1) and 17α-hydroxylase
653
(CYP17A1) in each sample by PCR as described by Batista et al. [25]. The presence of
654
CYP19A1 amplicons in theca samples or CYP17A1 in granulosa samples indicated
655
cross-contamination, and such samples were discarded.
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6.2.Total RNA extraction and cDNA synthesis Total RNA was extracted from each cell pool (oocytes, cumulus cells, TCs and
659
GCs) using TRI® reagent. Samples were homogenized in 500 µl of TRI® reagent and
660
extracted with 100 µl chloroform; after separation of the aqueous phase, RNA was
661
precipitated with isopropanol and washed in 70% (v/v) ethanol, and the RNA pellet was
662
eluted in MilliQ water. Then, to eliminate possible DNA contamination, all total RNA
663
samples were treated with RNase-free DNase (RQ1, Promega, Madison, USA)
664
according to the manufacturer's recommended protocol. Total RNA was quantified by
665
measuring the absorbance at 260 nm, and RNA purity was determined by the 260/280
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nm absorbance ratio using a NanoVue spectrophotometer (GE Healthcare Life
667
Sciences Chicago, Illinois, United States). For complementary DNA (cDNA), 1 µg of total RNA was mixed with 0.5 µg
669
random hexamers (Promega, Madison, WI, USA) and 0.5 µg oligo-d(T) primer
670
(Promega, Madison, WI, USA). The mixture was then subjected to denaturation at 70°C
671
for 5 min and immediately chilled in ice water for 5 min. Subsequently, 13 µL of cDNA
672
master mix consisting of 1 µL reverse transcriptase (GoScript™; Promega), 4 µL 5×
673
reaction buffer (GoScript™; Promega), 4 µL MgCl2 (25 mM; Promega), 1 µL dNTP
674
working stock (0.5mM; Promega), and 3 µL of nuclease-free water was added. The
675
samples underwent annealing at 25°C for 5 min, extension at 42°C for 60 min and
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inactivation at 70°C for 15 min.
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6.3.Real-time PCR
Quantitative real-time polymerase chain reaction (qPCR) was performed using a
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Rotor-Gene Q Real-Time PCR System (Qiagen, Hilden, Germany). Primers used were
681
designed based on the published sequences for goat adiponectin (GenBank:
682
KF452236.1),
683
JX573540.1).
684
dehydrogenase (GAPDH) and ubiquitin (UBQ) have been previously described [26].
685
Primers sequences are shown in Table 1.
(GenBank:
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AdipoR1
Primers
for
the
HQ846828.1)
reference
genes
and
AdipoR2
(GenBank:
glyceraldehyde-3-phosphate
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The qPCR assay was performed in a final reaction volume of 15 µL containing 2
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µL of the standardized sample at a 500 µg/mL concentration, 7.5 µL of qPCR Master
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Mix (GoTaq® qPCR Master Mix; Promega, Madison, USA), 0.5 µL of each forward
689
and reverse primer and 4.5 µl nuclease free water. The protocol consisted of one
28
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activation phase (95°C for 2 min) and one unfolding phase (95°C for 15 sec) followed
691
by 40 annealing/extension cycles (60°C for 60 sec). Samples were measured in duplicate with a negative control for each primer
693
evaluated. Calculation of the relative expression level of adiponectin, AdipoR1 and
694
AdipoR2 genes was conducted based on the comparative cycle threshold method
695
(∆∆CT) [27] and normalized using the geometrical means of reference gene expression
696
levels: GAPDH and UBQ. Expression of adiponectin, AdipoR1 and AdipoR2 genes was
697
calculated by the equation 2−∆∆CT, where ∆CT value was determined by subtracting the
698
corresponding geometrical means of reference genes (GAPDH and UBQ) CT value
699
from the specific CT of the target. Calculation of ∆∆CT involved using the highest
700
sample ∆CT value (i.e., the sample with the lowest target expression) as an arbitrary
701
constant to subtract from all other ∆CT sample values.
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6.4. Immunohistochemistry
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Goat ovaries were collected from a commercial abattoir, bisected, and fixed in
705
4% paraformaldehyde in PBS for 24 hours. Fixed tissues were subsequently dehydrated,
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diaphanized and included in paraffin. Serial sections (4 µm) were mounted on silanized
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slides (S4651; Sigma, St. Louis, USA), dried overnight at 37°C, deparaffinized in
708
xylene and hydrated in decreasing concentrations of ethanol.
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Endogenous peroxidase activity was blocked by tissue incubation in a
710
peroxidase blocking reagent (Dako, Carpinteria, USA) for 30 min. Antigen retrieval
711
was performed by immersing the sections in citrate buffer (pH 6.0) in a microwave
712
oven. Then, non-specific reactions were blocked with normal goat serum (1:10; Dako,
713
Glostrup, Denmark) in PBS for 30 min. The rabbit polyclonal antibodies anti-
714
adiponectin (N-20-R, sc-17044, Santa Cruz Biotechnology, Santa Cruz, CA, USA), 29
ACCEPTED MANUSCRIPT anti-AdipoR1 (H-40, sc-99183, Santa Cruz Biotechnology) or anti-AdipoR2 (M -44, sc-
716
99184; Santa Cruz Biotechnology) diluted 1:50 in blocking buffer were incubated with
717
tissues overnight at 4°C. Antibodies used in this study are recommended for the
718
detection of adiponectin and its receptors in most animal species, including rat, human,
719
equine, swine, canine and bovine. Sections were then washed in PBS and incubated
720
with a peroxidase-conjugated polymer (EnVision ™ + Dual Link System-HRP; Dako,
721
Carpinteria, USA) in a humidified chamber at room temperature for 30 min.
722
Immunostaining was revealed by incubation at room temperature with 3-3'-
723
diaminobenzidine
724
counterstained with hematoxylin, photographed and examined by a Leica DM 500 light
725
microscope coupled with a Leica ICC50 HD camera and EZ LAS 4.3 software (Leica
726
Microsystems Nussloch GmbH, Nussloch, Germany). In the negative controls, the
727
primary antibody was omitted from the procedure or primary antibodies were
728
preincubated with blocking peptide (sc-17044P, Santa Cruz Biotechnology, Santa Cruz,
729
CA, USA) or adiponectin at a ratio of 1:100. No immunoreaction was observed in the
730
control preparations.
733
SC
Carpinteria,
USA).
Finally,
sections
were
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Dako,
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(DAB,
6.5.In vitro maturation (IVM)
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731
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715
Adult goat ovaries were collected from commercial abattoir and transported to
734
the laboratory at 38°C in PBS containing antibiotic/antimycotic solution (Ab/Am, 100
735
U/mL penicillin, 100 µg/mL streptomycin and 0.25 µg/mL amphotericin B; Gibco, Life
736
Technologies, Grand Island, NY, USA) within two hours of slaughter. COCs were
737
obtained by aspiration of antral follicles between 2 and 8 mm in diameter with an 18G
738
needle connected to a 10 mL syringe, which was previously filled with 3 mL of
739
HEPES-buffered TCM199 and supplemented with Ab/Am solution. The samples were 30
ACCEPTED MANUSCRIPT 740
selected under a stereomicroscope (Nikon Corporation, Tokyo, Japan), and only those
741
with at least one layer of compact cumulus cells and homogeneous cytoplasm were
742
selected. COCs were washed three times in serum-free maturation medium (TCM-199-
744
Bicarbonate, containing 2 mM L-glutamine, 0.3 mM sodium pyruvate and 50 µg/mL
745
gentamycin) and randomly distributed on 35 mm petri dishes (Nunc, Roskilde,
746
Denmark) containing 25-35 oocytes in 80 µL drops of serum-free maturation medium
747
with or without adiponectin (0, 5 or 10 µg/mL) or 10% (v/v) fetal bovine serum (FBS)
748
as a positive control, under mineral oil. These concentrations were chosen based on
749
plasma and follicular fluid levels reported in earlier studies in goats [28, 29], and bovine
750
[24]. COCs were cultured for 27 h at 38.5° C in humidified atmosphere of 5% CO2.
751
Recombinant human adiponectin (rh) (full-length human adiponectin, RD 172023100)
752
derived from mammalian cells (HEK-293 cells) was purchased from BioVendor
753
Laboratory Medicine (Heidelberg, Germany). This experiment was repeated seven
754
times (n = 660 oocytes).
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After the maturation period, some oocytes were denuded of cumulus cells by
756
careful and repeated pipetting in PBS-PVP. The denuded oocytes were incubated with
757
10 µg/mL Hoechst 33342 in PBS-PVP for 30 min at room temperature, washed three
758
times in PBS-PVP and mounted on slides with the mounting medium ProLong® Gold
759
(Molecular Probes, Life Technologies, Eugene, OR, USA), covered by coverslips
760
supported by paraffin columns and sealed with nail polish. Samples were observed
761
using a Zeiss Axioplan fluorescence microscope (Carl Zeiss, Inc., Göttingen, Germany).
762
Images were acquired using AxioVision software and an AxioCam MRm digital camera
763
(Carl Zeiss, Inc., Göttingen, Germany). The oocytes were classified according to the
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ACCEPTED MANUSCRIPT 764
nuclear configuration as germinal vesicle (GV; Fig. 1A), germinal vesicle breakdown
765
(GVBD; Fig. 1B), metaphase I (MI; Fig. 1C) and metaphase II (MII; Fig. 1D).
766
6.6.Statistical analyses
RI PT
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Categorical data were analyzed using the GLIMMIX Procedure of SAS fitted to
769
a binary distribution. However, due the outcome 0 or 100% some analyses were
770
performed using Fisher’s exact test using the FREQ procedure of SAS. Data were tested
771
for normality of residuals, and data with residuals not normally distributed were
772
transformed before analysis. Quantitative PCR data were analyzed using the GLIMMIX
773
procedure of SAS fitted to a Gaussian distribution with the fixed effects of cell type and
774
follicle size and the random effect of the sample.
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The GLIMMIX procedure (ANOVA) of SAS was used with generalized linear
776
model methodology. For the data analyses, a Gaussian distribution was used. The
777
variables were analyzed using a mathematical model that included the effects of the
778
treatment. The residual method was used to calculate the denominator degrees of
779
freedom to approximate the F tests in the mixed models. The relative proportion of the
780
oocytes in each nuclear stage of maturation was calculated with the following equation:
781
Relative proportion = number of the oocytes in each stage/total of oocytes. The
782
statistical comparisons were performed using means adjusted by the least squares mean
783
method.
EP
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Differences with P ≤ 0.05 were considered significant, and those with 0.05 < P ≤
785
0.10 were considered tendencies. Results are presented as the mean ± standard error of
786
the mean (SEM).
787
32
ACCEPTED MANUSCRIPT 788
7. Results
789
7.1.Analysis of gene expression qPCR revealed adiponectin mRNA in cumulus cells from small follicles and in
791
GCs and TCs of both follicular sizes but not in oocytes, regardless of size, or in the
792
cumulus cells from large follicles (Figure 2A).
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Adiponectin mRNA levels in small antral follicles were significantly higher (P
794
<0.05) in the cumulus cells compared to those in GCs and TCs, and mRNA levels did
795
not differ between GCs and TCs. In large antral follicles, adiponectin mRNA levels
796
were significantly higher (P <0.05) in granulosa than those in TCs (Figure 2A).
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AdipoR1 and AdipoR2 expression was detected in all evaluated cell types
798
(oocytes, cumulus cells, GCs and TCs) of large and small antral follicles. AdipoR1 and
799
AdipoR2 showed significant differences (P <0.05) between the cell types derived only
800
from large antral follicles. AdipoR1 expression levels were significantly (P < 0.05)
801
lower in TCs compared with those in cumulus and GCs but did not differ (P > 0.05)
802
compared to oocyte levels (Figure 2B). AdipoR2 mRNA levels in TCs were
803
significantly (P < 0.05) lower than those of other cell types (Figure 2C).
806
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7.2. Protein expression analysis
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Positive immunolocalisation for adiponectin, AdipoR1 and AdipoR2 were found
807
in oocyte, cumulus cells and granulosa cells of the follicles at all stages of development
808
(Fig. 3). Oocytes from preantral and antral follicles showed intense and uniform
809
cytoplasmic staining for the adiponectin (Fig. 3A-C), AdipoR1 (Fig. 3E-G) and
810
AdipoR2 (Fig. 3I, J and L) proteins. In addition, theca cells showed moderate
33
ACCEPTED MANUSCRIPT 811
immunostaining for all proteins (Fig. 3D, H and K). Control tissue samples showed no
812
positive staining (Fig. 3X, Y and Z).
813
7.3.Adiponectin effects on meiotic progression
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Figure 4 shows the effects of adiponectin on goat oocyte meiotic maturation.
816
The proportion of GV or GVBD stage-blocked oocytes (Figure 4A-B) was significantly
817
reduced (P <0.05) in the 5 or 10 µg/mL adiponectin-treated groups compared to that of
818
the control group. Maturation in the presence of 5 µg/mL adiponectin resulted in higher
819
rates of MI compared to those of the group without adiponectin (P <0.05; Figure 4C).
820
Additionally, the proportion of oocytes that progressed to MII was significantly higher
821
(P <0.05) in the 5 and 10 µg/mL adiponectin-treated groups (Figure 4D) than that in the
822
control groups. Groups treated with adiponectin showed similar percentages of MII
823
compared to the group cultured with FBS.
824
825
8. Discussion
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815
This study demonstrated the presence of the adiponectin system in goat follicular
827
cells. Although expression and immunolocalization of the adiponectin system has
828
already been studied in other species, as well as in different cell types, the gene and
829
protein expression of adiponectin and its receptors had not been studied in goats.
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Our results demonstrated that adiponectin was not expressed at detectable levels
831
in oocytes of small and large goat antral follicles or cumulus cells from large antral
832
follicles. These results differ from those reported by Maillard et al. [15] and Tabandeh
833
et al. [30], who found adiponectin expression in oocytes and cumulus cells of bovine
34
ACCEPTED MANUSCRIPT 834
antral follicles, indicating that there may be species-specific differences in ovarian
835
expression of the adiponectin gene. The lack of adiponectin mRNA in oocytes and cumulus cells from large antral
837
follicles is intriguing. However, mRNA samples from several pools of denuded oocytes
838
and cumulus cells from large antral follicles were analyzed, and none generated
839
amplicons after qPCR. Therefore, it is unlikely to be a methodological problem because
840
the reference genes GAPDH and UBQ were easily amplified in these samples, and we
841
detected AdipoR1 and AdipoR2 mRNAs in oocytes and cumulus cells.
SC
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836
Quantitatively, relative adiponectin expression in cumulus cells was significantly
843
higher than that in GCs and TCs from small follicles. In large follicles, relative
844
expression in GCs was significantly higher compared with that in TCs. These data differ
845
from what has been observed in chicken ovaries, in which the expression of adiponectin
846
in TCs was 10-30-fold higher than that in GCs [16]. In addition, adiponectin expression
847
was also low in GCs of mice [17]. However, Maillard et al. [15] observed good
848
adiponectin expression in bovine GCs.
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Receptor expression analysis showed decreased expression of AdipoR1 and
850
Adipo2 in TCs of large follicles compared with expression of receptors in GCs. These
851
results differ from those found by Tabandeh et al. [30] in cattle, where AdipoR1 and
852
AdipoR2 expression was higher in large follicle TCs than that in GCs. Our findings also
853
differ from results observed in mice, in which receptor expression in GCs was lower
854
than in TCs [17]. However, similar results were observed in chickens, where AdipoR1
855
expression was twice as high in GCs as that in TCs, and AdipoR2 expression was
856
similar in both cell types [16]. This discrepancy suggests a species-specific mode of
857
action of the adiponectin system on follicular development.
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35
ACCEPTED MANUSCRIPT In the present study, adiponectin and its receptors AdipoR1 and AdipoR2 were
859
immunolocalized in oocytes, cumulus cells, GCs and TCs in ovarian follicles at all
860
stages of development. These findings corroborate those obtained in bovines [15], mice
861
[17] and humans [21] and further support the physiological relevance of this hormone
862
on ovarian function.
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Adiponectin protein was detected in the oocytes by immunohistochemistry,
864
although no mRNA was observed, indicating that adiponectin must be produced
865
elsewhere and then transported to the oocyte. This is likely because adiponectin is a
866
secreted protein, is found in follicular fluid [29], and binds to its receptors on granulosa,
867
cumulus and oocyte cells; receptor-bound adiponectin has been shown to be internalized
868
in several cell lines [31,32]. The detection of adiponectin appears to be specific because
869
preincubation of the antibody with blocking peptide abolished staining.
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863
Oocyte meiotic maturation and acquisition of developmental competence is an
871
essential physiological process for survival of the species. The presence of AdipoR1 and
872
AdipoR2 mRNA and protein in both oocytes and cumulus cells suggests that both cell
873
types are sensitive to adiponectin and that adiponectin may also affect oocyte
874
maturation.
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In the present work, we demonstrated that adiponectin addition (5 or 10 µg/mL)
876
during IVM affected goat oocyte meiotic maturation. However, conflicting results have
877
been reported in the literature. In cattle, supplementation of IVM medium with
878
adiponectin (5 or 10 µg/mL) did not affect bovine oocyte meiotic maturation [15,24]. In
879
pigs, however, Chappaz et al. [18] reported that recombinant porcine adiponectin (30
880
µg/mL) significantly decreased the proportion of immature oocytes, suggesting that
881
adiponectin accelerated porcine oocyte meiotic maturation.
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36
ACCEPTED MANUSCRIPT These apparently controversial IVM results reported in the literature are
883
probably dependent on the species studied or on the culture medium used. The
884
experiment described in the present study was performed with serum-free medium and
885
in the absence of any growth factor or hormone other than adiponectin. However, other
886
studies have usually added gonadotropins or growth factors to the culture media; these
887
additives could have influenced the action of adiponectin or affected its pathways,
888
resulting in different responses. Thus, possible interactions between these additives and
889
the possible pathways by which adiponectin affects oocyte maturation remain unclear
890
and require further investigation.
SC
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In conclusion, this study detected the expression of adiponectin and its receptors,
892
AdipoR1 and AdipoR2, in goat ovarian follicles. In addition, adiponectin was shown to
893
enhance the progression of goat oocyte nuclear maturation in vitro. The present findings
894
provide evidence for paracrine/autocrine effects of the analyzed hormone. However,
895
future studies are needed to elucidate the mechanisms underlying the effect of
896
adiponectin on meiotic maturation and to understand the role of the adiponectin system
897
in goat fertility.
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900 901 902 903 904 905
Declaration of interest
The authors declare that there is no conflict of interest that could be perceived as
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prejudicing the impartiality of the research reported.
Acknowledgements The authors thank FACEPE (Fundação de Amparo à Ciência e Tecnologia do Estado de Pernambuco) for financial support (APQ-1115-5.05/14).
906
37
ACCEPTED MANUSCRIPT 907
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2005;26:439–51. doi:10.1210/er.2005-0005. [14] Yamauchi T, Kamon J, Ito Y, Tsuchida A, Yokomizo T, Kita S, et al. Cloning of adiponectin receptors that mediate antidiabetic metabolic effects. Nature
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[19] Nishio SI, Gibert Y, Bernard L, Brunet F, Triqueneaux G, Laudet V. Adiponectin and adiponectin receptor genes are coexpressed during zebrafish embryogenesis
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The expression and localization of leptin and its receptor in goat ovarian follicles.
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Anim Reprod Sci 2013;141:142–7. doi:10.1016/j.anireprosci.2013.08.007.
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[26] Frota IM a, Leitão CCF, Costa JJN, Brito IR, van den Hurk R, Silva JR V.
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Stability of housekeeping genes and expression of locally produced growth
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factors and hormone receptors in goat preantral follicles. Zygote 2011;19:71–83.
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[30] Tabandeh MR, Hosseini A, Saeb M, Kafi M, Saeb S. Changes in the gene expression of adiponectin and adiponectin receptors (AdipoR1 and AdipoR2) in
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ovarian follicular cells of dairy cow at different stages of development.
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Theriogenology 2010;73:659–69. doi:10.1016/j.theriogenology.2009.11.006.
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[31] Ding Q, Wang Z, Chen Y. Endocytosis of adiponectin receptor 1 through a clathrin- and Rab5-dependent pathway 2009;19:317–27.
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[32] Almabouada F, Diaz-ruiz A, Rabanal-ruiz Y, Peinado JR, Vazquez-martinez R,
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Malagon MM. Adiponectin Receptors Form Homomers and Heteromers
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Exhibiting Distinct Ligand Binding and Intracellular Signaling 2013;288:3112–
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25. doi:10.1074/jbc.M112.404624.
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1024 1025 1026 1027
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ACCEPTED MANUSCRIPT 1032
Table Legend
1033
Table 1. Oligonucleotide primer sequences used to perform qPCR.
1034
Figure Legends
1036
Figure 1. Representative images of goat oocytes stained with Hoechst 33342 and
1037
evaluated under fluorescence microscopy. Oocytes in germinal vesicle (GV, A),
1038
germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
1039
D) stages are shown.
SC
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1035
1040
Figure 2. Adiponectin (A); AdipoR1 (B) and AdipoR2 (C) mRNA expression in oocyte
1042
– O, cumulus cells – C, granulosa cells – G and theca cells – T isolated from small (< 3
1043
mm) and large (≥ 3 mm) goat antral follicles. Different superscripts denote the statistical
1044
significance between different cells types isolated from follicles in the same size
1045
category (P < 0.05).
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1046
Figure 3. Immunolocalization of adiponectin, AdipoR1 and AdipoR2 in goat ovaries.
1048
Positive staining of adiponectin, AdipoR1 and AdipoR2 was observed in oocytes and
1049
granulosa cells of primordial (A, E and I), primary (B and I) and secondary follicles (C,
1050
F and J). Antral follicles with positive immunostaining of adiponectin, AdipoR1 and
1051
AdipoR2 in oocytes, cumulus, theca and granulosa cells (D, G, H, K and L). No staining
1052
was observed in the negative control (X, Y and Z). g, granulosa; t, theca, c, cumulus; o,
1053
oocytes.
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1054 1055
Figure 4. Effects of recombinant adiponectin (0, 5 or 10 µg/mL) on the progression of
1056
meiotic maturation of goat oocytes in vitro matured for 27 h. Germinal vesicle (GV, A),
43
ACCEPTED MANUSCRIPT germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
1058
D). The data are expressed as the mean ± SEM. Different superscripts denote the
1059
statistical significance among experimental groups within the same stage of meiotic
1060
maturation (P < 0.05).
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21
ACCEPTED MANUSCRIPT 1
Table 1. Oligonucleotide primer sequences used to perform qPCR.
2 Gene
Primer sequences (5'-3')
GAPDH
Ubiquitin
CYP17A1
Forward
5'-GAAGGTGGTGTTCGGGATGT-3'
Reverse
5'-CAGTGTGGAAGAGCCAGGAG-3'
Forward
5'-GCTCTCAGGCTCAGGAAAGG-3'
Reverse
5'-AAGCCAGACGCCTCTACAAG-3'
Forward
5'- TGTTTGTGATGGGCGTGAACCA-3'
Reverse
5'-ATGGCGTGGACAGTGGTCATAA-3'
Forward
5'-GAAGATGGCCGCACTCTTCTGAT-3'
Reverse
5’-ATCCTGGATCTTGGCCTTCACGTT-3'
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5'-CCGCATAGACCCCATTGTGA-3'
Forward
5'-ACTGAATGCCTTTGCCCTGT-3'
Reverse
5'-CTGATTATGTTGGTGACCGCC-3'
Forward
5'-CATCCTCAATACCAGGTCCCA-3'
Reverse
5'-GGTTTCCTCTCCACATACCCA-3'
3
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CYP19A1
Reverse
KF452236.1
HQ846828.1
SC
AdipoR2
5'-GCTCCGTGCTCCTCTATCTG-3'
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AdipoR1
Forward
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Adiponectin
Accession no.
JX573540.1
AJ431207.1
GI:57163956
AF251387
AY148883
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ACCEPTED MANUSCRIPT Highlights •
Expression of the members of the adiponectin system was determined in the ovary of goats. Adiponectin mRNA was not expressed at detectable levels in oocytes.
•
AdipoR1 and AdipoR2 expression was detected in all evaluated follicle cells.
•
Adiponectin was shown to enhance the progression of goat oocyte nuclear
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maturation in vitro.
S0093-691X(17)30398-9
DOI:
10.1016/j.theriogenology.2017.08.013
Reference:
THE 14233
To appear in:
Theriogenology
Received Date: 5 May 2017 Revised Date:
30 July 2017
Accepted Date: 10 August 2017
Please cite this article as: Oliveira BSP, Costa JAS, Gomes ET, Silva DMF, Torres SM, Monteiro Jr. PLJ, Santos Filho AntôS, Guerra MMP, Carneiro GF, Wischral A, Batista AndréM, Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary and its effect on oocyte nuclear maturation in vitro, Theriogenology (2017), doi: 10.1016/j.theriogenology.2017.08.013. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
Revised
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Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary
2
and its effect on oocyte nuclear maturation in vitro
3
Bruna S. P. Oliveiraa, Joana A. S. Costaa, Elizabete T. Gomesa, Diogo M. F. Silvaa,
4
Sandra M. Torresa, Pedro L. J. Monteiro Jrb, Antônio S. Santos Filhoc, Maria Madalena
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P.Guerraa, Gustavo F. Carneirod, Aurea Wischrala, André M. Batistaa,*
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a
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Pernambuco, Brazil.
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b
Department of Animal Science, University of São Paulo, Piracicaba, SP, Brazil.
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Agronomic Institute of Pernambuco, Arcoverde, PE, Brazil.
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UAG/University Federal Rural of Pernambuco, Garanhuns, PE, Brazil.
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Department of Veterinary Medicine, Federal Rural University of Pernambuco, Recife,
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* Corresponding author: Department of Veterinary Medicine, Rural Federal
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University of Pernambuco, Dom Manoel de Medeiros street, s/n, Dois Irmãos, CEP
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52171-900, Recife, Pernambuco, Brazil. Tel.: +55 81 3320 6414; fax: +55 81 3320
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6057. E-mail address: [email protected]
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ACCEPTED MANUSCRIPT ABSTRACT
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Adiponectin is an adipokine secreted primarily by adipocytes and is involved in the
28
control of male and female reproductive functions. Circulating levels of adiponectin are
29
inversely correlated with body fat mass, and its biological effects are predominantly
30
mediated through two receptors, AdipoR1 and AdipoR2. The aim of the present study
31
was to verify the expression of the adiponectin system (adiponectin and its receptors,
32
AdipoR1 and AdipoR2) in goat ovary using qPCR and immunohistochemistry analyses
33
and further investigate the in vitro effects of recombinant adiponectin (5 µg/mL and 10
34
µg/mL) on goat oocyte nuclear maturation. We demonstrated that the mRNA and
35
proteins of the adiponectin system are present in goat ovary. Gene and protein
36
expression of AdipoR1 and AdipoR2 was detected in follicular cells (oocyte, cumulus,
37
granulosa and theca) of small and large antral follicles, while adiponectin mRNA was
38
not detected in oocytes from small and large follicles or in large follicle cumulus cells.
39
Finally, addition of various concentrations of adiponectin in maturation medium
40
affected the number of oocytes that reached metaphase II. In conclusion, in the present
41
study, we detected expression of adiponectin and its receptors AdipoR1 and AdipoR2 in
42
goat ovarian follicles. Furthermore, we demonstrated that recombinant adiponectin
43
increases nuclear maturation of goat oocytes in vitro.
44
Keywords: follicle, ovary, goat, adipose tissue, gene expression
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1. Introduction
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Increased livestock productivity has become a major research topic in response
48
to increases in the population and consumption [1]. In this context, understanding the
49
reproductive physiology of these animals is key to improving reproductive techniques
50
and, consequently, increasing productivity. In ruminants, reproductive function can be 2
ACCEPTED MANUSCRIPT 51
influenced at different levels of the hypothalamic-pituitary-gonadal axis by energetic
52
alterations related to diet [2], with a well-known relationship between energetic balance
53
and reproduction [3]. Adipose tissue, once recognized only for its role as an energy reservoir, has been
55
identified as an important modulator of this relationship [4,5]. Now recognized as an
56
endocrine organ, adipose tissue releases a wide variety of protein factors called
57
adipokines [6]. These adipokines have important effects on various physiological
58
processes, including reproduction [7]. Adiponectin, a 30 kDa, 244 amino acid protein,
59
has an N-terminal signal sequence, a species-dependent variable sequence, a collagen
60
domain, and a C-terminal globular domain [8,9]. Its secretion is inversely related to
61
adipose tissue levels [10], and its circulating levels are two to three times higher in
62
females than those in males [11].
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Adiponectin acts through two specific membrane receptors, AdipoR1 and
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AdipoR2 [12]. These receptors are formed by seven transmembrane domains, with an
65
intracellular N-terminus and an extracellular C-terminus, and have an opposite
66
orientation to that of classical G-proteins-coupled receptors [13,14]. The adiponectin
67
system was identified in different organs of the female reproductive system in various
68
species. Adiponectin, AdipoR1 and AdipoR2 were observed in ovarian cells of cattle
69
[15], chickens [16], mice [17] and swine [18]. AdipoR1 and AdipoR2 were also
70
identified in ovarian fish cells [19] and humans [20,21]. Adiponectin protein was also
71
visualized in ovine follicular cells [22].
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The literature suggests that adiponectin has a steroidogenic effect on ovarian
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function. In pigs, in vitro studies have shown that adiponectin reduced basal
74
testosterone secretion in internal theca cells; in granulosa cells, it increased secretion of
75
estradiol and, in combination with insulin, increased secretion of progesterone [23]. In
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77
progesterone and estradiol [20]. In chickens, adiponectin was also shown to modify the
78
progesterone secretion pattern induced by LH, FSH or IGF-1 in granulosa cells [16].
79
This adipokine effect was also verified in oocyte maturation in vitro. In pigs,
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adiponectin promoted nuclear maturation of treated oocytes [18]; however this effect
81
was not observed in cattle [15,24].
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Regarding caprine species, no reports were found on the adiponectin system and
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its influence on female reproduction. Thus, the objective of this work was first to
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investigate mRNA and protein expression of the adiponectin system (adiponectin,
85
AdipoR1 and AdipoR2) in goat ovary and second to study the effects of recombinant
86
adiponectin on goat oocyte maturation in vitro.
87
2. Materials and methods
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2.1.Tissue collection
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Antral follicles were dissected from the ovaries of adult goats (Capra hircus),
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collected independently of the stage of estrous cycle, obtained from a commercial
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slaughterhouse and transported to the laboratory in saline solution on ice. Isolated
93
follicles were classified based on the diameter as small (<3 mm) and large (≥ 3 mm)
94
antral follicles.
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Follicles were pooled (10-15 follicles/category) separately into petri dishes in
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phosphate-buffered saline (PBS) and then sectioned under a stereomicroscope (Nikon
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Corporation, Tokyo, Japan). Granulosa cells (GCs) adhering to follicle wall were
98
removed by gentle scraping with a scalpel blade. After removal of all cumulus-oocyte
99
complexes (COCs) from the petri dish, GCs were recovered by centrifugation at 1200 g
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for 1 min. Then, the theca cell layers (TC) were vortexed for 1 min in 1 ml PBS, 4
ACCEPTED MANUSCRIPT 101
transferred to 1 ml of fresh buffer and centrifuged for 1 min. The GC and TC pellets
102
were homogenized in 0.5 ml of TRI® Reagent (Invitrogen, Thermo Fisher Scientific,
103
Inc., Carlsbad, CA, USA) and stored at - 80°C until RNA extraction. Cumulus-oocyte complexes were aspirated from small and large antral follicles.
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Cumulus cells were mechanically separated by careful and repeated pipetting until no
106
adherent cumulus cells could be observed under the stereomicroscope. Pools of 10-15
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denuded oocytes and cumulus cells of 10-15 COCs, of each category of follicle, were
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collected and immediately subjected to total RNA extraction using TRI® reagent. Six
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samples of each tissue pool were analyzed.
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Cross-contamination of granulosa and theca cells was tested by detection of
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mRNA encoding the cytochrome P450 aromatase (CYP19A1) and 17α-hydroxylase
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(CYP17A1) in each sample by PCR as described by Batista et al. [25]. The presence of
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CYP19A1 amplicons in theca samples or CYP17A1 in granulosa samples indicated
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cross-contamination, and such samples were discarded.
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2.2.Total RNA extraction and cDNA synthesis
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Total RNA was extracted from each cell pool (oocytes, cumulus cells, GCs and
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TCs) using TRI® reagent. Samples were homogenized in 500 µl of TRI® reagent and
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extracted with 100 µl chloroform; after separation of the aqueous phase, RNA was
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precipitated with isopropanol and washed in 70% (v/v) ethanol, and the RNA pellet was
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eluted in MilliQ water. Then, to eliminate possible DNA contamination, all total RNA
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samples were treated with RNase-free DNase (RQ1, Promega, Madison, USA)
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according to the manufacturer's recommended protocol. Total RNA was quantified by
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measuring the absorbance at 260 nm, and RNA purity was determined by the 260/280
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nm absorbance ratio using a NanoVue spectrophotometer (GE Healthcare Life
126
Sciences Chicago, Illinois, United States). For complementary DNA (cDNA), 1 µg of total RNA was mixed with 0.5 µg
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random hexamers (Promega, Madison, WI, USA) and 0.5 µg oligo-d(T) primer
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(Promega, Madison, WI, USA). The mixture was then subjected to denaturation at 70°C
130
for 5 min and immediately chilled in ice water for 5 min. Subsequently, 13 µL of cDNA
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master mix consisting of 1 µL reverse transcriptase (GoScript™; Promega), 4 µL 5×
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reaction buffer (GoScript™; Promega), 4 µL MgCl2 (25 mM; Promega), 1 µL dNTP
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working stock (0.5mM; Promega), and 3 µL of nuclease-free water was added. The
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samples underwent annealing at 25°C for 5 min, extension at 42°C for 60 min and
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inactivation at 70°C for 15 min.
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2.3.Real-time PCR
Quantitative real-time polymerase chain reaction (qPCR) was performed using a
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Rotor-Gene Q Real-Time PCR System (Qiagen, Hilden, Germany). Primers used were
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designed based on the published sequences for goat adiponectin (GenBank:
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KF452236.1),
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JX573540.1).
143
dehydrogenase (GAPDH) and ubiquitin (UBQ) have been previously described [26].
144
Primers sequences are shown in Table 1.
(GenBank:
EP
AdipoR1
Primers
for
the
HQ846828.1)
reference
genes
and
AdipoR2
(GenBank:
glyceraldehyde-3-phosphate
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The qPCR assay was performed in a final reaction volume of 15 µL containing 2
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µL of the standardized sample at a 500 µg/mL concentration, 7.5 µL of qPCR Master
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Mix (GoTaq® qPCR Master Mix; Promega, Madison, USA), 0.5 µL of each forward
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and reverse primer and 4.5 µl nuclease free water. The protocol consisted of one
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activation phase (95°C for 2 min) and one unfolding phase (95°C for 15 sec) followed
150
by 40 annealing/extension cycles (60°C for 60 sec). Samples were measured in duplicate with a negative control for each primer
152
evaluated. Calculation of the relative expression level of adiponectin, AdipoR1 and
153
AdipoR2 genes was conducted based on the comparative cycle threshold method
154
(∆∆CT) [27] and normalized using the geometrical means of reference gene expression
155
levels: GAPDH and UBQ. Expression of adiponectin, AdipoR1 and AdipoR2 genes was
156
calculated by the equation 2−∆∆CT, where ∆CT value was determined by subtracting the
157
corresponding geometrical means of reference genes (GAPDH and UBQ) CT value
158
from the specific CT of the target. Calculation of ∆∆CT involved using the highest
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sample ∆CT value (i.e., the sample with the lowest target expression) as an arbitrary
160
constant to subtract from all other ∆CT sample values.
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2.4.Immunohistochemistry
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Goat ovaries were collected from a commercial abattoir, bisected, and fixed in
164
4% paraformaldehyde in PBS for 24 hours. Fixed tissues were subsequently dehydrated,
165
diaphanized and included in paraffin. Serial sections (4 µm) were mounted on silanized
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slides (S4651; Sigma, St. Louis, USA), dried overnight at 37°C, deparaffinized in
167
xylene and hydrated in decreasing concentrations of ethanol.
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Endogenous peroxidase activity was blocked by tissue incubation in a
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peroxidase blocking reagent (Dako, Carpinteria, USA) for 30 min. Antigen retrieval
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was performed by immersing the sections in citrate buffer (pH 6.0) in a microwave
171
oven. Then, non-specific reactions were blocked with normal goat serum (1:10; Dako,
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Glostrup, Denmark) in PBS for 30 min. The rabbit polyclonal antibodies anti-
173
adiponectin (N-20-R, sc-17044, Santa Cruz Biotechnology, Santa Cruz, CA, USA), 7
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99184; Santa Cruz Biotechnology) diluted 1:50 in blocking buffer were incubated with
176
tissues overnight at 4°C. Antibodies used in this study are recommended for the
177
detection of adiponectin and its receptors in most animal species, including rat, human,
178
equine, swine, canine and bovine. Sections were then washed in PBS and incubated
179
with a peroxidase-conjugated polymer (EnVision ™ + Dual Link System-HRP; Dako,
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Carpinteria, USA) in a humidified chamber at room temperature for 30 min.
181
Immunostaining was revealed by incubation at room temperature with 3-3'-
182
diaminobenzidine
183
counterstained with hematoxylin, photographed and examined by a Leica DM 500 light
184
microscope coupled with a Leica ICC50 HD camera and EZ LAS 4.3 software (Leica
185
Microsystems Nussloch GmbH, Nussloch, Germany). In the negative controls, the
186
primary antibody was omitted from the procedure or primary antibodies were
187
preincubated with blocking peptide (sc-17044P, Santa Cruz Biotechnology, Santa Cruz,
188
CA, USA) or adiponectin at a ratio of 1:100. No immunoreaction was observed in the
189
control preparations.
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Carpinteria,
USA).
Finally,
sections
were
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(DAB,
2.5.In vitro maturation (IVM)
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Adult goat ovaries were collected from commercial abattoir and transported to
193
the laboratory at 38°C in PBS containing antibiotic/antimycotic solution (Ab/Am, 100
194
U/mL penicillin, 100 µg/mL streptomycin and 0.25 µg/mL amphotericin B; Gibco, Life
195
Technologies, Grand Island, NY, USA) within two hours of slaughter. COCs were
196
obtained by aspiration of antral follicles between 2 and 8 mm in diameter with an 18G
197
needle connected to a 10 mL syringe, which was previously filled with 3 mL of
198
HEPES-buffered TCM199 and supplemented with Ab/Am solution. The samples were 8
ACCEPTED MANUSCRIPT 199
selected under a stereomicroscope (Nikon Corporation, Tokyo, Japan), and only those
200
with at least one layer of compact cumulus cells and homogeneous cytoplasm were
201
selected. COCs were washed three times in serum-free maturation medium (TCM-199-
203
Bicarbonate, containing 2 mM L-glutamine, 0.3 mM sodium pyruvate and 50 µg/mL
204
gentamycin) and randomly distributed on 35 mm petri dishes (Nunc, Roskilde,
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Denmark) containing 25-35 oocytes in 80 µL drops of serum-free maturation medium
206
with or without adiponectin (0, 5 or 10 µg/mL) or 10% (v/v) fetal bovine serum (FBS)
207
as a positive control, under mineral oil. These adiponectin concentrations were chosen
208
based on plasma and follicular fluid levels reported in earlier studies in goats [28, 29],
209
and bovine [24]. COCs were cultured for 27 h at 38.5° C in humidified atmosphere of
210
5% CO2. Recombinant human adiponectin (rh) (full-length human adiponectin, RD
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172023100) derived from mammalian cells (HEK-293 cells) was purchased from
212
BioVendor Laboratory Medicine (Heidelberg, Germany). This experiment was repeated
213
seven times (n = 660 oocytes).
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After the maturation period, some oocytes were denuded of cumulus cells by
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careful and repeated pipetting in PBS-PVP. The denuded oocytes were incubated with
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10 µg/mL Hoechst 33342 in PBS-PVP for 30 min at room temperature, washed three
217
times in PBS-PVP and mounted on slides with the mounting medium ProLong® Gold
218
(Molecular Probes, Life Technologies, Eugene, OR, USA), covered by coverslips
219
supported by paraffin columns and sealed with nail polish. Samples were observed
220
using a Zeiss Axioplan fluorescence microscope (Carl Zeiss, Inc., Göttingen, Germany).
221
Images were acquired using AxioVision software and an AxioCam MRm digital camera
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(Carl Zeiss, Inc., Göttingen, Germany). The oocytes were classified according to the
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nuclear configuration as germinal vesicle (GV; Fig. 1A), germinal vesicle breakdown
224
(GVBD; Fig. 1B), metaphase I (MI; Fig. 1C) and metaphase II (MII; Fig. 1D).
225
2.6.Statistical analyses
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Categorical data were analyzed using the GLIMMIX Procedure of SAS fitted to
228
a binary distribution. However, due the outcome 0 or 100% some analyses were
229
performed using Fisher’s exact test using the FREQ procedure of SAS. Data were tested
230
for normality of residuals, and data with residuals not normally distributed were
231
transformed before analysis. Quantitative PCR data were analyzed using the GLIMMIX
232
procedure of SAS fitted to a Gaussian distribution with the fixed effects of cell type and
233
follicle size and the random effect of the sample.
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The GLIMMIX procedure (ANOVA) of SAS was used with generalized linear
235
model methodology. For the data analyses, a Gaussian distribution was used. The
236
variables were analyzed using a mathematical model that included the effects of the
237
treatment. The residual method was used to calculate the denominator degrees of
238
freedom to approximate the F tests in the mixed models. The relative proportion of the
239
oocytes in each nuclear stage of maturation was calculated with the following equation:
240
Relative proportion = number of the oocytes in each stage/total of oocytes. The
241
statistical comparisons were performed using means adjusted by the least squares mean
242
method.
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Differences with P ≤ 0.05 were considered significant, and those with 0.05 < P ≤
244
0.10 were considered tendencies. Results are presented as the mean ± standard error of
245
the mean (SEM).
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3. Results
248
3.1.Analysis of gene expression qPCR revealed adiponectin mRNA in cumulus cells from small follicles and in
250
GCs and TCs of both follicular sizes but not in oocytes, regardless of size, or in the
251
cumulus cells from large follicles (Figure 2A).
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Adiponectin mRNA levels in small antral follicles were significantly higher (P
253
<0.05) in the cumulus cells compared to those in GCs and TCs, and mRNA levels did
254
not differ between GCs and TCs. In large antral follicles, adiponectin mRNA levels
255
were significantly higher (P <0.05) in granulosa than those in TCs (Figure 2A).
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AdipoR1 and AdipoR2 expression was detected in all evaluated cell types
257
(oocytes, cumulus cells, GCs and TCs) of large and small antral follicles. AdipoR1 and
258
AdipoR2 showed significant differences (P <0.05) between the cell types derived only
259
from large antral follicles. AdipoR1 expression levels were significantly (P < 0.05)
260
lower in TCs compared with those in cumulus and GCs but did not differ (P > 0.05)
261
compared to oocyte levels (Figure 2B). AdipoR2 mRNA levels in TCs were
262
significantly (P < 0.05) lower than those of other cell types (Figure 2C).
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3.2. Protein expression analysis
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Positive immunolocalisation for adiponectin, AdipoR1 and AdipoR2 were found
266
in oocyte, cumulus cells and granulosa cells of the follicles at all stages of development
267
(Fig. 3). Oocytes from preantral and antral follicles showed intense and uniform
268
cytoplasmic staining for the adiponectin (Fig. 3A-C), AdipoR1 (Fig. 3E-G) and
269
AdipoR2 (Fig. 3I, J and L) proteins. In addition, theca cells showed moderate
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immunostaining for all proteins (Fig. 3D, H and K). Control tissue samples showed no
271
positive staining (Fig. 3X, Y and Z).
272
3.3. Adiponectin effects on meiotic progression
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Figure 4 shows the effects of adiponectin on goat oocyte meiotic maturation.
275
The proportion of GV or GVBD stage-blocked oocytes (Figure 4A-B) was significantly
276
reduced (P <0.05) in the 5 or 10 µg/mL adiponectin-treated groups compared to that of
277
the control group. Maturation in the presence of 5 µg/mL adiponectin resulted in higher
278
rates of MI compared to those of the group without adiponectin (P <0.05; Figure 4C).
279
Additionally, the proportion of oocytes that progressed to MII was significantly higher
280
(P <0.05) in the 5 and 10 µg/mL adiponectin-treated groups (Figure 4D) than that in the
281
control groups. Groups treated with adiponectin showed similar percentages of MII
282
compared to the group cultured with FBS.
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4. Discussion
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This study demonstrated the presence of the adiponectin system in goat follicular
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cells. Although expression and immunolocalization of the adiponectin system has
287
already been studied in other species, as well as in different cell types, the gene and
288
protein expression of adiponectin and its receptors had not been studied in goats.
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Our results demonstrated that adiponectin was not expressed at detectable levels
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in oocytes of small and large goat antral follicles or cumulus cells from large antral
291
follicles. These results differ from those reported by Maillard et al. [15] and Tabandeh
292
et al. [30], who found adiponectin expression in oocytes and cumulus cells of bovine
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antral follicles, indicating that there may be species-specific differences in ovarian
294
expression of the adiponectin gene. The lack of adiponectin mRNA in oocytes and cumulus cells from large antral
296
follicles is intriguing. However, mRNA samples from several pools of denuded oocytes
297
and cumulus cells from large antral follicles were analyzed, and none generated
298
amplicons after qPCR. Therefore, it is unlikely to be a methodological problem because
299
the reference genes GAPDH and UBQ were easily amplified in these samples, and we
300
detected AdipoR1 and AdipoR2 mRNAs in oocytes and cumulus cells.
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Quantitatively, relative adiponectin expression in cumulus cells was significantly
302
higher than that in GCs and TCs from small follicles. In large follicles, relative
303
expression in GCs was significantly higher compared with that in TCs. These data differ
304
from what has been observed in chicken ovaries, in which the expression of adiponectin
305
in TCs was 10-30-fold higher than that in GCs [16]. In addition, adiponectin expression
306
was also low in GCs of mice [17]. However, Maillard et al. [15] observed good
307
adiponectin expression in bovine GCs.
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Receptor expression analysis showed decreased expression of AdipoR1 and
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Adipo2 in TCs of large follicles compared with expression of receptors in GCs. These
310
results differ from those found by Tabandeh et al. [30] in cattle, where AdipoR1 and
311
AdipoR2 expression was higher in large follicle TCs than that in GCs. Our findings also
312
differ from results observed in mice, in which receptor expression in GCs was lower
313
than in TCs [17]. However, similar results were observed in chickens, where AdipoR1
314
expression was twice as high in GCs as that in TCs, and AdipoR2 expression was
315
similar in both cell types [16]. This discrepancy suggests a species-specific mode of
316
action of the adiponectin system on follicular development.
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ACCEPTED MANUSCRIPT In the present study, adiponectin and its receptors AdipoR1 and AdipoR2 were
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immunolocalized in oocytes, cumulus cells, GCs and TCs in ovarian follicles at all
319
stages of development. These findings corroborate those obtained in bovines [15], mice
320
[17] and humans [21] and further support the physiological relevance of this hormone
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on ovarian function.
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Adiponectin protein was detected in the oocytes by immunohistochemistry,
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although no mRNA was observed, indicating that adiponectin must be produced
324
elsewhere and then transported to the oocyte. This is likely because adiponectin is a
325
secreted protein, is found in follicular fluid [29], and binds to its receptors on granulosa,
326
cumulus and oocyte cells; receptor-bound adiponectin has been shown to be internalized
327
in several cell lines [31,32]. The detection of adiponectin appears to be specific because
328
preincubation of the antibody with blocking peptide abolished staining.
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Oocyte meiotic maturation and acquisition of developmental competence is an
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essential physiological process for survival of the species. The presence of AdipoR1 and
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AdipoR2 mRNA and protein in both oocytes and cumulus cells suggests that both cell
332
types are sensitive to adiponectin and that adiponectin may also affect oocyte
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maturation.
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In the present work, we demonstrated that adiponectin addition (5 or 10 µg/mL)
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during IVM affected goat oocyte meiotic maturation. However, conflicting results have
336
been reported in the literature. In cattle, supplementation of IVM medium with
337
adiponectin (5 or 10 µg/mL) did not affect bovine oocyte meiotic maturation [15,24]. In
338
pigs, however, Chappaz et al. [18] reported that recombinant porcine adiponectin (30
339
µg/mL) significantly decreased the proportion of immature oocytes, suggesting that
340
adiponectin accelerated porcine oocyte meiotic maturation.
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ACCEPTED MANUSCRIPT These apparently controversial IVM results reported in the literature are
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probably dependent on the species studied or on the culture medium used. The
343
experiment described in the present study was performed with serum-free medium and
344
in the absence of any growth factor or hormone other than adiponectin. However, other
345
studies have usually added gonadotropins or growth factors to the culture media; these
346
additives could have influenced the action of adiponectin or affected its pathways,
347
resulting in different responses. Thus, possible interactions between these additives and
348
the possible pathways by which adiponectin affects oocyte maturation remain unclear
349
and require further investigation.
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In conclusion, this study detected the expression of adiponectin and its receptors,
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AdipoR1 and AdipoR2, in goat ovarian follicles. In addition, adiponectin was shown to
352
enhance the progression of goat oocyte nuclear maturation in vitro. The present findings
353
provide evidence for paracrine/autocrine effects of the analyzed hormone. However,
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future studies are needed to elucidate the mechanisms underlying the effect of
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adiponectin on meiotic maturation and to understand the role of the adiponectin system
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in goat fertility.
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Declaration of interest
The authors declare that there is no conflict of interest that could be perceived as
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prejudicing the impartiality of the research reported.
Acknowledgements The authors thank FACEPE (Fundação de Amparo à Ciência e Tecnologia do Estado de Pernambuco) for financial support (APQ-1115-5.05/14).
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2005;26:439–51. doi:10.1210/er.2005-0005. [14] Yamauchi T, Kamon J, Ito Y, Tsuchida A, Yokomizo T, Kita S, et al. Cloning of adiponectin receptors that mediate antidiabetic metabolic effects. Nature
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[15] Maillard V, Uzbekova S, Guignot F, Perreau C, Ramé C, Coyral-Castel S, et al.
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[16] Chabrolle C, Tosca L, Crochet S, Tesseraud S, Dupont J. Expression of
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adiponectin and its receptors (AdipoR1 and AdipoR2) in chicken ovary: Potential
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role in ovarian steroidogenesis. Domest Anim Endocrinol 2007;33:480–7.
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doi:10.1016/j.domaniend.2006.08.002. [17] Chabrolle C, Tosca L, Dupont J. Regulation of adiponectin and its receptors in rat ovary by human chorionic gonadotrophin treatment and potential involvement
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of adiponectin in granulosa cell steroidogenesis. Reproduction 2007;133:719–31.
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doi:10.1530/REP-06-0244.
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[18] Chappaz E, Albornoz MS, Campos D, Che L, Palin MF, Murphy BD, et al.
Adiponectin enhances in vitro development of swine embryos. Domest Anim
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Endocrinol 2008;35:198–207. doi:10.1016/j.domaniend.2008.05.007.
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[19] Nishio SI, Gibert Y, Bernard L, Brunet F, Triqueneaux G, Laudet V. Adiponectin and adiponectin receptor genes are coexpressed during zebrafish embryogenesis
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and regulated by food deprivation. Dev Dyn 2008;237:1682–90.
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doi:10.1002/dvdy.21559.
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[20] Chabrolle C, Tosca L, Ramé C, Lecomte P, Royère D, Dupont J. Adiponectin increases insulin-like growth factor I-induced progesterone and estradiol
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secretion in human granulosa cells. Fertil Steril 2009;92:1988–96.
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doi:10.1016/j.fertnstert.2008.09.008.
[21] Comim F V., Hardy K, Franks S. Adiponectin and its receptors in the ovary:
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Further evidence for a link between obesity and hyperandrogenism in polycystic
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ovary syndrome. PLoS One 2013;8:1–9. doi:10.1371/journal.pone.0080416.
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[22] Ortega HH, Rey F, Velazquez MML, Padmanabhan V. Developmental programming: effect of prenatal steroid excess on intraovarian components of
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insulin signaling pathway and related proteins in sheep. Biol Reprod
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2010;82:1065–75. doi:10.1095/biolreprod.109.082719.
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[23] Kiezun M, Smolinska N, Maleszka A, Dobrzyn K, Szeszko K, Kaminski T. Adiponectin expression in the porcine pituitary during the estrous cycle and its
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effect on LH and FSH secretion. Am J Physiol Endocrinol Metab
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2014;307:E1038-46. doi:10.1152/ajpendo.00299.2014.
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[24] Divar MR, Kafi M, Mohammadi A, Azari M. The In Vitro Effect of Adiponectin on Early Bovine Embryonic Development and Transcriptomic Markers of Oocyte
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Competence. J Fertil Vitr - IVF-Worldwide, Reprod Med Genet Stem Cell Biol
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2016;4:1–7. doi:10.4172/2375-4508.1000172.
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[25] Batista AM, Silva DMF, Rêgo MJBM, Silva FLM, Silva ECB, Beltrão EIC, et al.
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The expression and localization of leptin and its receptor in goat ovarian follicles.
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Anim Reprod Sci 2013;141:142–7. doi:10.1016/j.anireprosci.2013.08.007.
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[26] Frota IM a, Leitão CCF, Costa JJN, Brito IR, van den Hurk R, Silva JR V.
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Stability of housekeeping genes and expression of locally produced growth
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factors and hormone receptors in goat preantral follicles. Zygote 2011;19:71–83.
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doi:10.1017/S0967199410000080.
[27] Livak KJ, Schmittgen TD. Analysis of relative gene expression data using real-
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time quantitative PCR and. Methods 2001;25:402–8.
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doi:10.1006/meth.2001.1262.
[28] Guzel S, Yibar A, Belenli D, Cetin I, Tanriverdi M. The concentrations of
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adipokines in goat milk: relation to plasma levels, inflammatory status, milk
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quality and composition. J Vet Med Sci 2017;79:602-607. doi:10.1292/jvms.16-
460 461
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0061.
[29] Wang Z, Meng C, Ding X, Zhang G, Wang F. Effect of body condition on
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follicle transcriptome in estrous. Peerj Prepr 2016;4:1–34.
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doi:https://doi.org/10.7287/peerj.preprints.2177v1.
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[30] Tabandeh MR, Hosseini A, Saeb M, Kafi M, Saeb S. Changes in the gene expression of adiponectin and adiponectin receptors (AdipoR1 and AdipoR2) in
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ovarian follicular cells of dairy cow at different stages of development.
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Theriogenology 2010;73:659–69. doi:10.1016/j.theriogenology.2009.11.006.
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[31] Ding Q, Wang Z, Chen Y. Endocytosis of adiponectin receptor 1 through a clathrin- and Rab5-dependent pathway 2009;19:317–27.
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doi:10.1038/cr.2008.299.
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[32] Almabouada F, Diaz-ruiz A, Rabanal-ruiz Y, Peinado JR, Vazquez-martinez R,
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Malagon MM. Adiponectin Receptors Form Homomers and Heteromers
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Exhibiting Distinct Ligand Binding and Intracellular Signaling 2013;288:3112–
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25. doi:10.1074/jbc.M112.404624.
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Table Legend
492
Table 1. Oligonucleotide primer sequences used to perform qPCR.
493
Figure Legends
495
Figure 1. Representative images of goat oocytes stained with Hoechst 33342 and
496
evaluated under fluorescence microscopy. Oocytes in germinal vesicle (GV, A),
497
germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
498
D) stages are shown.
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Figure 2. Adiponectin (A); AdipoR1 (B) and AdipoR2 (C) mRNA expression in oocyte
501
– O, cumulus cells – C, granulosa cells – G and theca cells – T isolated from small (< 3
502
mm) and large (≥ 3 mm) goat antral follicles. Different superscripts denote the statistical
503
significance between different cells types isolated from follicles in the same size
504
category (P < 0.05).
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Figure 3. Immunolocalization of adiponectin, AdipoR1 and AdipoR2 in goat ovaries.
507
Positive staining of adiponectin, AdipoR1 and AdipoR2 was observed in oocytes and
508
granulosa cells of primordial (A, E and I), primary (B and I) and secondary follicles (C,
509
F and J). Antral follicles with positive immunostaining of adiponectin, AdipoR1 and
510
AdipoR2 in oocytes, cumulus, theca and granulosa cells (D, G, H, K and L). No staining
511
was observed in the negative control (X, Y and Z). g, granulosa; t, theca, c, cumulus; o,
512
oocytes.
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Figure 4. Effects of recombinant adiponectin (0, 5 or 10 µg/mL) on the progression of
515
meiotic maturation of goat oocytes in vitro matured for 27 h. Germinal vesicle (GV, A),
21
ACCEPTED MANUSCRIPT 516
germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
517
D). The data are expressed as the mean ± SEM. Different superscripts denote the
518
statistical significance among experimental groups within the same stage of meiotic
519
maturation (P < 0.05).
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532 533 534 535 536
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Revised Highlighted
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Expression of adiponectin and its receptors (AdipoR1 and AdipoR2) in goat ovary
542
and its effect on oocyte nuclear maturation in vitro
543
Bruna S. P. Oliveiraa, Joana A. S. Costaa, Elizabete T. Gomesa, Diogo M. F. Silvaa,
544
Sandra M. Torresa, Pedro L. J. Monteiro Jrb, Antônio S. Santos Filhoc, Maria Madalena
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P.Guerraa, Gustavo F. Carneirod, Aurea Wischrala, André M. Batistaa,*
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546 547
a
548
Pernambuco, Brazil.
549
b
Department of Animal Science, University of São Paulo, Piracicaba, SP, Brazil.
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C
Agronomic Institute of Pernambuco, Arcoverde, PE, Brazil.
551
d
UAG/University Federal Rural of Pernambuco, Garanhuns, PE, Brazil.
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Department of Veterinary Medicine, Federal Rural University of Pernambuco, Recife,
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* Corresponding author: Department of Veterinary Medicine, Rural Federal
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University of Pernambuco, Dom Manoel de Medeiros street, s/n, Dois Irmãos, CEP
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52171-900, Recife, Pernambuco, Brazil. Tel.: +55 81 3320 6414; fax: +55 81 3320
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6057. E-mail address: [email protected]
560 561 562 563 564 565
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ACCEPTED MANUSCRIPT ABSTRACT
567
Adiponectin is an adipokine secreted primarily by adipocytes and is involved in the
568
control of male and female reproductive functions. Circulating levels of adiponectin are
569
inversely correlated with body fat mass, and its biological effects are predominantly
570
mediated through two receptors, AdipoR1 and AdipoR2. The aim of the present study
571
was to verify the expression of the adiponectin system (adiponectin and its receptors,
572
AdipoR1 and AdipoR2) in goat ovary using qPCR and immunohistochemistry analyses
573
and further investigate the in vitro effects of recombinant adiponectin (5 µg/mL and 10
574
µg/mL) on goat oocyte nuclear maturation. We demonstrated that the mRNA and
575
proteins of the adiponectin system are present in goat ovary. Gene and protein
576
expression of AdipoR1 and AdipoR2 was detected in follicular cells (oocyte, cumulus,
577
granulosa and theca) of small and large antral follicles, while adiponectin mRNA was
578
not detected in oocytes from small and large follicles or in large follicle cumulus cells.
579
Finally, addition of various concentrations of adiponectin in maturation medium
580
affected the number of oocytes that reached metaphase II. In conclusion, in the present
581
study, we detected expression of adiponectin and its receptors AdipoR1 and AdipoR2 in
582
goat ovarian follicles. Furthermore, we demonstrated that recombinant adiponectin
583
increases nuclear maturation of goat oocytes in vitro.
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Keywords: follicle, ovary, goat, adipose tissue, gene expression
5. Introduction
588
Increased livestock productivity has become a major research topic in response
589
to increases in the population and consumption [1]. In this context, understanding the
590
reproductive physiology of these animals is key to improving reproductive techniques 24
ACCEPTED MANUSCRIPT 591
and, consequently, increasing productivity. In ruminants, reproductive function can be
592
influenced at different levels of the hypothalamic-pituitary-gonadal axis by energetic
593
alterations related to diet [2], with a well-known relationship between energetic balance
594
and reproduction [3]. Adipose tissue, once recognized only for its role as an energy reservoir, has been
596
identified as an important modulator of this relationship [4,5]. Now recognized as an
597
endocrine organ, adipose tissue releases a wide variety of protein factors called
598
adipokines [6]. These adipokines have important effects on various physiological
599
processes, including reproduction [7]. Adiponectin, a 30 kDa, 244 amino acid protein,
600
has an N-terminal signal sequence, a species-dependent variable sequence, a collagen
601
domain, and a C-terminal globular domain [8,9]. Its secretion is inversely related to
602
adipose tissue levels [10], and its circulating levels are two to three times higher in
603
females than those in males [11].
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Adiponectin acts through two specific membrane receptors, AdipoR1 and
605
AdipoR2 [12]. These receptors are formed by seven transmembrane domains, with an
606
intracellular N-terminus and an extracellular C-terminus, and have an opposite
607
orientation to that of classical G-proteins-coupled receptors [13,14]. The adiponectin
608
system was identified in different organs of the female reproductive system in various
609
species. Adiponectin, AdipoR1 and AdipoR2 were observed in ovarian cells of cattle
610
[15], chickens [16], mice [17] and swine [18]. AdipoR1 and AdipoR2 were also
611
identified in ovarian fish cells [19] and humans [20,21]. Adiponectin protein was also
612
visualized in ovine follicular cells [22].
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The literature suggests that adiponectin has a steroidogenic effect on ovarian
614
function. In pigs, in vitro studies have shown that adiponectin reduced basal
615
testosterone secretion in internal theca cells; in granulosa cells, it increased secretion of
25
ACCEPTED MANUSCRIPT estradiol and, in combination with insulin, increased secretion of progesterone [23]. In
617
human primary granulosa cells, adiponectin increased IGF-1-induced secretion of
618
progesterone and estradiol [20]. In chickens, adiponectin was also shown to modify the
619
progesterone secretion pattern induced by LH, FSH or IGF-1 in granulosa cells [16].
620
This adipokine effect was also verified in oocyte maturation in vitro. In pigs,
621
adiponectin promoted nuclear maturation of treated oocytes [18]; however this effect
622
was not observed in cattle [15,24].
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Regarding caprine species, no reports were found on the adiponectin system and
624
its influence on female reproduction. Thus, the objective of this work was first to
625
investigate mRNA and protein expression of the adiponectin system (adiponectin,
626
AdipoR1 and AdipoR2) in goat ovary and second to study the effects of recombinant
627
adiponectin on goat oocyte maturation in vitro.
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6. Materials and methods
630
6.1.Tissue collection
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Antral follicles were dissected from the ovaries of adult goats (Capra hircus),
632
collected independently of the stage of estrous cycle, obtained from a commercial
633
slaughterhouse and transported to the laboratory in saline solution on ice. Isolated
634
follicles were classified based on the diameter as small (<3 mm) and large (≥ 3 mm)
635
antral follicles.
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Follicles were pooled (10-15 follicles/category) separately into petri dishes in
637
phosphate-buffered saline (PBS) and then sectioned under a stereomicroscope (Nikon
638
Corporation, Tokyo, Japan). Granulosa cells (GCs) adhering to follicle wall were
639
removed by gentle scraping with a scalpel blade. After removal of all cumulus-oocyte
640
complexes (COCs) from the petri dish, GCs were recovered by centrifugation at 1200 g 26
ACCEPTED MANUSCRIPT 641
for 1 min. Then, the theca cell layers (TC) were vortexed for 1 min in 1 ml PBS,
642
transferred to 1 ml of fresh buffer and centrifuged for 1 min. The TC and GC pellets
643
were homogenized in 0.5 ml of TRI® Reagent (Invitrogen, Thermo Fisher Scientific,
644
Inc., Carlsbad, CA, USA) and stored at - 80°C until RNA extraction. Cumulus-oocyte complexes were aspirated from small and large antral follicles.
646
Cumulus cells were mechanically separated by careful and repeated pipetting until no
647
adherent cumulus cells could be observed under the stereomicroscope. Pools of 10-15
648
denuded oocytes and cumulus cells of 10-15 COCs, of each category of follicle, were
649
collected and immediately subjected to total RNA extraction using TRI® reagent. Six
650
samples of each tissue pool were analyzed.
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Cross-contamination of granulosa and theca cells was tested by detection of
652
mRNA encoding the cytochrome P450 aromatase (CYP19A1) and 17α-hydroxylase
653
(CYP17A1) in each sample by PCR as described by Batista et al. [25]. The presence of
654
CYP19A1 amplicons in theca samples or CYP17A1 in granulosa samples indicated
655
cross-contamination, and such samples were discarded.
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6.2.Total RNA extraction and cDNA synthesis Total RNA was extracted from each cell pool (oocytes, cumulus cells, TCs and
659
GCs) using TRI® reagent. Samples were homogenized in 500 µl of TRI® reagent and
660
extracted with 100 µl chloroform; after separation of the aqueous phase, RNA was
661
precipitated with isopropanol and washed in 70% (v/v) ethanol, and the RNA pellet was
662
eluted in MilliQ water. Then, to eliminate possible DNA contamination, all total RNA
663
samples were treated with RNase-free DNase (RQ1, Promega, Madison, USA)
664
according to the manufacturer's recommended protocol. Total RNA was quantified by
665
measuring the absorbance at 260 nm, and RNA purity was determined by the 260/280
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nm absorbance ratio using a NanoVue spectrophotometer (GE Healthcare Life
667
Sciences Chicago, Illinois, United States). For complementary DNA (cDNA), 1 µg of total RNA was mixed with 0.5 µg
669
random hexamers (Promega, Madison, WI, USA) and 0.5 µg oligo-d(T) primer
670
(Promega, Madison, WI, USA). The mixture was then subjected to denaturation at 70°C
671
for 5 min and immediately chilled in ice water for 5 min. Subsequently, 13 µL of cDNA
672
master mix consisting of 1 µL reverse transcriptase (GoScript™; Promega), 4 µL 5×
673
reaction buffer (GoScript™; Promega), 4 µL MgCl2 (25 mM; Promega), 1 µL dNTP
674
working stock (0.5mM; Promega), and 3 µL of nuclease-free water was added. The
675
samples underwent annealing at 25°C for 5 min, extension at 42°C for 60 min and
676
inactivation at 70°C for 15 min.
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6.3.Real-time PCR
Quantitative real-time polymerase chain reaction (qPCR) was performed using a
680
Rotor-Gene Q Real-Time PCR System (Qiagen, Hilden, Germany). Primers used were
681
designed based on the published sequences for goat adiponectin (GenBank:
682
KF452236.1),
683
JX573540.1).
684
dehydrogenase (GAPDH) and ubiquitin (UBQ) have been previously described [26].
685
Primers sequences are shown in Table 1.
(GenBank:
EP
AdipoR1
Primers
for
the
HQ846828.1)
reference
genes
and
AdipoR2
(GenBank:
glyceraldehyde-3-phosphate
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The qPCR assay was performed in a final reaction volume of 15 µL containing 2
687
µL of the standardized sample at a 500 µg/mL concentration, 7.5 µL of qPCR Master
688
Mix (GoTaq® qPCR Master Mix; Promega, Madison, USA), 0.5 µL of each forward
689
and reverse primer and 4.5 µl nuclease free water. The protocol consisted of one
28
ACCEPTED MANUSCRIPT 690
activation phase (95°C for 2 min) and one unfolding phase (95°C for 15 sec) followed
691
by 40 annealing/extension cycles (60°C for 60 sec). Samples were measured in duplicate with a negative control for each primer
693
evaluated. Calculation of the relative expression level of adiponectin, AdipoR1 and
694
AdipoR2 genes was conducted based on the comparative cycle threshold method
695
(∆∆CT) [27] and normalized using the geometrical means of reference gene expression
696
levels: GAPDH and UBQ. Expression of adiponectin, AdipoR1 and AdipoR2 genes was
697
calculated by the equation 2−∆∆CT, where ∆CT value was determined by subtracting the
698
corresponding geometrical means of reference genes (GAPDH and UBQ) CT value
699
from the specific CT of the target. Calculation of ∆∆CT involved using the highest
700
sample ∆CT value (i.e., the sample with the lowest target expression) as an arbitrary
701
constant to subtract from all other ∆CT sample values.
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6.4. Immunohistochemistry
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Goat ovaries were collected from a commercial abattoir, bisected, and fixed in
705
4% paraformaldehyde in PBS for 24 hours. Fixed tissues were subsequently dehydrated,
706
diaphanized and included in paraffin. Serial sections (4 µm) were mounted on silanized
707
slides (S4651; Sigma, St. Louis, USA), dried overnight at 37°C, deparaffinized in
708
xylene and hydrated in decreasing concentrations of ethanol.
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Endogenous peroxidase activity was blocked by tissue incubation in a
710
peroxidase blocking reagent (Dako, Carpinteria, USA) for 30 min. Antigen retrieval
711
was performed by immersing the sections in citrate buffer (pH 6.0) in a microwave
712
oven. Then, non-specific reactions were blocked with normal goat serum (1:10; Dako,
713
Glostrup, Denmark) in PBS for 30 min. The rabbit polyclonal antibodies anti-
714
adiponectin (N-20-R, sc-17044, Santa Cruz Biotechnology, Santa Cruz, CA, USA), 29
ACCEPTED MANUSCRIPT anti-AdipoR1 (H-40, sc-99183, Santa Cruz Biotechnology) or anti-AdipoR2 (M -44, sc-
716
99184; Santa Cruz Biotechnology) diluted 1:50 in blocking buffer were incubated with
717
tissues overnight at 4°C. Antibodies used in this study are recommended for the
718
detection of adiponectin and its receptors in most animal species, including rat, human,
719
equine, swine, canine and bovine. Sections were then washed in PBS and incubated
720
with a peroxidase-conjugated polymer (EnVision ™ + Dual Link System-HRP; Dako,
721
Carpinteria, USA) in a humidified chamber at room temperature for 30 min.
722
Immunostaining was revealed by incubation at room temperature with 3-3'-
723
diaminobenzidine
724
counterstained with hematoxylin, photographed and examined by a Leica DM 500 light
725
microscope coupled with a Leica ICC50 HD camera and EZ LAS 4.3 software (Leica
726
Microsystems Nussloch GmbH, Nussloch, Germany). In the negative controls, the
727
primary antibody was omitted from the procedure or primary antibodies were
728
preincubated with blocking peptide (sc-17044P, Santa Cruz Biotechnology, Santa Cruz,
729
CA, USA) or adiponectin at a ratio of 1:100. No immunoreaction was observed in the
730
control preparations.
733
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Carpinteria,
USA).
Finally,
sections
were
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Dako,
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(DAB,
6.5.In vitro maturation (IVM)
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Adult goat ovaries were collected from commercial abattoir and transported to
734
the laboratory at 38°C in PBS containing antibiotic/antimycotic solution (Ab/Am, 100
735
U/mL penicillin, 100 µg/mL streptomycin and 0.25 µg/mL amphotericin B; Gibco, Life
736
Technologies, Grand Island, NY, USA) within two hours of slaughter. COCs were
737
obtained by aspiration of antral follicles between 2 and 8 mm in diameter with an 18G
738
needle connected to a 10 mL syringe, which was previously filled with 3 mL of
739
HEPES-buffered TCM199 and supplemented with Ab/Am solution. The samples were 30
ACCEPTED MANUSCRIPT 740
selected under a stereomicroscope (Nikon Corporation, Tokyo, Japan), and only those
741
with at least one layer of compact cumulus cells and homogeneous cytoplasm were
742
selected. COCs were washed three times in serum-free maturation medium (TCM-199-
744
Bicarbonate, containing 2 mM L-glutamine, 0.3 mM sodium pyruvate and 50 µg/mL
745
gentamycin) and randomly distributed on 35 mm petri dishes (Nunc, Roskilde,
746
Denmark) containing 25-35 oocytes in 80 µL drops of serum-free maturation medium
747
with or without adiponectin (0, 5 or 10 µg/mL) or 10% (v/v) fetal bovine serum (FBS)
748
as a positive control, under mineral oil. These concentrations were chosen based on
749
plasma and follicular fluid levels reported in earlier studies in goats [28, 29], and bovine
750
[24]. COCs were cultured for 27 h at 38.5° C in humidified atmosphere of 5% CO2.
751
Recombinant human adiponectin (rh) (full-length human adiponectin, RD 172023100)
752
derived from mammalian cells (HEK-293 cells) was purchased from BioVendor
753
Laboratory Medicine (Heidelberg, Germany). This experiment was repeated seven
754
times (n = 660 oocytes).
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After the maturation period, some oocytes were denuded of cumulus cells by
756
careful and repeated pipetting in PBS-PVP. The denuded oocytes were incubated with
757
10 µg/mL Hoechst 33342 in PBS-PVP for 30 min at room temperature, washed three
758
times in PBS-PVP and mounted on slides with the mounting medium ProLong® Gold
759
(Molecular Probes, Life Technologies, Eugene, OR, USA), covered by coverslips
760
supported by paraffin columns and sealed with nail polish. Samples were observed
761
using a Zeiss Axioplan fluorescence microscope (Carl Zeiss, Inc., Göttingen, Germany).
762
Images were acquired using AxioVision software and an AxioCam MRm digital camera
763
(Carl Zeiss, Inc., Göttingen, Germany). The oocytes were classified according to the
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ACCEPTED MANUSCRIPT 764
nuclear configuration as germinal vesicle (GV; Fig. 1A), germinal vesicle breakdown
765
(GVBD; Fig. 1B), metaphase I (MI; Fig. 1C) and metaphase II (MII; Fig. 1D).
766
6.6.Statistical analyses
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Categorical data were analyzed using the GLIMMIX Procedure of SAS fitted to
769
a binary distribution. However, due the outcome 0 or 100% some analyses were
770
performed using Fisher’s exact test using the FREQ procedure of SAS. Data were tested
771
for normality of residuals, and data with residuals not normally distributed were
772
transformed before analysis. Quantitative PCR data were analyzed using the GLIMMIX
773
procedure of SAS fitted to a Gaussian distribution with the fixed effects of cell type and
774
follicle size and the random effect of the sample.
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The GLIMMIX procedure (ANOVA) of SAS was used with generalized linear
776
model methodology. For the data analyses, a Gaussian distribution was used. The
777
variables were analyzed using a mathematical model that included the effects of the
778
treatment. The residual method was used to calculate the denominator degrees of
779
freedom to approximate the F tests in the mixed models. The relative proportion of the
780
oocytes in each nuclear stage of maturation was calculated with the following equation:
781
Relative proportion = number of the oocytes in each stage/total of oocytes. The
782
statistical comparisons were performed using means adjusted by the least squares mean
783
method.
EP
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Differences with P ≤ 0.05 were considered significant, and those with 0.05 < P ≤
785
0.10 were considered tendencies. Results are presented as the mean ± standard error of
786
the mean (SEM).
787
32
ACCEPTED MANUSCRIPT 788
7. Results
789
7.1.Analysis of gene expression qPCR revealed adiponectin mRNA in cumulus cells from small follicles and in
791
GCs and TCs of both follicular sizes but not in oocytes, regardless of size, or in the
792
cumulus cells from large follicles (Figure 2A).
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Adiponectin mRNA levels in small antral follicles were significantly higher (P
794
<0.05) in the cumulus cells compared to those in GCs and TCs, and mRNA levels did
795
not differ between GCs and TCs. In large antral follicles, adiponectin mRNA levels
796
were significantly higher (P <0.05) in granulosa than those in TCs (Figure 2A).
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AdipoR1 and AdipoR2 expression was detected in all evaluated cell types
798
(oocytes, cumulus cells, GCs and TCs) of large and small antral follicles. AdipoR1 and
799
AdipoR2 showed significant differences (P <0.05) between the cell types derived only
800
from large antral follicles. AdipoR1 expression levels were significantly (P < 0.05)
801
lower in TCs compared with those in cumulus and GCs but did not differ (P > 0.05)
802
compared to oocyte levels (Figure 2B). AdipoR2 mRNA levels in TCs were
803
significantly (P < 0.05) lower than those of other cell types (Figure 2C).
806
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7.2. Protein expression analysis
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Positive immunolocalisation for adiponectin, AdipoR1 and AdipoR2 were found
807
in oocyte, cumulus cells and granulosa cells of the follicles at all stages of development
808
(Fig. 3). Oocytes from preantral and antral follicles showed intense and uniform
809
cytoplasmic staining for the adiponectin (Fig. 3A-C), AdipoR1 (Fig. 3E-G) and
810
AdipoR2 (Fig. 3I, J and L) proteins. In addition, theca cells showed moderate
33
ACCEPTED MANUSCRIPT 811
immunostaining for all proteins (Fig. 3D, H and K). Control tissue samples showed no
812
positive staining (Fig. 3X, Y and Z).
813
7.3.Adiponectin effects on meiotic progression
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Figure 4 shows the effects of adiponectin on goat oocyte meiotic maturation.
816
The proportion of GV or GVBD stage-blocked oocytes (Figure 4A-B) was significantly
817
reduced (P <0.05) in the 5 or 10 µg/mL adiponectin-treated groups compared to that of
818
the control group. Maturation in the presence of 5 µg/mL adiponectin resulted in higher
819
rates of MI compared to those of the group without adiponectin (P <0.05; Figure 4C).
820
Additionally, the proportion of oocytes that progressed to MII was significantly higher
821
(P <0.05) in the 5 and 10 µg/mL adiponectin-treated groups (Figure 4D) than that in the
822
control groups. Groups treated with adiponectin showed similar percentages of MII
823
compared to the group cultured with FBS.
824
825
8. Discussion
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This study demonstrated the presence of the adiponectin system in goat follicular
827
cells. Although expression and immunolocalization of the adiponectin system has
828
already been studied in other species, as well as in different cell types, the gene and
829
protein expression of adiponectin and its receptors had not been studied in goats.
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Our results demonstrated that adiponectin was not expressed at detectable levels
831
in oocytes of small and large goat antral follicles or cumulus cells from large antral
832
follicles. These results differ from those reported by Maillard et al. [15] and Tabandeh
833
et al. [30], who found adiponectin expression in oocytes and cumulus cells of bovine
34
ACCEPTED MANUSCRIPT 834
antral follicles, indicating that there may be species-specific differences in ovarian
835
expression of the adiponectin gene. The lack of adiponectin mRNA in oocytes and cumulus cells from large antral
837
follicles is intriguing. However, mRNA samples from several pools of denuded oocytes
838
and cumulus cells from large antral follicles were analyzed, and none generated
839
amplicons after qPCR. Therefore, it is unlikely to be a methodological problem because
840
the reference genes GAPDH and UBQ were easily amplified in these samples, and we
841
detected AdipoR1 and AdipoR2 mRNAs in oocytes and cumulus cells.
SC
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836
Quantitatively, relative adiponectin expression in cumulus cells was significantly
843
higher than that in GCs and TCs from small follicles. In large follicles, relative
844
expression in GCs was significantly higher compared with that in TCs. These data differ
845
from what has been observed in chicken ovaries, in which the expression of adiponectin
846
in TCs was 10-30-fold higher than that in GCs [16]. In addition, adiponectin expression
847
was also low in GCs of mice [17]. However, Maillard et al. [15] observed good
848
adiponectin expression in bovine GCs.
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Receptor expression analysis showed decreased expression of AdipoR1 and
850
Adipo2 in TCs of large follicles compared with expression of receptors in GCs. These
851
results differ from those found by Tabandeh et al. [30] in cattle, where AdipoR1 and
852
AdipoR2 expression was higher in large follicle TCs than that in GCs. Our findings also
853
differ from results observed in mice, in which receptor expression in GCs was lower
854
than in TCs [17]. However, similar results were observed in chickens, where AdipoR1
855
expression was twice as high in GCs as that in TCs, and AdipoR2 expression was
856
similar in both cell types [16]. This discrepancy suggests a species-specific mode of
857
action of the adiponectin system on follicular development.
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35
ACCEPTED MANUSCRIPT In the present study, adiponectin and its receptors AdipoR1 and AdipoR2 were
859
immunolocalized in oocytes, cumulus cells, GCs and TCs in ovarian follicles at all
860
stages of development. These findings corroborate those obtained in bovines [15], mice
861
[17] and humans [21] and further support the physiological relevance of this hormone
862
on ovarian function.
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Adiponectin protein was detected in the oocytes by immunohistochemistry,
864
although no mRNA was observed, indicating that adiponectin must be produced
865
elsewhere and then transported to the oocyte. This is likely because adiponectin is a
866
secreted protein, is found in follicular fluid [29], and binds to its receptors on granulosa,
867
cumulus and oocyte cells; receptor-bound adiponectin has been shown to be internalized
868
in several cell lines [31,32]. The detection of adiponectin appears to be specific because
869
preincubation of the antibody with blocking peptide abolished staining.
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863
Oocyte meiotic maturation and acquisition of developmental competence is an
871
essential physiological process for survival of the species. The presence of AdipoR1 and
872
AdipoR2 mRNA and protein in both oocytes and cumulus cells suggests that both cell
873
types are sensitive to adiponectin and that adiponectin may also affect oocyte
874
maturation.
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In the present work, we demonstrated that adiponectin addition (5 or 10 µg/mL)
876
during IVM affected goat oocyte meiotic maturation. However, conflicting results have
877
been reported in the literature. In cattle, supplementation of IVM medium with
878
adiponectin (5 or 10 µg/mL) did not affect bovine oocyte meiotic maturation [15,24]. In
879
pigs, however, Chappaz et al. [18] reported that recombinant porcine adiponectin (30
880
µg/mL) significantly decreased the proportion of immature oocytes, suggesting that
881
adiponectin accelerated porcine oocyte meiotic maturation.
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36
ACCEPTED MANUSCRIPT These apparently controversial IVM results reported in the literature are
883
probably dependent on the species studied or on the culture medium used. The
884
experiment described in the present study was performed with serum-free medium and
885
in the absence of any growth factor or hormone other than adiponectin. However, other
886
studies have usually added gonadotropins or growth factors to the culture media; these
887
additives could have influenced the action of adiponectin or affected its pathways,
888
resulting in different responses. Thus, possible interactions between these additives and
889
the possible pathways by which adiponectin affects oocyte maturation remain unclear
890
and require further investigation.
SC
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In conclusion, this study detected the expression of adiponectin and its receptors,
892
AdipoR1 and AdipoR2, in goat ovarian follicles. In addition, adiponectin was shown to
893
enhance the progression of goat oocyte nuclear maturation in vitro. The present findings
894
provide evidence for paracrine/autocrine effects of the analyzed hormone. However,
895
future studies are needed to elucidate the mechanisms underlying the effect of
896
adiponectin on meiotic maturation and to understand the role of the adiponectin system
897
in goat fertility.
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900 901 902 903 904 905
Declaration of interest
The authors declare that there is no conflict of interest that could be perceived as
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prejudicing the impartiality of the research reported.
Acknowledgements The authors thank FACEPE (Fundação de Amparo à Ciência e Tecnologia do Estado de Pernambuco) for financial support (APQ-1115-5.05/14).
906
37
ACCEPTED MANUSCRIPT 907
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The expression and localization of leptin and its receptor in goat ovarian follicles.
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Anim Reprod Sci 2013;141:142–7. doi:10.1016/j.anireprosci.2013.08.007.
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Stability of housekeeping genes and expression of locally produced growth
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factors and hormone receptors in goat preantral follicles. Zygote 2011;19:71–83.
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time quantitative PCR and. Methods 2001;25:402–8.
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[30] Tabandeh MR, Hosseini A, Saeb M, Kafi M, Saeb S. Changes in the gene expression of adiponectin and adiponectin receptors (AdipoR1 and AdipoR2) in
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ovarian follicular cells of dairy cow at different stages of development.
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Theriogenology 2010;73:659–69. doi:10.1016/j.theriogenology.2009.11.006.
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[31] Ding Q, Wang Z, Chen Y. Endocytosis of adiponectin receptor 1 through a clathrin- and Rab5-dependent pathway 2009;19:317–27.
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[32] Almabouada F, Diaz-ruiz A, Rabanal-ruiz Y, Peinado JR, Vazquez-martinez R,
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Malagon MM. Adiponectin Receptors Form Homomers and Heteromers
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Exhibiting Distinct Ligand Binding and Intracellular Signaling 2013;288:3112–
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25. doi:10.1074/jbc.M112.404624.
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ACCEPTED MANUSCRIPT 1032
Table Legend
1033
Table 1. Oligonucleotide primer sequences used to perform qPCR.
1034
Figure Legends
1036
Figure 1. Representative images of goat oocytes stained with Hoechst 33342 and
1037
evaluated under fluorescence microscopy. Oocytes in germinal vesicle (GV, A),
1038
germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
1039
D) stages are shown.
SC
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1040
Figure 2. Adiponectin (A); AdipoR1 (B) and AdipoR2 (C) mRNA expression in oocyte
1042
– O, cumulus cells – C, granulosa cells – G and theca cells – T isolated from small (< 3
1043
mm) and large (≥ 3 mm) goat antral follicles. Different superscripts denote the statistical
1044
significance between different cells types isolated from follicles in the same size
1045
category (P < 0.05).
TE D
M AN U
1041
1046
Figure 3. Immunolocalization of adiponectin, AdipoR1 and AdipoR2 in goat ovaries.
1048
Positive staining of adiponectin, AdipoR1 and AdipoR2 was observed in oocytes and
1049
granulosa cells of primordial (A, E and I), primary (B and I) and secondary follicles (C,
1050
F and J). Antral follicles with positive immunostaining of adiponectin, AdipoR1 and
1051
AdipoR2 in oocytes, cumulus, theca and granulosa cells (D, G, H, K and L). No staining
1052
was observed in the negative control (X, Y and Z). g, granulosa; t, theca, c, cumulus; o,
1053
oocytes.
AC C
EP
1047
1054 1055
Figure 4. Effects of recombinant adiponectin (0, 5 or 10 µg/mL) on the progression of
1056
meiotic maturation of goat oocytes in vitro matured for 27 h. Germinal vesicle (GV, A),
43
ACCEPTED MANUSCRIPT germinal vesicle breakdown (GVBD, B), metaphase I (MI, C), and metaphase II (MII,
1058
D). The data are expressed as the mean ± SEM. Different superscripts denote the
1059
statistical significance among experimental groups within the same stage of meiotic
1060
maturation (P < 0.05).
AC C
EP
TE D
M AN U
SC
RI PT
1057
44
21
ACCEPTED MANUSCRIPT 1
Table 1. Oligonucleotide primer sequences used to perform qPCR.
2 Gene
Primer sequences (5'-3')
GAPDH
Ubiquitin
CYP17A1
Forward
5'-GAAGGTGGTGTTCGGGATGT-3'
Reverse
5'-CAGTGTGGAAGAGCCAGGAG-3'
Forward
5'-GCTCTCAGGCTCAGGAAAGG-3'
Reverse
5'-AAGCCAGACGCCTCTACAAG-3'
Forward
5'- TGTTTGTGATGGGCGTGAACCA-3'
Reverse
5'-ATGGCGTGGACAGTGGTCATAA-3'
Forward
5'-GAAGATGGCCGCACTCTTCTGAT-3'
Reverse
5’-ATCCTGGATCTTGGCCTTCACGTT-3'
RI PT
5'-CCGCATAGACCCCATTGTGA-3'
Forward
5'-ACTGAATGCCTTTGCCCTGT-3'
Reverse
5'-CTGATTATGTTGGTGACCGCC-3'
Forward
5'-CATCCTCAATACCAGGTCCCA-3'
Reverse
5'-GGTTTCCTCTCCACATACCCA-3'
3
AC C
EP
CYP19A1
Reverse
KF452236.1
HQ846828.1
SC
AdipoR2
5'-GCTCCGTGCTCCTCTATCTG-3'
M AN U
AdipoR1
Forward
TE D
Adiponectin
Accession no.
JX573540.1
AJ431207.1
GI:57163956
AF251387
AY148883
22
ACCEPTED MANUSCRIPT 1
Figure 1
4 5 6 7 8 9 10
AC C
3
EP
TE D
M AN U
SC
RI PT
2
23
ACCEPTED MANUSCRIPT 11
Figure 2
AC C
EP
TE D
M AN U
SC
RI PT
12
13 14
24
ACCEPTED MANUSCRIPT 15
Figure 3
SC
RI PT
16
17
M AN U
18 19 20 21
25 26 27 28 29 30 31 32 33
EP
24
AC C
23
TE D
22
25
ACCEPTED MANUSCRIPT 34
Figure 4
M AN U
SC
RI PT
35
36
40 41 42 43 44 45 46 47 48
EP
39
AC C
38
TE D
37
ACCEPTED MANUSCRIPT Highlights •
Expression of the members of the adiponectin system was determined in the ovary of goats. Adiponectin mRNA was not expressed at detectable levels in oocytes.
•
AdipoR1 and AdipoR2 expression was detected in all evaluated follicle cells.
•
Adiponectin was shown to enhance the progression of goat oocyte nuclear
RI PT
•
AC C
EP
TE D
M AN U
SC
maturation in vitro.