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COP1 plays a prominent role in drought stress tolerance in Arabidopsis and Pea
Accepted Manuscript COP1 plays a prominent role in drought stress tolerance in Arabidopsis and pea Maryam Moazzam Jazi, Samaneh Ghasemi, Seyed Mahdi Seyedi, Vahid Niknam PII:
S0981-9428(18)30353-X
DOI:
10.1016/j.plaphy.2018.08.015
Reference:
PLAPHY 5376
To appear in:
Plant Physiology and Biochemistry
Received Date: 5 July 2018 Accepted Date: 8 August 2018
Please cite this article as: M.M. Jazi, S. Ghasemi, S.M. Seyedi, V. Niknam, COP1 plays a prominent role in drought stress tolerance in Arabidopsis and pea, Plant Physiology et Biochemistry (2018), doi: 10.1016/j.plaphy.2018.08.015. 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.
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COP1 plays a prominent role in drought stress tolerance in Arabidopsis and Pea
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Maryam Moazzam Jazi1, Samaneh Ghasemi2, Seyed Mahdi Seyedi1*, Vahid Niknam2
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Biotechnology, Tehran, Iran
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Tehran, Iran
Plant
Biotechnology
Department,
National
Correspondence: Seyed Mahdi Seyedi ([email protected])
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Genetic
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Abstract
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Constitutively photomorphogenic 1(COP1) is an E3 ubiquitin ligase that has been studied extensively in
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the photomorphogenesis- and light-related processes in Arabidopsis. However, the possible role of COP1
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in plant drought stress response remains unknown. Hence, in the present study, the stomatal behavior as
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one of the key elements in plant dehydration response was investigated in Arabidopsis cop1-4 and pea
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light-independent photomorphogenesis (lip1) mutants. We observed that water loss rate in the cop1-4 and
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lip1 detached leaves were significantly much faster than wild-type, resulting from failing to reduce the
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stomatal aperture by the mutants. But, interestingly, the cop1-4 and lip1 isolated leaves treated with
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abscisic acid (ABA) as well as cop1-4 soil-grown under drought stress could close their stomata as wild-
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type. Hence, COP1 plays a fundamental role in the regulation of stomatal movements in response to
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dehydration and its function was conserved during evolution in both Arabidopsis and pea. Further
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evaluations showed the cop1-4 mutant was not significantly damaged from the oxidative stress derived
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from soil water limiting conditions when compared to wild-type. Similarly, the up-regulation level of
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several key stress-responsive genes was relatively lower in cop1-4 than wild-type. Therefore, COP1
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might be considered as a potential key regulator of both short-and long-term dehydration response.
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Multiple stress-related cis-elements were also detected in the COP1 promoter region, which supported its
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up-regulation in response to drought, salt, and cold stresses. Besides, we figured out the constitutively
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open stomata of cop1-4 in darkness can be as a result of the reduced AtMYB61 expression.
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Key words: Arabidopsis, COP1, Drought stress, Pea, Stomata, Water loss.
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Abbreviations
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ABA, abscisic acid; ABRE, abscisic acid-responsive elements; CAT, catalase; COP1, constitutively
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photomorphogenic 1; COR15a, cold-regulated protein 15a; CRT, cryptochromes; CTAB, cetyltrimethyl
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ammonium bromide; DRE, dehydration response element; ERD1, early response to dehydration 1; FC,
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field capacity; HSF, heat shock transcription factor; HY5, long hypocotyl 5; LIP, light-independent
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photomorphogenesis; MDA, Malondialdehyde; PHOT, phototropins; PHYA, phytochrome A; PHYB,
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phytochrome B; PVP, Polyvinylpyrrolidone; ROS, reactive oxygen species; RWC, relative water content;
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SOD, superoxide dismutase; SUMO, Small ubiquitin-related modifier; TBA, thiobarbituric acid
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Introduction
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Water deficiency, as a result of climate change, is a major threat to supply global food resources for the
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increasing population worldwide. Drought stress is considered as one of the most important limiting
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factor for sustainable agriculture, particularly in arid and semi-arid areas, resulting in reduced crop yield
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by more than 50% every year (Atkinson and Urwin, 2012; Singh et al., 2015). It is adversely affects the
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plant growth, development, survival and productivity, hence the investigation of plant drought stress
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responses has gained widespread attention over recent years. Plants have evolved specific defence
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mechanisms in response to environmental stresses, including drought, which is characterized with a series
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of morphological, physiological, biochemical, and molecular changes in stressed plants (Krishnan and
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Pereira, 2008; Wang, 2014). Osmotic adjustment through the accumulation of compatible solutes, such as
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proline is a prevalent physiological response in plants exposed to various abiotic stresses, such as drought,
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salinity and cold (Krasensky and Jonak, 2012). Proline acts as an osmoprotectant, a molecular chaperone
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stabilizing macromolecules, and reactive oxygen species (ROS) scavenger (Szabados and Savouré, 2010).
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The glutamate-originated pathway appears to be the predominant proline biosynthesis pathway, especially
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under stress conditions (Hayat et al., 2012).
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Oxidative stress resulted from the extensive generation of ROS is an unavoidable aspect of different
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stresses (Noctor et al., 2014). Under drought conditions, stress-induced stomatal closure and the restricted
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CO2 uptake leads to the over-reduction of photosynthetic electron transport chain, favouring the electron
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transfer to oxygen and producing various kinds of ROS in the chloroplasts (Harb et al., 2010; Noctor et
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al., 2014). Although ROSs plays a key role in the signal transduction pathways at their steady-state level,
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they can initiate destructive oxidative processes such as lipid peroxidation and chlorophyll bleaching in
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the stressed plants (Miller et al., 2008; Sharma et al., 2012). Therefore, to scavenge ROS and alleviate the
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oxidative damages, plants have developed a wide range of enzymatic and non-enzymatic antioxidants,
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which superoxide dismutase (SOD) and catalase (CAT) comprised the primary enzymatic antioxidants.
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Similarly, flavonoids, cartenoids and anthocyanin are the main non-enzymatic antioxidants, accumulating
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in response to oxidative stress in most plant species (Sharma et al., 2012; You and Chan, 2015).
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Principally, plant drought responses are modulated by multiple stress-responsive genes, like RD22 and
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P5CS. The gene expression alternation ultimately promotes the cellular homeostasis, toxins detoxification
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and growth recovery of stressed plants (Nuruzzaman et al., 2013). At least six independent systems
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regulate gene expression in response to water deprivation in Arabidopsis, three of which are abscisic acid
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(ABA)-independent and the other three are ABA-dependent (Yamaguchi-Shinozaki and Shinozaki, 2006;
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Yoshida et al., 2014). Under water stress, the ABA-induced stomatal closure followed by reduced water
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loss is one of the essential aspects of drought tolerance in plants, and it is considered as a drought
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avoidance mechanism (Basu et al., 2016; Buckley, 2005). Two R2R3-MYB transcription factors,
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AtMYB60 and AtMYB61, are the main regulators of stomatal movements. The AtMYB60 expression is
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induced by white and blue light and repressed by darkness and drought stress; hence the stomatal aperture
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size is correlated with the AtMYB60 transcript level (Daszkowska-Golec and Szarejko, 2013). Contrary to
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AtMYB60, darkness promotes the expression of AtMYB61, leading to decreased stomatal aperture while
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other stomatal closuring signals, like ABA, salt and drought do not altered the AtMYB61 expression
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pattern (Liang et al., 2005).
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Among environmental signals, light is a major factor in the reflection of various plant cell movements and
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developmental processes including, stomatal movements, de-etiolation, and cotyledon opening (Ma et al.,
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2002). It has been revealed that phototropins (PHOT) and cryptochromes (CRY) are involved in blue
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light-induced stomatal opening and that COP1, a negative regulator of photomorphogenesis, likely acts
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downstream of CRY and PHOT signaling pathway to repress stomatal opening (Smirnova et al., 2012).
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COP1 is an E3 ubiquitin-ligase contributed to the degradation of photomorphogenic-related factors,
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including long hypocotyl 5 (HY5), phytochrome A (PHYA), phytochrome B (PHYB) and cryptochrome
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(CRY), resulting in photomorphogenesis repression (Jia et al., 2014; Osterlund et al., 2000).
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It has been proved that the occurrence of partial duplication within the pea homolog of COP1 give rise to
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create lip1 mutant (Sullivan and Gray, 2000). The lip1 mutants showed light-grown development when
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grown in darkness as they displayed short stems along with open and expanded shoots, like cop1-4
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(Seyyedi et al., 1999; Stoop‐Myer et al., 1999). COP1 function has been well documented during
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Arabidopsis developmental modifications in the presence and absence of light (Chang et al., 2011; Chen
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et al., 2015; Subramanian et al., 2004). However, to the best of knowledge, there is no report elucidating
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the involvement of COP1 in response to drought stress in Arabidopsis and pea. It was very recently
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demonstrated that Small ubiquitin-related modifier (SUMO) conjugation mediated by AtSIZ1 negatively
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regulated through the E3 ubiquitin-ligase activity of COP1 under abiotic stresses, thereby COP1 controls
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Arabidopsis abiotic stresses response via the modulation of the AtSIZ1 level (Kim et al., 2016). However,
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the impact of COP1 on the plant physiological and molecular responses under abiotic treatments was not
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reported.
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In the present study, wild-type (Col-0) and cop1-4 mutant of Arabidopsis (Arabidopsis thaliana) were
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subjected to dehydration treatment at two levels, short-term and long term by detaching leaves and
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stopping irrigation, respectively. In order to uncover the probable COP1 role in Arabidopsis drought
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response, some of major physiological and molecular parameters were evaluated. We also used abi1-1
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mutant, which is the drought-sensitive and ABA-insensitive plant as the control for the experiment.
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Furthermore, wild-type pea (Pisum sativum cv Alaska) and lip1 mutant were utilized to evaluate their
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stomata response to short-term and long-term dehydration.
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Materials and Methods
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Plant growth conditions and abiotic treatments
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Arabidopsis (A. thaliana), ecotype Columbia (Col-0), cop1-4, and abi1-1 mutants as well as pea (P.
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sativum cv Alaska) and lip1 mutant were used in this study. Surface-sterilized seeds were directly sown
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on pots containing a mixture of perlite, vermiculite and peat and stratified at 4°C in dark for 2 days. The
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seedlings were grown under controlled conditions at 22˚C and 70% relative humidity under long-day
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conditions (16h/8h, light/dark cycle). Short-term dehydration was imposed by excising leaf and placing
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on the laboratory bench at 23˚C and 27% relative humidity.
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Long-term drought treatment was applied to four-week-old plants (Arabidopsis and pea) by water
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withholding. The level of drought stress was gravimetrically checked (Ramegowda et al., 2013); briefly,
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pots along with plants were weighed daily until the end of experiment. Control plants were maintained at
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100% soil field capacity (FC). Upon the arrival of 75% FC (after 2 days) and 50% FC (after 4 days),
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leaves were sampled. For salt treatment, Arabidopsis plants were hydroponically grown in Hoagland’s
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nutrient solution with aeration, and the nutrient solution was renewed every three days. Four-week-old
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plants were exposed to salt stress (200 mM) by adding NaCl to the solution and leaves were collected at
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1, 3, and 5 days of salt application. For cold treatment, four-week-old soil-grown Arabidopsis plants were
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transferred to a growth chamber with 4°C for 3 days (cold acclimation), then subjected to -7°C for 6
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hours, followed by transferring to 4°C for one day. The leaves were collected after each step. For dark
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treatment, four-week-old plants grown in soil were kept at darkness for 2 days, and then leaves sampled
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under faint green light. In all cases, sampled leaves were frozen immediately in liquid nitrogen and stored
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at -80°C until use. All experiments were conducted in three biological replicates.
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Leaf relative water content
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Relative water content (RWC) was calculated by the following formula: RWC = [(fresh mass - dry mass)
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/ (saturated mass - dry mass)] × 100.
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Water loss assay
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For transpirational water loss assay, leaves from several four-week-old plants were detached, so that the
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leaves area of cop1-4 and lip1 mutants was similar to the corresponding wild-type. The leaves were
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placed in the filter paper on a laboratory bench at 23°C and 27% relative humidity and weighted at
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designated time intervals. The loss in fresh weight presented as the percentage of initial fresh weight at
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each time point (Li et al., 2008).
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Stomatal aperture measurement
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The abaxial epidermis was peeled from the leaves of multiple four-week-old plants under drought
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treatment as well as normal growth conditions and the stomata were observed by light microscopy (Zeiss
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) connected to a fitted camera. The stomatal pore width was measured using ProgRes Capture Pro 2.1
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software. For ABA-induced stomatal closure assay, the leaves were floated in the opening buffer
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containing 10 mM KCl, 10 mM CaCl2, and 10 mM MES, 0.01% Tween 20, pH 6.5 at 22°C for 2 hours to
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open the stomata. Then, the leaves were transferred to the same buffer supplemented with 10 µmol ABA,
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maintained in these conditions for 2 hours and the pore size was calculated (Tanaka et al., 2005).
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Stomatal density (i.e. the number of stomata per unit area) in both adaxial and abaxial leaf surface was
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determined in the four-week-old plants. Ten random parts (each part consisted of 0.1 mm2) from four
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leaves were counted for determination of stomatal density.
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Hydrogen peroxide and lipid peroxidation level measurement
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The H2O2 concentration was determined using the standard curve generated with known concentrations of
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H2O2 as described by (Loreto and Velikova, 2001). Malondialdehyde (MDA) level as the main index of
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lipid peroxidation was determined by the thiobarbituric acid (TBA) reaction according to Du and
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Bramlage (Du and Bramlage, 1992). The MDA concentration was calculated using extinction coefficient
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of absorbance 155 mM-1 cm-1.
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Proline content measurement
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Proline content was determined via reaction with ninhydrin reagent (Magné and Larher, 1992). Briefly,
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100 mg of fresh leaves was homogenized in 1.2 ml of 3% (w/v) aqueous sulphosalycylic acid and the
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homogenate filtered. After adding 2 ml ninhydrin (1%, w/v) to the supernatant and incubating at 98°C for
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one hour, the micro tubes were cooled and treated with 2 ml toluene. The absorbance of the upper phase
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was spectrophotometrically assessed at 518 nm after. The proline concentration was calculated according
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to a calibration curve.
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Enzymatic and non-enzymatic antioxidant assay
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For enzymatic antioxidant activity assay, 200 mg of fresh leaves was homogenized in 0.1 M Trise-HCl
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buffer (pH 7.8) containing 1 mM EDTA and 4% Polyvinylpyrrolidone (PVP) at 4°C. The resulting
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supernatant was used for enzyme assays. Proteins were quantified according to Bradford (Bradford, 1976)
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using albumin bovine serum as a standard. The per unit SOD activity was estimated by adding 40 µl of
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the enzymatic extract to a solution containing 13 mM methionine, 75 µM p-nitroblue tetrazolium chloride
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(NBT), 100 µM EDTA and 2 µM riboflavin in a 50 mm potassium phosphate buffer pH 7.5. The reaction
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started with 10 min illumination under a 30 W fluorescent lamp and stopped by turning light off. Non-
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illuminated and illuminated reactions without supernatant served as calibration standards, and the final
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reaction products were measured at 560 nm (Dhindsa et al., 1981).
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The CAT activity was assessed following the modified method by measuring the decrease in absorbance
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at 240 nm of the reaction mixture with a final volume of 2 ml containing 15 mM H2O2 in 50 mM K-
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phosphate buffer (pH 7.0) and 10 µL extract (Aebi, 1984).
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As the non-enzymatic antioxidant, the anthocyanin level was measured by homogenising leaves (50 mg)
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in acidic methanol (99:1, v/v) and recording the absorbance of the supernatant at 530 and 657 nm (Laby et
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al., 2000). The anthocyanin content expressed as follows:
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Relative units of anthocyanin/g fresh weight of tissue = OD530 - (0.25×OD657) × extraction volume (ml)
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× 1 / weight of tissue sample (g).
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Total RNA isolation and gene expression analysis
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Total RNA was extracted from 200 mg of leaves using a modified CTAB (cetyltrimethyl ammonium
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bromide) method (Moazzam-Jazi et al., 2015). After the treatment of extracted RNA with RNase free
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DNase I (Fermentas), single-stranded cDNA was synthesized from total RNA according to the
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manufacturer’s instructions (RevertAid First Strand cDNA Synthesis Kit, Fermentas). Real-time PCR was
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performed using the SYBR Green Real-time PCR master mix (Ampliqon, Denmark). The reaction
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mixture contained 1 µL of cDNA sample, 0.5 µL of each the forward and reverse primers (10 µM) and 10
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µL real-time master mix with a final volume of 20 µL. The cycling conditions were set as follows, initial
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activation of DNA polymerase at 95°C for 15 min, followed by 40 cycles 94°C for 30s, 58-60°C for 30s
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and 72°C for 30s for all genes except for P5CS1 that was 90s. The relative gene expressions of KIN2,
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P5CS1, RD22, NCED3, ABI1, MYB60, and COP1 were analysed by Pfaffl formula (Pfaffl, 2001) within
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REST 2009 software. Also, APK2a was used as the internal control. All samples were amplified in
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triplicate. The primer sequences are available in Table 1.
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Table1. Primer pairs were used for gene expression analysis Gene name
Gene Identifier
Forward primer sequence 5´-3´
APK2a
NM_101304.4
GGAGAGATACTTTCATCGCCTAA CC
GACCTGCTTTTGCCAATCCG
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KIN2
NM_121602.4
CAAAACACACATCAAAAACG
AACATTGCTCTTCTCCTCAG
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RD22
NM_122472.4
CACAAGGGAAGACCGATTTAC
TTCTCCTCTCCACTAACTTTTC TG
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P5CS1
NM_001202785.1
GTCATTTTGGTGTCATCTGGTGC
CATCAAGCTGGTCAAACATAG TC
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NCED3
NM_112304.3
TCCAGCTCTTCATTTCCCTAA
CGGCCATTGAAATAGACCAA
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ABI1
NM_118741.3
GATATCTCCGCCGGAGATGAGAT C
CATTCCACTGAATCACTTTTC CTC
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MYB60
NM_100755.3
GGACCATGGACTCCTGAAGA
CCACGTTTAATTCCAGGTCT
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COP1
NM_128855.4
TTGTTCCAGCGGTGAAACCT
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Tm (ºC)
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Reverse primer sequence 5´-3´
CAGATCCGGTGCTCCAATCT
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Promoter analysis
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The 1 kb upstream sequence from the translational initiation codon of COP1 in A. thaliana was obtained.
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In order to assess the transcription factor binding sites within the promoter region, the sequence was
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analysed using the web-based tool, “The Plant Promoter Analysis Navigator (PlantPAN 2.0;
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http://PlantPAN2.itps.ncku.edu.tw).” This tool provides resources for detecting cis-regulatory elements
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and the corresponding transcription factors in a gene promoter (Chow et al., 2016). The biological
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function
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(http://bioinfo.cau.edu.cn/agriGO/) via the singular enrichment analysis tool. The analysis was conducted
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with Fisher’s exact test and FDR cutoff of 0.05 was considered for significance.
all
transcription
factors
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using
AgriGO
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Statistical analysis
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A completely randomized design with three biological replicates was considered and all physiologic data
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analyzed using SPSS software (version of 22). The mean comparison was performed by Duncan's
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Multiple Range Test (DMRT) at the 0.05 level of confidence.
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Results
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The contrasting response of cop1-4 stomata to dehydration
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One of the earliest plant responses to drought stress is the restriction of transpirational water loss through
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stomatal closure. Previous studies revealed that the COP1 possess the regulatory role in the stomatal
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movements (Mao et al., 2005). With this information in mind, the sensitivity of cop1-4 mutant leaves to
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short-term dehydration was examined by leaf detachment. We measured the water loss rate of wild-type
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and cop1-4 leaves after incubation at 22°C in the light. Based on our results, the weight of detached
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leaves reached to the half of initial weight in the wild type and cop1-4 mutant after 180 and 30 minutes of
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leaf detachment, respectively (Fig. 1), implying that the water loss rate in the mutant leaves was much
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faster than the wild type and responsible for the appearance of wilt symptoms in the mutant.
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Fig.1. Rate of leaf water loss in cop1-4 mutant and wild-type during short-term dehydration. Water loss
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rate is expressed as the percentage of initial fresh weight. Each data point is presented as the mean ± SD
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(n=3).
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Considering the water loss assay and the central role of stomata in the modulation of transpiration rate, we
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estimated the stomatal aperture of leaves under control conditions and 10, 20, and 30 minutes after leaf
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detachment. We observed that the stomatal aperture of cop1-4 leaves was much larger than wild-type
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under normal growth conditions; the average stomatal aperture of 200 stomata was 2.8 µm in the wild-
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type while it was 6.3 µm in cop1-4 (Fig. 2). The wild-type stomata started to close after 20 minutes of leaf
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detachment and their average aperture reached to 1.5 µm, but, interestingly, the cop1-4 stomata remained
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open in the same conditions (Fig. 2A).
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Considering the key role of ABA in the coordination of stomatal conductance with the plant water supply
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(Aasamaa and Sõber, 2011), we incubated leaves with exogenous ABA (10 µmol) for 40 and 120 minutes
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to explore whether ABA treatment induces a change on the stomatal aperture of cop1-4. Following the
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assessment of stomata status, we found that the cop1-4 stomata were sensitive to ABA and their stomatal
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pores reduced in response to exogenous ABA as the wild-type plants only after 120 minutes. As
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illustrated in Fig. 2B, the average stomatal aperture of wild-type and cop1-4 leaves from 2.6 and 5.4 µm
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before ABA application, respectively, were decreased to 1.2 and 2.5 µm in response to ABA treatment for
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120 minutes (Fig. 2B), suggesting that the cop1-4 stomata is not defective in ABA-mediated stomatal
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closure, but they are less sensitive to ABA than wild-type.
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As our results demonstrated, the cop1-4 mutant is defective to sense the leaf detachment-imposed
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dehydration and reduces their stomatal aperture. Consequently, we speculated that it may result in the
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enhanced drought sensitivity at the whole plant, too. To address this possibility, wild-type and cop1-4
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mutant were planted in the soil and four-week-old plants subjected to drought treatment by withholding
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water. After the stomata status evaluation, surprisingly, we found out that the stomatal behaviour was
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similar in both with-type and mutant in response to soil water deficiency. As shown in Fig. 2C, the
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stomatal aperture average significantly decreased in the stressed plants, it was reached to 1.7 µm and 2.54
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µm from 3 µm and 6.5 µm in the wild type and cop1-4 leaves, respectively, after four days of drought
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stress (Fig. 2C).
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Fig.2. Stomatal apertures of cop1-4
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mutant and wild-type leave. (A) The
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conditions and short-term dehydration imposed by leaf detachment. (B) The cop1-4 mutant and wild-type stomata response to the leaf treatment with 10
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stomatal aperture under normal growth
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µmol ABA. (C) The cop1-4 mutant and wild-type stomatal aperture in response
to
soil
water
shortage
conditions. Data are the average stomatal aperture of 200 stomata. Means followed by the same letter(s) are not significantly different at 0.05 level of probability (DMRT).
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A representative illustration of open and closed stomata of cop1-4 and wild-type was shown in Fig. 3.
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Fig.3. Representative image of open
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and closed stomata of cop-1-4 and wild-type. (A) Wild-type, open. (B)
Wild-type, closed. (C) cop1-4, open.
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(4) cop1-4, closed.
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Furthermore, we investigated the adaxial and abaxial stomatal density of wild-type and cop1-4 mutant
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under control growth conditions (Fig. 4 A). As Fig. 4 showed, there is no significant difference in the
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number of stomata per unit of leaf area between wild-type and cop1-4 under normal growth conditions.
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Surveying the abaxial stomatal density in plants under soil drought stress revealed that this parameter has
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remained constant after 2 and 4 days of drought stress in both wild-type and cop1-4 (Fig. 4B).
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Fig.4 Adexial and abexial stomatal density of wild-type and cop1-4 mutant under normal growth
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conditions (A) and the abexial stomatal density of wild-type and cop1-4 mutant under soil drought stress
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(B). Data are the average stomatal density of 120 stomata.
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Interestingly, we observed that cop1-4 mutants soil-grown were more tolerant to drought stress than wild-
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type under our experimental conditions (Fig.5).
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Fig.5. Phenotypic picture of plants
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under normal growth conditions (A)
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treatment (B), imposed by withholding
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water.
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and after 4 days of soil drought
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The lip1 stomata contrasting response to dehydration and ABA treatment
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As LIP1 in pea is ortholog for COP1 and the lip1 mutant exhibits the similar characteristics to cop1-4
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(Sullivan and Gray, 2000), we were curious to assess its stomatal behaviour in response to dehydration as
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well as exogenous ABA treatment. Interestingly, we found a resemblance in stomatal response between
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cop1-4 and lip1 mutants under our experimental conditions. Water loss assay showed that the lip1
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detached leaves weight attained to the half of initial weight after 40 minutes while wild-type isolated
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leaves required 10.5 hours to reach the same weight, implying that lip1 fails to close its stomata in
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response to short-term dehydration as cop1-4 (Fig. 6A).
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The lip1 stomata are significantly wider than wild-type under normal growth conditions similar to those
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of cop1-4. Based on our microscopic measurements, the average stomatal aperture is 4.2 and 6.5 µm in
369
wild-type and lip1 mutant, respectively (Fig. 6B). But, the treatment of detached leaves with 10 µmol
370
ABA for 120 minutes resulted in a reduced stomatal pores in both wild-type and lip1 mutant, so that the
371
stomatal aperture of wild-type and lip1 decreased to 2.9 and 3.5 µm in response to ABA treatment.
372
Therefore, neither cop1-4 nor lip1 appear impaired in the ABA-induced stomatal closure (Fig. 6B). Our
373
findings suggested that COP1 can play an essential role in regulating the stomatal movements in both
374
Arabidopsis and pea.
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Fig.6. lip1 mutant and wild-type
376
stomatal behaviour. (A) lip1 mutant
377
and wild-type stomatal behaviour in
378
response to short-term dehydration as
379
evidenced by leaf water loss assay.
380
Water loss rate is expressed as the
381
percentage of initial fresh weight.
382
Each data point is presented as the
383
mean ± SD (n=3). (B) The lip1 mutant
384
and wild-type stomata response to the
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385
leaf treatment with 10 µmol ABA. (C)
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The lip1 mutant and wild-type stomata
387
after 2 and 4 days of drought stress.
388
Data are the average stomatal aperture
389
of 200 stomata. Means followed by
390
the same letter(s) are not significantly
391
different at 0.05 level of probability
392
(DMRT).
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Furthermore, drought treatment was applied on the soil-grown pea lip1 mutant and wild-type by water
399
withholding and the stomatal behaviour surveyed after 2 and 4 days of soil drought stress. Interestingly,
400
we observed that lip1 stomatal aperture decreased in response to soil water shortage as wild-type (Fig.
401
6C). As Fig. 6C showed, the average of stomatal aperture reduced to 4.3 µm and 2.8 µm from 6.1 µm and
402
4.3 µm in lip1 mutant and wild-type, respectively, after 4 days of drought stress.
403 404
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Evaluation of main physiological parameters related to drought stress in cop1-4
405 406
RWC content
407
RWC is an important index of plant water status and reflects the balance between the water supply and
408
transpiration rate. Hence, in order to estimate the whole plant transpiration under drought stress, we
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examined the RWC level of wild-type and cop1-4 plants after two and four days of the cessation of
410
irrigation. Based on the results, there was no difference between wild-type and cop1-4 mutant in the RWC
411
content during drought treatment, the RWC of both wild-type and cop1-4 plants significantly diminished
412
after two days of drought stress (Fig. 7A). The similarity in the level of RWC under soil water shortage
413
conditions further support that in contrast to cop1-4 detached leaves, the cop1-4 whole plant could limit
414
the transpirational water loss via the stomatal closure and maintain the RWC as wild-type plants.
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415 Proline content
417
It is well documented that proline has an important role in protecting plants under drought stress. To
418
evaluate this hypothesis and to determine the effects of cop1 mutation on drought-induced proline
419
accumulation, proline level was measured in wild-type, cop1-4, and abi1-1 mutants under normal and
420
long-term drought stress conditions. Interestingly, we found that proline content in cop1-4 mutant leaves
421
was about 4.5 fold higher than that of the wild-type under normal growth conditions (Fig. 7B). As shown
422
in Fig. 7B, soil water deficiency resulted in proline accumulation in wild-type and abi1-1 mutant leaves
423
while the level of this compatible solute remained relatively constant until the fourth day of drought
424
treatment, when significantly increased when compared to well-watered conditions. However, the cop-1-4
425
leaves exhibited the lowest proline content while abi1-1 and col had the highest proline level at the end of
426
drought treatment.
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H2O2 and MDA content
429
Since the increased ROS production is one of the major effects of a drought stress on plants and can
430
induce lipid peroxidation, the levels of H2O2 (the main ROS in plants) and MDA (the key by-product of
431
lipid peroxidation) were measured to survey the oxidative damage level during drought stress. As
432
illustrated in Figs. 7C and 7D, the H2O2 and MDA content showed no significant difference between
433
wild-type and mutant plants under normal growth conditions. However, H2O2 level was increased 2- and
434
6-fold in wild-type and abi1-1 mutant leaves, respectively, after four days of water withholding as
435
compared with the control conditions. Interestingly, no significant change in the H2O2 content was
436
observed in the cop1-4 leaves in these conditions (Fig. 7C). Regarding MDA content, in contrast to wild-
437
type and abi1-1 mutant, the MDA content was not significantly altered in the cop1-4 leaves during soil
438
water deficient treatment. However, the highest MDA content was obtained from wild-type and abi1-1
439
mutant plants after four days of stopping irrigation (Fig. 7D). Based on the results, cop1-4 mutant
440
suffered from the lower level of drought-induced oxidative damage than wild-type under our
441
experimental conditions.
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442 443
Fig.7. RWC (A), Proline (B), H2O2 (C) and MDA (D) levels in cop1-4, abi1-1 mutants as well as wild-
444
type leave in response to soil water shortage conditions. Data represent the mean ± SD (n = 3). Means
445
followed by the same letter(s) are not significantly different at 0.05 level of probability (DMRT).
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448
ROS level is modulated by a well-defined detoxification system, involving a number of antioxidants that
449
reduce the reactive oxygen species content and minimize their deleterious effects. Here, the activity of
450
two main antioxidant enzymes, SOD and CAT were surveyed to monitor enzymatic ROS detoxification
451
in the plants under drought stress. Based on our results, there was no significant difference in SOD and
452
CAT activities among wild-type and the two mutants, cop1-4 and abi1-1 leaves under normal growth
453
conditions (Fig. 8A). While the CAT activity tends to be increased during drought treatment in wild-type
454
and reached to its highest activity (2.4 fold) at the end of experiment, cop1-4 exhibited no significant
455
change in the enzyme activity. The CAT activity was enhanced after two days of drought stress in abi1-1
456
leaves, and then significantly deceased after four days of water shortage in this mutant (Fig. 8A). In the
457
case of SOD activity, wild-type and abi1-1 leaves elevated SOD activity by 1.6 and 2.2 fold after four
458
days of drought treatment as compared to the control growth conditions whereas no alternation in the
459
enzyme activity was observed in drought-stressed cop1-4 mutant leaves (Fig. 8B).
460
Furthermore, anthocyanins are a large class of water-soluble pigments in the flavonoid group found in all
461
plant tissues, which can decrease leaf osmotic potential and operate as antioxidant in plants under abiotic
462
stresses (Rossel et al., 2007). Hence, to examine the effects of water deficiency on this non-enzymatic
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antioxidant level, especially in the cop1-4, anthocyanin content in wild-type and two mutants, cop1-4 and
464
abi1-1 leaves was measured. As shown in Fig. 8C, there was no significant difference in anthocyanin
465
content among wild-type, cop1-4, and abi1-1 plants under normal growth conditions, while soil water
466
deficiency gave rise to an excess production of anthocyanin in all plants. The anthocyanin level was
467
elevated by about 2.5 times in wild-type and cop1-4 leaves and 4 times in abi1-1 at the end of experiment
468
(fourth day of treatment). The more anthocyanin accumulation in abi1-1 leaves may implicate the severe
469
dehydration stress in the mutant.
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Fig.8. Enzymatic antioxidant activities
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level of CAT (A) and SOD (B) as well
473
as the non-enzymatic antioxidant level,
474
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anthocyanin (C) content, in cop1-4,
475
abi1-1 mutants, and wild-type leaves in
476
response to soil water stress. Data
477
represent the mean ± SD (n = 3). Means
478
followed by the same letter(s) are not
479
significantly different at 0.05 level of
480
484 485 486 487 488 489 490 491
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probability (DMRT).
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Gene expression analysis in cop1-4
493
Plant drought response is a complex biological process that needs to be surveyed at both physiological
494
and molecular levels. Here, to explore the effects of cop1 mutation on drought tolerance at the molecular
495
level, the expression profiling of several key stress-responsive genes, including MYB60, P5CS1, RD22,
496
KIN2, NCED3, and ABI1 was evaluated by qRT-PCR analysis in the wild-type and the two mutants’
16
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leaves, cop1-4 and abi1-1 under controlled and drought treatment conditions. Also, the COP1 expression
498
pattern was assessed in the plants under control, drought, salt and cold treatments as well as in the
499
presence and the absence of light. Furthermore, considering the fact that the cop1-4 stomata are
500
constitutively open in darkness (Mao et al., 2005) and AtMYB61 plays a major role in dark-induced
501
stomatal closure (Liang et al., 2005), the expression pattern of AtMYB61 was monitored in wild-type and
502
cop1-4 under light and darkness.
503
Based on the expression analysis of AtMYB60 gene, the transcript level of AtMYB60 was significantly
504
decreased after two days of drought treatment in the wild-type and cop1-4 leaves. The reduced gene
505
expression pattern was retained until the fourth day of treatment, when wild-type and cop1-4 leaves
506
accumulated the lowest level of AtMYB60 transcript, so that there was about 4 folds reduction in gene
507
expression at this time. As compared with wild-type and cop1-4 mutant, the gene expression was
508
diminished with a delay of two days, after four days of desiccation in abi1-1 mutant (Fig. 9A). Given that
509
the AtMYB60 function in the drought-induced stomatal closure, our results are consistent with the
510
stomatal behaviour at the stressed plants and illustrated that cop1-4 whole plant can lessen their stomatal
511
aperture via the reduced AtMYB60 transcript level in response to soil water limiting conditions.
512
In regards to stress-responsive genes, the wild-type as well as the mutants, cop1-4 and abi1-1 exhibited
513
elevated levels of KIN2, RD22, and P5CS1 under dehydration treatment compared with normal growth
514
conditions. But, interestingly, the up-regulation level of the genes was significantly lower in cop1-4
515
leaves than wild-type under drought treatment compared to normal growth conditions as illustrated in
516
Figs. 9B-9D
517
As ABA plays a fundamental role in the stress signalling pathway, leading to plant adaptation to adverse
518
growth conditions, the mRNA level of NCED3 and ABI1 genes involved in ABA biosynthesis and signal
519
transduction pathways, respectively, were assessed during drought treatment. As presented in Figs.9E and
520
9F, the transcripts abundance had no difference between wild-type and cop1-4 mutant under normal
521
growth conditions. However, the enhanced transcript level of NCED3 and ABI1 were observed in wild-
522
type, cop1-4 and abi1-1 after two days of desiccation. The induction of these genes in cop1-4 mutant can
523
suggest that this mutant is not deficient in ABA-related pathways.
525 526
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Fig. 9. Relative expression level of MYB60, KIN2, RD22, P5C1, NCED3 and ABI1 (A-F) in cop1-4, abi1-
529
1 mutants and wild-type leaves in response to soil water limiting conditions. Data represent the mean ±
530
SD (n = 3). Means followed by the same letter(s) are not significantly different at 0.05 level of probability
531
(DMRT).
532
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To elucidate the potential involvement of COP1 gene in plant abiotic stresses response, we evaluated its
534
expression under drought, salinity, and cold stresses. Our results, surprisingly demonstrated that COP1
535
expression was strongly induced by the applied stresses in wild-type and abi1-1 leaves, but not
536
significantly in the cop1-4 (Fig. 10). As illustrated in Fig. 10, in contrast to cop1-4 mutant, the COP1
537
transcript was accumulated in wild-type and abi1-1 leaves after two days of drought treatment until the
538
end of experiment (Fig. 10). Similarly, the same trend was detected in response to salt and cold stresses
539
(Fig. 10). As Fig. 10 displays, wild-type and abi1-1 mutant exhibited the elevated COP1 transcript level
540
after one day salinity treatment until five days of treatment while cop1-4 mutant accumulated this
541
transcript after three days of salt stress, however, the transcript abundance in cop1-4 leaves was
542
significantly lower than wild-type (Fig. 10). In the case of cold stress, while the COP1 transcript level
543
was notably increased in the wild-type and abi1-1 mutant at 4°C and -7°C, the transcript abundance was
544
approximately remained constant in cop1-4 leaves (Fig. 10).
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546 547
Fig. 10. Relative expression level of COP1 in cop1-4, abi1-1 mutants and wild-type leaves in response to
548
drought, salt, and cold stresses. Data represent the mean ± SD (n = 3). Means followed by the same
549
letter(s) are not significantly different at 0.05 level of probability (DMRT).
550
Earlier studies revealed that the stomatal aperture of cop1-4 mutant was much larger than wild-type and
552
our findings determined that the mutant was extremely sensitive to leaf detachment-imposed dehydration
553
(Fig. 1). With this information in mind, we assessed the expression level of NCED3 and COP1 genes in
554
detached leaves of wild-type and cop1-4 mutant at 10, 20, and 30 minutes after leaf detachment. As
555
shown in Figs. 11A and 11B, NCED3 and COP1 transcript accumulation were significantly induced in
556
both wild-type and cop1-4 leaves within 20 and 30 min after leaf detachment, respectively, implicating
557
that similar to NCED3, the COP1 could be an early-responsive gene. This broad responsiveness of COP1
558
to various types of abiotic stresses suggests it may be a component of plant abiotic stress response.
560 561 562 563
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566 567
Fig. 11. Relative expression levels of
568
NCED3 (A) and (B) COP1 (B) in
569
cop1-4
570
response to short-term dehydration
571
imposed by leaf detachment. Data
572
represent the mean ± SD (n = 3).
573
Means followed by the same letter(s)
574
are not significantly different at 0.05
575
level of probability (DMRT).
wild-type
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576
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577 578 579 580 581 582
We also investigated the probable effect of cop1 mutation on the steady-state mRNA level of AtMYB61 in
584
the presence and absence of light. Surprisingly, wild-type and cop1-4 plants showed the opposite
585
expression pattern. As Fig. 12A illustrates, in contrast to cop1-4, the transcript abundance of AtMYB61 is
586
significantly higher in the darkness than the light presence in wild-type plants. Similarly, the expression
587
analysis of COP1 demonstrated that both wild-type and cop1-4 displayed the decreased transcript
588
abundance in darkness when compared to the presence of light, but the reduction level was much higher
589
(11 folds) in cop1-4 than wild-type in darkness (Fig. 12B). Our results can infer that COP1 expression in
590
darkness is required for the expression of AtMYB61 that is essential for dark-induced stomatal closure.
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597 Fig.12. Relative expression levels of
599
MYB61 (A) and COP1 (B) in cop1-4
600
and wild-type leaves in the presence
601
and absence of light. Data represent
602
the mean ± SD (n = 3). Means
603
followed by the same letter(s) are not
604
significantly different at 0.05 level of
605
probability (DMRT).
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608 609 610 611 612 613 614 Promoter analysis
616
The gene expression induction or suppression under various developmental and environmental conditions
617
is mainly regulated via gene promoters and their cis-acting elements (Hernandez-Garcia and Finer, 2014).
618
In the current study, the altered expression pattern of COP1 gene in response to various abiotic stresses
619
prompted us to survey its promoter region for the probable stress-related cis-acting elements and the
620
corresponding transcription factors. The survey of 1 kb upstream sequences from translational initiation
621
codon of COP1 revealed the presence of multiple stress-associated cis-acting elements, including 3
622
abscisic acid-responsive elements (ABRE), 16 ABRE-like sequence required for etiolation-induced
623
expression of ERD1 (early response to dehydration 1) and 2 dehydration response element (DRE) in the
624
promoter region (Supplementary file S1). In addition, one salt-tolerance zinc finger protein binding site,
625
12 MYB recognition sites, one binding site for cold-regulated protein 15a (COR15a), and 20 heat shock
626
transcription factor (HSF) binding sites were detected in the COP1 promoter. The results implied that
627
COP1 is an abiotic stress-responsive gene that whose expression regulated in both ABA-dependent and
628
ABA-independent pathways. It is consistent with the altered COP1 expression level in response to
629
drought, salt, and cold stresses in both wild-type and abi1 mutant. Furthermore, in order to get insight into
630
the function of associated transcription factors (TFs) to COP1 promoter, all identified TFs were subjected
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to singular enrichment analysis embedded in AgriGO. Based on the analysis, several gene ontology (GO)
632
terms related to abiotic stresses including, response to stress (GO:0006950), response to abiotic stimulus
633
(GO:0009628), response to water deprivation (GO:0009414), response to abscisic acid stimulus
634
(GO:0009737), abscisic acid mediated signaling pathway (GO:0009738), response to salt stress
635
(GO:0009651), response to cold (GO:0009409), cellular response to heat (GO:0034605), response to
636
osmotic stress (GO:0006970), response to hydrogen peroxide (GO:0042542), and hyperosmotic salinity
637
response (GO:0042538) were significantly enriched (FDR < 0.01), which further support the COP1
638
function under various stresses. The complete list of significantly enriched GO term is presented in
639
Supplementary file S2.
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640 641 Discussion
643
Understanding the drought signal transduction pathway and the consequent plant response to reduce the
644
detrimental effects of water scarcity has continued to be one of the main objectives for scientists
645
(Obidiegwu et al., 2015; Pinheiro and Chaves, 2010). Drought stress response was extensively studied
646
in various plants, especially in Arabidopsis (Oh et al., 2005; Todaka et al., 2015; Wang et al., 2008). The
647
current study as the first attempt to uncover the different attributes of cop1-4 as well as lip1 mutants in
648
response to drought stress added the novel and main player, COP1, to drought signalling pathway. The
649
COP1 importance in plant drought response is related to its pivotal roles in developing stomata and
650
regulating stomatal movements (Mao et al., 2005). Stomatal closure is an early and rapid plant reaction to
651
water deficiency that is regulated through a complex network of signalling pathways (Merilo et al., 2015).
652
Here, we found that the lip1 stomatal apertures, like cop1-4, are significantly larger than wild-type under
653
normal growth conditions. It suggests that the COP1 function in the regulation of stomatal pore size is
654
conserved during evolution, in both Arabidopsis and pea. Interestingly, we discovered that contrary to
655
wild-type, the cop1-4 and lip1 detached leaves failed to decrease their stomatal aperture in response to
656
leaf detachment imposed dehydration, accounting for up to 50% of water loss during only 30 and 90
657
minutes after leaf excising in cop1-4 and lip1, respectively. It suggested that the COP1 plays a prominent
658
role in the sense and the rapid stomata response to short-term dehydration in the detached leaves in both
659
Arabidopsis and pea.
660
Guard cell ABA signaling is important for regulating basal stomatal openness and rapid stomatal
661
responses to environmental stimuli (Merilo et al., 2015). However, the appropriate hormone functioning
662
relies on the proper level of biologically active ABA, correlating with several processes including, ABA
663
biosynthesis, catabolism, conjugation, deconjugation, transport, and perception (Daszkowska-Golec and
664
Szarejko, 2013). Here, the sensitivity of cop1-4 detached leaves to exogenous ABA treatment after 120
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minutes, not after 40 minutes, implied that cop1-4 stomata is less sensitive to ABA than wild-type.
666
Similarly, Khanna et al (2014) reported that the stomata of GFP–TUA6,cop1-4 line resulted from
667
crossing GFP–TUA6 line with the cop1-4 mutant did not respond to 40 minutes treatment with 10 µM
668
ABA (Khanna et al., 2014). Although, ABA-mediated stomatal closure is not defective in the cop1-4
669
mutant, the delay in stomatal response to ABA may be long enough to induce rapid wilting in detached
670
leaves.
671
In Arabidopsis, ABA was synthesized mainly in leaves via the induction of NCED3 expression (Merilo et
672
al., 2015). NCED3 is considered to be the main regulatory enzyme, which its transcript up-regulated
673
within 15–30 min after leaf detachment or dehydration (Behnam et al., 2013; Xiong and Zhu, 2003).
674
Although, we could clearly detect the enhanced level of NCED3 transcript level within 20 minutes in both
675
wild-type and cop1-4 detached leaves, the cop1-4 stomata remained open, unlike wild-type. It can
676
propose that the accumulation of NCED3 transcript and the subsequent ABA biosynthesis appear to occur
677
normally in cop1-4 mutant; however, it is not sufficient for rapid stomatal closure in response to short-
678
term dehydration.
679
Unexpectedly, cop1-4 and lip1 whole plants were not as sensitive as the detached leaves to drought
680
treatment as they exhibited the decreased stomatal apertures accompanied by the similar level of RWC
681
between the mutant and wild-type during soil water deficient. This discrepancy highlights the root-shoot
682
signalling role in plant stress response. Contrary to detached leaves, as stress was imposed gradually on
683
the intact plants and the root-shoot signalling precede the ABA-induced stomatal closure, the ABA
684
concentration and time is enough to induce stomatal closure in the mutants as wild-type. Christmann et al
685
(2007) reported soil water stress generates a hydraulic signal in the shoot, which acts upstream of ABA
686
signalling and stomatal closure; however, both hydraulic signal and ABA is required for stomatal closure
687
in response to water stress. Another study by Pantin et al (2013) showed that ABA has two effects on
688
stomata: a direct biochemical effect on the guard cells and an indirect hydraulic impact by reducing leaf
689
water permeability triggered within vascular tissues. Under drought stress, ABA concentration rises in the
690
vascular parenchyma as a result of importing root-derived ABA and locally synthesized ABA. ABA
691
signalling in the bundle sheath by inactivating bundle sheath aquaporins (PIP) resulted in the reduced leaf
692
hydraulic conductance. Vascular ABA then transfers to the guard cells and promotes stomatal closure
693
(Pantin et al., 2013). Overall, our findings can suggest that the COP1 plays an important but a transient
694
role in initiating the rapid stomatal response to short-term dehydration and this role was evolutionary
695
conserved in both Arabidopsis and Pea.
696
Moreover, surveying the adaxial and abaxial stomatal density of wild-type and cop1-4 mutant under
697
control growth conditions and soil drought treatment revealed that there is no significant difference in
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stomatal density between wild-type and mutant. The similar results reported by previous studies
699
(Balcerowicz et al., 2014; Kang et al., 2009).
700
Although the stomatal aperture of cop1-4 was much wider than wild-type, both wild-type and cop1-4
701
displayed the similar level of RWC under normal growth conditions. As RWC implies the balance
702
between transpiration rate and water reservation, it indicated that cop1-4 mutant is able to conserve leaf
703
water probably via an efficient osmo-regulation system. It has been shown that proline accumulation
704
resulted in lowered cell osmotic potential and facilitated the cell turgor pressure maintenance (Hayat et
705
al., 2012). In line with this report, we found that cop1-4 leaves significantly contained more proline level
706
than wild-type under well-watered conditions. Therefore, the proline accumulation may be the essential
707
factor for compensating the increased water loss via the wide stomatal aperture and maintaining relative
708
leaf water content in cop1-4 mutants as wild-type plants.
709
The enhanced proline content as a common phenomenon in the stressed plants has also been widely
710
described; it is important not only for osmoregulation, but also for protecting cells by enhancing the
711
protein and cell membrane stability (Bhaskara et al., 2015; Estrada-Melo et al., 2015; Szabados and
712
Savouré, 2010). In the present study, while the increased content of proline was detected in wild-type and
713
abi1-1 after two days of drought stress, cop1-4 significantly accumulated this osmolyte after four days of
714
desiccation. It appears that the high constitutive levels of proline in cop1-4 can protect cell against the
715
detrimental effects of stress without additional proline enhancement until mutant exposed to longer
716
treatment periods or more severe stress, leading to further proline accumulation. The similar situation has
717
been also described in a drought-tolerant citrus genotype (Zandalinas et al., 2016).
718
Plants suffering from various stresses, including water deficiency often exhibit oxidative stress symptoms
719
as evidenced by the elevated reactive oxygen species and MDA levels (Das and Roychoudhury, 2014).
720
Compared with other ROS, H2O2 is a relatively long-lived molecule that is able to diffuse across cell
721
membranes. This characteristic is compatible with its role as a signalling molecule during growth and
722
stress plant response (Sharma et al., 2012). However, the high concentration of H2O2 can be a sign of
723
undesirable situation and extremely harmful for organism survival. Here, H2O2 and MDA content were
724
presented the positive association as also described by previous studies (Murshed et al., 2013; Ren et al.,
725
2016). In contrast to cop1-4 leaves, both H2O2 and MDA level were significantly incremented in wild-
726
type and abi1-1 under drought treatment. It implicated that cop1-4 mutant did not undergo the detectable
727
oxidative damage resulting from applied drought stress.
728
Enzymatic and non-enzymatic antioxidants are considered as an efficient defence system to cope with
729
excessive ROS and ameliorate the oxidative damage level. Among the enzymatic antioxidants, SOD acts
730
as one of the central and preliminary antioxidants by converting O2.− into H2O2 and maintaining the
731
intracellular O2.− within normal range (Das and Roychoudhury, 2014). In consistent with previous studies
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in Arabidopsis (Jung, 2004) and rubber tree (Wang, 2014), SOD activity was enhanced in wild-type and
733
abi1-1 leaves during drought stress while no significant change was detected in cop1-4 mutants, it is
734
probably due to either superoxide radical levels was not as high as for SOD activation in the mutant or the
735
non-enzymatic antioxidants such as anthocyanin play a main role in these conditions. Similarly, the lack
736
of significant CAT activity enhancement in cop1-4 can refer to the low level of H2O2 in the mutant as
737
reported that catalase breaks down high concentration of H2O2 because of its low affinity (high Km) for
738
this substrate (Mhamdi et al., 2010). It has been demonstrated that environmental stresses cause either
739
enhancement or depletion of CAT activity, depending on the intensity, duration, and type of the stress
740
(Janiak et al., 2015). Therefore, the drought-induced reductions in CAT activities in abi1-1 leaves may be
741
as a result of sever oxidative stress as also evidenced by the increased H2O2 and MDA levels. Overall, the
742
antioxidants activity was in accordance to H2O2 and MDA content during drought stress and may confirm
743
that oxidative damage level in cop1-4 and abi1-1 leaves is lower and higher than wild-type leaves,
744
respectively.
745
Many drought-inducible genes with various functions respond to water deficiency at the transcriptional
746
level. K1N2, RD22, and COR15a are of key stress-responsive genes encode the variety of LEA and like-
747
LEA proteins that are able to act as chaperones to stabilize proteins and membrane structure in the
748
stressed plants to confer cellular tolerance to dehydration (Goyal et al., 2005; Janiak et al., 2015). Based
749
on our results, the expression of these genes were induced in leaves of wild-type and two mutants, cop1-4
750
and abi1-1 in response to water deficiency; however, their expression levels in cop1-4 leaves were not as
751
high as wild-type, hence the improved drought tolerance of cop1-4 whole plant might not be correlated
752
with these genes. The expression of stress-inducible genes is regulated by the ABA-dependent and ABA-
753
independent pathways (Joshi et al., 2016). A similar expression pattern of the above-mentioned genes in
754
abi1-1 mutant in our study indicated that their induction is ABA-independent, as previous studies have
755
been also reported (Jensen et al., 1996).
756
There are two closely related P5CS genes in Arabidopsis that mainly P5CS1 expression is promoted by
757
drought and salt stresses (Ben Rejeb et al., 2015; Székely et al., 2008). In agreement with previous
758
researches, the increased steady state level of P5CS1 mRNA was detected in the drought stressed plants.
759
While the proline content of cop1-4 leaves was significantly higher than wild-type under normal growth
760
conditions, the P5CS1 transcript accumulation had not been followed the same pattern. It can refer to the
761
proline feedback inhibition effect as previous studies was also reported that proline biosynthesis in plants
762
primarily regulated at the transcriptional level by end product (Porcel et al., 2004; Sharma and Verslues,
763
2010). Although the role of ABA in regulating proline accumulation requires further examination due to
764
contradictory data obtained in various species by different researchers (Guan et al., 2014; Verslues and
765
Bray, 2005), we could clearly observed the enhanced P5CS1 transcript and proline levels in abi1-1
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mutant leaves, suggesting that no ABA involvement is required for proline accumulation or drought-
767
induced P5CS1 is regulated by both ABA-dependent and ABA-independent pathways.
768
In Arabidopsis genome, at least nine genes are identified to code NCED that among them NCED3 showed
769
higher expression in both roots and shoots in response to drought stress (Rasheed et al., 2016). Similarly,
770
we found the elevated NCED3 expression in wild-type and two mutants, cop1-4 and abi1-1 leaves under
771
water limiting conditions. Hence, the mutation in COP1 gene does not interfere with ABA biosynthesis
772
pathway at least at the transcription level. Further, Barrero et al revealed that there is a positive
773
correlation between the enhanced NCED3 transcript level and ABA content (Barrero et al., 2006). Thus,
774
the cop1-4 mutant can produce enough ABA, which facilitates the stomatal closure as evidenced by the
775
reduced stomatal pores in cop1-4 whole plant in response to soil water deficiency. Besides the
776
environmental signals, Arabidopsis stomatal aperture was modulated by several transcription factors,
777
including AtMYB60 and AtMYB61. Here, we found that the steady-state level of AtMYB60 was reduced in
778
wild-type, cop1-4, and abi1-1 leaves. The AtMYB60 response in abi1-1 refers to the presence of cis-acting
779
elements responsible for down-regulating gene expression in response to dehydration in an ABA-
780
independent manner (Rusconi et al., 2013). However, abi1-1 could not able to close their stomata in
781
response to water shortage conditions, it may propose that the ABA-independent pathway mediated
782
AtMYB60 down-regulation is not enough for drought-induced stomatal closure. The down-regulated
783
AtMYB60 was in line with decreased stomatal pore in wild-type as reported by previous report (Cominelli
784
et al., 2005) as well as cop1-4 leaves in response to soil water deficiency. Consequently, the diminished
785
stomatal aperture in the stressed cop1-4 whole plant could be resulted from the reduced AtMYB60
786
transcript level.
787
AtMYB61 is a pleiotropic regulator of plant stomatal aperture, lateral root formation, and xylem cell
788
differentiation. It has suggested that this gene has an active role for stomatal opening inhibition in
789
darkness (Baldoni et al., 2015). Here, we figured out cop1-4 leaves accumulated AtMYB61 and COP1 in
790
much lower than wild-type in darkness. Considering that stomatal closure was impaired in the cop1-4
791
leaves in darkness and COP1 expression can complement the constitutive stomatal opening phenotype in
792
this mutant (Mao et al., 2005), our findings can uncover that the expression of both COP1 and AtMYB61
793
may essential for the reduced stomatal pores in darkness and AtMYB61 might play a key role on the
794
downstream of COP1 for promoting darkness-induced stomatal closure.
795
Additionally, we deciphered that COP1 expression pattern can undergo by various abiotic stresses
796
(drought, salinity, and cold), offering the COP1 could be a stress-responsive gene. While COP1 transcript
797
abundance remained relatively constant in cop1-4 mutant, it was significantly up-regulated in wild-type
798
and abi1-1 mutant during abiotic stresses. The COP1 expression in abi1-1 mutant revealed that its
799
expression is regulated through both ABA-dependent and ABA-independent pathways in response to
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unfavourable conditions as also evidenced by the presence of both ABRE and DRE cis-acting elements in
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the COP1 promoter region. Similarly, the existence of several enriched ABA- and stress-related GO terms
802
among the biological functions of transcription factors associated to the COP1 promoter could further
803
confirm the altered gene expression pattern in response to applied various abiotic treatments.
804
Taken together, COP1 can act as a central regulator of abiotic stresses response pathway with diverse
805
roles in detached leaves and whole plant levels. The conserved function of COP1 in both Arabidopsis and
806
pea during evolution can emphasis its crucial importance. Our study adds a new level of complexity to the
807
overall understanding of main effectors required for stomatal closure as well as the root-shoot signalling
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pathway under drought stress. Further efforts are needed to resolve exactly how COP1 mediates plant
809
response to both short-term and long-term dehydration.
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Acknowledgements
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We are grateful to Prof. Xing-Wang Deng for providing cop1-4 seeds as well as Dr. William Thompson
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and Dr. Shannon Frances for providing lip1 seeds.
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Supporting information
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Supplementary file 2. List of significantly enriched GO terms associated with all transcriptions factors
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bind to COP1 promoter region.
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Supplementary file 1. List of stress-related cis-acting elements in COP1 promoter region.
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Highlights
2. COP1 is an abiotic stress-responsive gene in Arabidopsis.
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1. COP1 plays a fundamental role in the regulation of stomatal movements in response to dehydration in both Arabidopsis and Pea.
3. cop1-4 mutant stomata respond to short-term and long-term dehydration in a different manner in
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Arabidopsis.
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Author contributions M.M.J, S.GH, and S.M.S designed the research. M.M.J and S.GH carried out the experiment and analyzed the data. M.M.J wrote the manuscript. S.M.S and V.N supervised the project. All authors read
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and approved the manuscript.
S0981-9428(18)30353-X
DOI:
10.1016/j.plaphy.2018.08.015
Reference:
PLAPHY 5376
To appear in:
Plant Physiology and Biochemistry
Received Date: 5 July 2018 Accepted Date: 8 August 2018
Please cite this article as: M.M. Jazi, S. Ghasemi, S.M. Seyedi, V. Niknam, COP1 plays a prominent role in drought stress tolerance in Arabidopsis and pea, Plant Physiology et Biochemistry (2018), doi: 10.1016/j.plaphy.2018.08.015. 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.
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COP1 plays a prominent role in drought stress tolerance in Arabidopsis and Pea
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Maryam Moazzam Jazi1, Samaneh Ghasemi2, Seyed Mahdi Seyedi1*, Vahid Niknam2
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Biotechnology, Tehran, Iran
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Tehran, Iran
Plant
Biotechnology
Department,
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Correspondence: Seyed Mahdi Seyedi ([email protected])
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Department of Plant Biology, School of Biology, College of Sciences, Tehran University,
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Abstract
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Constitutively photomorphogenic 1(COP1) is an E3 ubiquitin ligase that has been studied extensively in
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the photomorphogenesis- and light-related processes in Arabidopsis. However, the possible role of COP1
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in plant drought stress response remains unknown. Hence, in the present study, the stomatal behavior as
33
one of the key elements in plant dehydration response was investigated in Arabidopsis cop1-4 and pea
34
light-independent photomorphogenesis (lip1) mutants. We observed that water loss rate in the cop1-4 and
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lip1 detached leaves were significantly much faster than wild-type, resulting from failing to reduce the
36
stomatal aperture by the mutants. But, interestingly, the cop1-4 and lip1 isolated leaves treated with
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abscisic acid (ABA) as well as cop1-4 soil-grown under drought stress could close their stomata as wild-
38
type. Hence, COP1 plays a fundamental role in the regulation of stomatal movements in response to
39
dehydration and its function was conserved during evolution in both Arabidopsis and pea. Further
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evaluations showed the cop1-4 mutant was not significantly damaged from the oxidative stress derived
41
from soil water limiting conditions when compared to wild-type. Similarly, the up-regulation level of
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several key stress-responsive genes was relatively lower in cop1-4 than wild-type. Therefore, COP1
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might be considered as a potential key regulator of both short-and long-term dehydration response.
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Multiple stress-related cis-elements were also detected in the COP1 promoter region, which supported its
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up-regulation in response to drought, salt, and cold stresses. Besides, we figured out the constitutively
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open stomata of cop1-4 in darkness can be as a result of the reduced AtMYB61 expression.
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Key words: Arabidopsis, COP1, Drought stress, Pea, Stomata, Water loss.
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Abbreviations
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ABA, abscisic acid; ABRE, abscisic acid-responsive elements; CAT, catalase; COP1, constitutively
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photomorphogenic 1; COR15a, cold-regulated protein 15a; CRT, cryptochromes; CTAB, cetyltrimethyl
55
ammonium bromide; DRE, dehydration response element; ERD1, early response to dehydration 1; FC,
56
field capacity; HSF, heat shock transcription factor; HY5, long hypocotyl 5; LIP, light-independent
57
photomorphogenesis; MDA, Malondialdehyde; PHOT, phototropins; PHYA, phytochrome A; PHYB,
58
phytochrome B; PVP, Polyvinylpyrrolidone; ROS, reactive oxygen species; RWC, relative water content;
59
SOD, superoxide dismutase; SUMO, Small ubiquitin-related modifier; TBA, thiobarbituric acid
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Introduction
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Water deficiency, as a result of climate change, is a major threat to supply global food resources for the
65
increasing population worldwide. Drought stress is considered as one of the most important limiting
66
factor for sustainable agriculture, particularly in arid and semi-arid areas, resulting in reduced crop yield
67
by more than 50% every year (Atkinson and Urwin, 2012; Singh et al., 2015). It is adversely affects the
68
plant growth, development, survival and productivity, hence the investigation of plant drought stress
69
responses has gained widespread attention over recent years. Plants have evolved specific defence
70
mechanisms in response to environmental stresses, including drought, which is characterized with a series
71
of morphological, physiological, biochemical, and molecular changes in stressed plants (Krishnan and
72
Pereira, 2008; Wang, 2014). Osmotic adjustment through the accumulation of compatible solutes, such as
73
proline is a prevalent physiological response in plants exposed to various abiotic stresses, such as drought,
74
salinity and cold (Krasensky and Jonak, 2012). Proline acts as an osmoprotectant, a molecular chaperone
75
stabilizing macromolecules, and reactive oxygen species (ROS) scavenger (Szabados and Savouré, 2010).
76
The glutamate-originated pathway appears to be the predominant proline biosynthesis pathway, especially
77
under stress conditions (Hayat et al., 2012).
78
Oxidative stress resulted from the extensive generation of ROS is an unavoidable aspect of different
79
stresses (Noctor et al., 2014). Under drought conditions, stress-induced stomatal closure and the restricted
80
CO2 uptake leads to the over-reduction of photosynthetic electron transport chain, favouring the electron
81
transfer to oxygen and producing various kinds of ROS in the chloroplasts (Harb et al., 2010; Noctor et
82
al., 2014). Although ROSs plays a key role in the signal transduction pathways at their steady-state level,
83
they can initiate destructive oxidative processes such as lipid peroxidation and chlorophyll bleaching in
84
the stressed plants (Miller et al., 2008; Sharma et al., 2012). Therefore, to scavenge ROS and alleviate the
85
oxidative damages, plants have developed a wide range of enzymatic and non-enzymatic antioxidants,
86
which superoxide dismutase (SOD) and catalase (CAT) comprised the primary enzymatic antioxidants.
87
Similarly, flavonoids, cartenoids and anthocyanin are the main non-enzymatic antioxidants, accumulating
88
in response to oxidative stress in most plant species (Sharma et al., 2012; You and Chan, 2015).
89
Principally, plant drought responses are modulated by multiple stress-responsive genes, like RD22 and
90
P5CS. The gene expression alternation ultimately promotes the cellular homeostasis, toxins detoxification
91
and growth recovery of stressed plants (Nuruzzaman et al., 2013). At least six independent systems
92
regulate gene expression in response to water deprivation in Arabidopsis, three of which are abscisic acid
93
(ABA)-independent and the other three are ABA-dependent (Yamaguchi-Shinozaki and Shinozaki, 2006;
94
Yoshida et al., 2014). Under water stress, the ABA-induced stomatal closure followed by reduced water
95
loss is one of the essential aspects of drought tolerance in plants, and it is considered as a drought
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avoidance mechanism (Basu et al., 2016; Buckley, 2005). Two R2R3-MYB transcription factors,
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AtMYB60 and AtMYB61, are the main regulators of stomatal movements. The AtMYB60 expression is
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induced by white and blue light and repressed by darkness and drought stress; hence the stomatal aperture
99
size is correlated with the AtMYB60 transcript level (Daszkowska-Golec and Szarejko, 2013). Contrary to
100
AtMYB60, darkness promotes the expression of AtMYB61, leading to decreased stomatal aperture while
101
other stomatal closuring signals, like ABA, salt and drought do not altered the AtMYB61 expression
102
pattern (Liang et al., 2005).
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Among environmental signals, light is a major factor in the reflection of various plant cell movements and
104
developmental processes including, stomatal movements, de-etiolation, and cotyledon opening (Ma et al.,
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2002). It has been revealed that phototropins (PHOT) and cryptochromes (CRY) are involved in blue
106
light-induced stomatal opening and that COP1, a negative regulator of photomorphogenesis, likely acts
107
downstream of CRY and PHOT signaling pathway to repress stomatal opening (Smirnova et al., 2012).
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COP1 is an E3 ubiquitin-ligase contributed to the degradation of photomorphogenic-related factors,
109
including long hypocotyl 5 (HY5), phytochrome A (PHYA), phytochrome B (PHYB) and cryptochrome
110
(CRY), resulting in photomorphogenesis repression (Jia et al., 2014; Osterlund et al., 2000).
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It has been proved that the occurrence of partial duplication within the pea homolog of COP1 give rise to
112
create lip1 mutant (Sullivan and Gray, 2000). The lip1 mutants showed light-grown development when
113
grown in darkness as they displayed short stems along with open and expanded shoots, like cop1-4
114
(Seyyedi et al., 1999; Stoop‐Myer et al., 1999). COP1 function has been well documented during
115
Arabidopsis developmental modifications in the presence and absence of light (Chang et al., 2011; Chen
116
et al., 2015; Subramanian et al., 2004). However, to the best of knowledge, there is no report elucidating
117
the involvement of COP1 in response to drought stress in Arabidopsis and pea. It was very recently
118
demonstrated that Small ubiquitin-related modifier (SUMO) conjugation mediated by AtSIZ1 negatively
119
regulated through the E3 ubiquitin-ligase activity of COP1 under abiotic stresses, thereby COP1 controls
120
Arabidopsis abiotic stresses response via the modulation of the AtSIZ1 level (Kim et al., 2016). However,
121
the impact of COP1 on the plant physiological and molecular responses under abiotic treatments was not
122
reported.
123
In the present study, wild-type (Col-0) and cop1-4 mutant of Arabidopsis (Arabidopsis thaliana) were
124
subjected to dehydration treatment at two levels, short-term and long term by detaching leaves and
125
stopping irrigation, respectively. In order to uncover the probable COP1 role in Arabidopsis drought
126
response, some of major physiological and molecular parameters were evaluated. We also used abi1-1
127
mutant, which is the drought-sensitive and ABA-insensitive plant as the control for the experiment.
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Furthermore, wild-type pea (Pisum sativum cv Alaska) and lip1 mutant were utilized to evaluate their
129
stomata response to short-term and long-term dehydration.
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Materials and Methods
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Plant growth conditions and abiotic treatments
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Arabidopsis (A. thaliana), ecotype Columbia (Col-0), cop1-4, and abi1-1 mutants as well as pea (P.
134
sativum cv Alaska) and lip1 mutant were used in this study. Surface-sterilized seeds were directly sown
135
on pots containing a mixture of perlite, vermiculite and peat and stratified at 4°C in dark for 2 days. The
136
seedlings were grown under controlled conditions at 22˚C and 70% relative humidity under long-day
137
conditions (16h/8h, light/dark cycle). Short-term dehydration was imposed by excising leaf and placing
138
on the laboratory bench at 23˚C and 27% relative humidity.
139
Long-term drought treatment was applied to four-week-old plants (Arabidopsis and pea) by water
140
withholding. The level of drought stress was gravimetrically checked (Ramegowda et al., 2013); briefly,
141
pots along with plants were weighed daily until the end of experiment. Control plants were maintained at
142
100% soil field capacity (FC). Upon the arrival of 75% FC (after 2 days) and 50% FC (after 4 days),
143
leaves were sampled. For salt treatment, Arabidopsis plants were hydroponically grown in Hoagland’s
144
nutrient solution with aeration, and the nutrient solution was renewed every three days. Four-week-old
145
plants were exposed to salt stress (200 mM) by adding NaCl to the solution and leaves were collected at
146
1, 3, and 5 days of salt application. For cold treatment, four-week-old soil-grown Arabidopsis plants were
147
transferred to a growth chamber with 4°C for 3 days (cold acclimation), then subjected to -7°C for 6
148
hours, followed by transferring to 4°C for one day. The leaves were collected after each step. For dark
149
treatment, four-week-old plants grown in soil were kept at darkness for 2 days, and then leaves sampled
150
under faint green light. In all cases, sampled leaves were frozen immediately in liquid nitrogen and stored
151
at -80°C until use. All experiments were conducted in three biological replicates.
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Leaf relative water content
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Relative water content (RWC) was calculated by the following formula: RWC = [(fresh mass - dry mass)
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/ (saturated mass - dry mass)] × 100.
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Water loss assay
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For transpirational water loss assay, leaves from several four-week-old plants were detached, so that the
159
leaves area of cop1-4 and lip1 mutants was similar to the corresponding wild-type. The leaves were
160
placed in the filter paper on a laboratory bench at 23°C and 27% relative humidity and weighted at
161
designated time intervals. The loss in fresh weight presented as the percentage of initial fresh weight at
162
each time point (Li et al., 2008).
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Stomatal aperture measurement
164
The abaxial epidermis was peeled from the leaves of multiple four-week-old plants under drought
165
treatment as well as normal growth conditions and the stomata were observed by light microscopy (Zeiss
166
) connected to a fitted camera. The stomatal pore width was measured using ProgRes Capture Pro 2.1
167
software. For ABA-induced stomatal closure assay, the leaves were floated in the opening buffer
168
containing 10 mM KCl, 10 mM CaCl2, and 10 mM MES, 0.01% Tween 20, pH 6.5 at 22°C for 2 hours to
169
open the stomata. Then, the leaves were transferred to the same buffer supplemented with 10 µmol ABA,
170
maintained in these conditions for 2 hours and the pore size was calculated (Tanaka et al., 2005).
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Stomatal density (i.e. the number of stomata per unit area) in both adaxial and abaxial leaf surface was
174
determined in the four-week-old plants. Ten random parts (each part consisted of 0.1 mm2) from four
175
leaves were counted for determination of stomatal density.
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Hydrogen peroxide and lipid peroxidation level measurement
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The H2O2 concentration was determined using the standard curve generated with known concentrations of
179
H2O2 as described by (Loreto and Velikova, 2001). Malondialdehyde (MDA) level as the main index of
180
lipid peroxidation was determined by the thiobarbituric acid (TBA) reaction according to Du and
181
Bramlage (Du and Bramlage, 1992). The MDA concentration was calculated using extinction coefficient
182
of absorbance 155 mM-1 cm-1.
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Proline content measurement
185
Proline content was determined via reaction with ninhydrin reagent (Magné and Larher, 1992). Briefly,
186
100 mg of fresh leaves was homogenized in 1.2 ml of 3% (w/v) aqueous sulphosalycylic acid and the
187
homogenate filtered. After adding 2 ml ninhydrin (1%, w/v) to the supernatant and incubating at 98°C for
188
one hour, the micro tubes were cooled and treated with 2 ml toluene. The absorbance of the upper phase
189
was spectrophotometrically assessed at 518 nm after. The proline concentration was calculated according
190
to a calibration curve.
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Enzymatic and non-enzymatic antioxidant assay
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For enzymatic antioxidant activity assay, 200 mg of fresh leaves was homogenized in 0.1 M Trise-HCl
194
buffer (pH 7.8) containing 1 mM EDTA and 4% Polyvinylpyrrolidone (PVP) at 4°C. The resulting
195
supernatant was used for enzyme assays. Proteins were quantified according to Bradford (Bradford, 1976)
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using albumin bovine serum as a standard. The per unit SOD activity was estimated by adding 40 µl of
197
the enzymatic extract to a solution containing 13 mM methionine, 75 µM p-nitroblue tetrazolium chloride
198
(NBT), 100 µM EDTA and 2 µM riboflavin in a 50 mm potassium phosphate buffer pH 7.5. The reaction
199
started with 10 min illumination under a 30 W fluorescent lamp and stopped by turning light off. Non-
200
illuminated and illuminated reactions without supernatant served as calibration standards, and the final
201
reaction products were measured at 560 nm (Dhindsa et al., 1981).
202
The CAT activity was assessed following the modified method by measuring the decrease in absorbance
203
at 240 nm of the reaction mixture with a final volume of 2 ml containing 15 mM H2O2 in 50 mM K-
204
phosphate buffer (pH 7.0) and 10 µL extract (Aebi, 1984).
205
As the non-enzymatic antioxidant, the anthocyanin level was measured by homogenising leaves (50 mg)
206
in acidic methanol (99:1, v/v) and recording the absorbance of the supernatant at 530 and 657 nm (Laby et
207
al., 2000). The anthocyanin content expressed as follows:
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Relative units of anthocyanin/g fresh weight of tissue = OD530 - (0.25×OD657) × extraction volume (ml)
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× 1 / weight of tissue sample (g).
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Total RNA isolation and gene expression analysis
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Total RNA was extracted from 200 mg of leaves using a modified CTAB (cetyltrimethyl ammonium
213
bromide) method (Moazzam-Jazi et al., 2015). After the treatment of extracted RNA with RNase free
214
DNase I (Fermentas), single-stranded cDNA was synthesized from total RNA according to the
215
manufacturer’s instructions (RevertAid First Strand cDNA Synthesis Kit, Fermentas). Real-time PCR was
216
performed using the SYBR Green Real-time PCR master mix (Ampliqon, Denmark). The reaction
217
mixture contained 1 µL of cDNA sample, 0.5 µL of each the forward and reverse primers (10 µM) and 10
218
µL real-time master mix with a final volume of 20 µL. The cycling conditions were set as follows, initial
219
activation of DNA polymerase at 95°C for 15 min, followed by 40 cycles 94°C for 30s, 58-60°C for 30s
220
and 72°C for 30s for all genes except for P5CS1 that was 90s. The relative gene expressions of KIN2,
221
P5CS1, RD22, NCED3, ABI1, MYB60, and COP1 were analysed by Pfaffl formula (Pfaffl, 2001) within
222
REST 2009 software. Also, APK2a was used as the internal control. All samples were amplified in
223
triplicate. The primer sequences are available in Table 1.
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Table1. Primer pairs were used for gene expression analysis Gene name
Gene Identifier
Forward primer sequence 5´-3´
APK2a
NM_101304.4
GGAGAGATACTTTCATCGCCTAA CC
GACCTGCTTTTGCCAATCCG
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KIN2
NM_121602.4
CAAAACACACATCAAAAACG
AACATTGCTCTTCTCCTCAG
58
RD22
NM_122472.4
CACAAGGGAAGACCGATTTAC
TTCTCCTCTCCACTAACTTTTC TG
58
P5CS1
NM_001202785.1
GTCATTTTGGTGTCATCTGGTGC
CATCAAGCTGGTCAAACATAG TC
60
NCED3
NM_112304.3
TCCAGCTCTTCATTTCCCTAA
CGGCCATTGAAATAGACCAA
58
ABI1
NM_118741.3
GATATCTCCGCCGGAGATGAGAT C
CATTCCACTGAATCACTTTTC CTC
58
MYB60
NM_100755.3
GGACCATGGACTCCTGAAGA
CCACGTTTAATTCCAGGTCT
58
COP1
NM_128855.4
TTGTTCCAGCGGTGAAACCT
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Tm (ºC)
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Reverse primer sequence 5´-3´
CAGATCCGGTGCTCCAATCT
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Promoter analysis
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The 1 kb upstream sequence from the translational initiation codon of COP1 in A. thaliana was obtained.
235
In order to assess the transcription factor binding sites within the promoter region, the sequence was
236
analysed using the web-based tool, “The Plant Promoter Analysis Navigator (PlantPAN 2.0;
237
http://PlantPAN2.itps.ncku.edu.tw).” This tool provides resources for detecting cis-regulatory elements
238
and the corresponding transcription factors in a gene promoter (Chow et al., 2016). The biological
239
function
240
(http://bioinfo.cau.edu.cn/agriGO/) via the singular enrichment analysis tool. The analysis was conducted
241
with Fisher’s exact test and FDR cutoff of 0.05 was considered for significance.
all
transcription
factors
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recognized
was
determined
using
AgriGO
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Statistical analysis
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A completely randomized design with three biological replicates was considered and all physiologic data
246
analyzed using SPSS software (version of 22). The mean comparison was performed by Duncan's
247
Multiple Range Test (DMRT) at the 0.05 level of confidence.
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Results
253
The contrasting response of cop1-4 stomata to dehydration
254
One of the earliest plant responses to drought stress is the restriction of transpirational water loss through
255
stomatal closure. Previous studies revealed that the COP1 possess the regulatory role in the stomatal
256
movements (Mao et al., 2005). With this information in mind, the sensitivity of cop1-4 mutant leaves to
257
short-term dehydration was examined by leaf detachment. We measured the water loss rate of wild-type
258
and cop1-4 leaves after incubation at 22°C in the light. Based on our results, the weight of detached
259
leaves reached to the half of initial weight in the wild type and cop1-4 mutant after 180 and 30 minutes of
260
leaf detachment, respectively (Fig. 1), implying that the water loss rate in the mutant leaves was much
261
faster than the wild type and responsible for the appearance of wilt symptoms in the mutant.
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Fig.1. Rate of leaf water loss in cop1-4 mutant and wild-type during short-term dehydration. Water loss
265
rate is expressed as the percentage of initial fresh weight. Each data point is presented as the mean ± SD
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(n=3).
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Considering the water loss assay and the central role of stomata in the modulation of transpiration rate, we
269
estimated the stomatal aperture of leaves under control conditions and 10, 20, and 30 minutes after leaf
270
detachment. We observed that the stomatal aperture of cop1-4 leaves was much larger than wild-type
271
under normal growth conditions; the average stomatal aperture of 200 stomata was 2.8 µm in the wild-
272
type while it was 6.3 µm in cop1-4 (Fig. 2). The wild-type stomata started to close after 20 minutes of leaf
273
detachment and their average aperture reached to 1.5 µm, but, interestingly, the cop1-4 stomata remained
274
open in the same conditions (Fig. 2A).
275
Considering the key role of ABA in the coordination of stomatal conductance with the plant water supply
276
(Aasamaa and Sõber, 2011), we incubated leaves with exogenous ABA (10 µmol) for 40 and 120 minutes
277
to explore whether ABA treatment induces a change on the stomatal aperture of cop1-4. Following the
278
assessment of stomata status, we found that the cop1-4 stomata were sensitive to ABA and their stomatal
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pores reduced in response to exogenous ABA as the wild-type plants only after 120 minutes. As
280
illustrated in Fig. 2B, the average stomatal aperture of wild-type and cop1-4 leaves from 2.6 and 5.4 µm
281
before ABA application, respectively, were decreased to 1.2 and 2.5 µm in response to ABA treatment for
282
120 minutes (Fig. 2B), suggesting that the cop1-4 stomata is not defective in ABA-mediated stomatal
283
closure, but they are less sensitive to ABA than wild-type.
284
As our results demonstrated, the cop1-4 mutant is defective to sense the leaf detachment-imposed
285
dehydration and reduces their stomatal aperture. Consequently, we speculated that it may result in the
286
enhanced drought sensitivity at the whole plant, too. To address this possibility, wild-type and cop1-4
287
mutant were planted in the soil and four-week-old plants subjected to drought treatment by withholding
288
water. After the stomata status evaluation, surprisingly, we found out that the stomatal behaviour was
289
similar in both with-type and mutant in response to soil water deficiency. As shown in Fig. 2C, the
290
stomatal aperture average significantly decreased in the stressed plants, it was reached to 1.7 µm and 2.54
291
µm from 3 µm and 6.5 µm in the wild type and cop1-4 leaves, respectively, after four days of drought
292
stress (Fig. 2C).
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Fig.2. Stomatal apertures of cop1-4
295
mutant and wild-type leave. (A) The
296
300 301 302 303 304 305 306 307 308
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conditions and short-term dehydration imposed by leaf detachment. (B) The cop1-4 mutant and wild-type stomata response to the leaf treatment with 10
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stomatal aperture under normal growth
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µmol ABA. (C) The cop1-4 mutant and wild-type stomatal aperture in response
to
soil
water
shortage
conditions. Data are the average stomatal aperture of 200 stomata. Means followed by the same letter(s) are not significantly different at 0.05 level of probability (DMRT).
309 310 311 312 10
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A representative illustration of open and closed stomata of cop1-4 and wild-type was shown in Fig. 3.
314 315 316 317 318 319 320 321 322 323 324 325 326 327 328
Fig.3. Representative image of open
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Wild-type, closed. (C) cop1-4, open.
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(4) cop1-4, closed.
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Furthermore, we investigated the adaxial and abaxial stomatal density of wild-type and cop1-4 mutant
332
under control growth conditions (Fig. 4 A). As Fig. 4 showed, there is no significant difference in the
333
number of stomata per unit of leaf area between wild-type and cop1-4 under normal growth conditions.
334
Surveying the abaxial stomatal density in plants under soil drought stress revealed that this parameter has
335
remained constant after 2 and 4 days of drought stress in both wild-type and cop1-4 (Fig. 4B).
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Fig.4 Adexial and abexial stomatal density of wild-type and cop1-4 mutant under normal growth
339
conditions (A) and the abexial stomatal density of wild-type and cop1-4 mutant under soil drought stress
340
(B). Data are the average stomatal density of 120 stomata.
341 342
Interestingly, we observed that cop1-4 mutants soil-grown were more tolerant to drought stress than wild-
343
type under our experimental conditions (Fig.5).
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344 345
Fig.5. Phenotypic picture of plants
346 347
under normal growth conditions (A)
348
treatment (B), imposed by withholding
349
water.
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and after 4 days of soil drought
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The lip1 stomata contrasting response to dehydration and ABA treatment
360
As LIP1 in pea is ortholog for COP1 and the lip1 mutant exhibits the similar characteristics to cop1-4
361
(Sullivan and Gray, 2000), we were curious to assess its stomatal behaviour in response to dehydration as
362
well as exogenous ABA treatment. Interestingly, we found a resemblance in stomatal response between
363
cop1-4 and lip1 mutants under our experimental conditions. Water loss assay showed that the lip1
364
detached leaves weight attained to the half of initial weight after 40 minutes while wild-type isolated
365
leaves required 10.5 hours to reach the same weight, implying that lip1 fails to close its stomata in
366
response to short-term dehydration as cop1-4 (Fig. 6A).
367
The lip1 stomata are significantly wider than wild-type under normal growth conditions similar to those
368
of cop1-4. Based on our microscopic measurements, the average stomatal aperture is 4.2 and 6.5 µm in
369
wild-type and lip1 mutant, respectively (Fig. 6B). But, the treatment of detached leaves with 10 µmol
370
ABA for 120 minutes resulted in a reduced stomatal pores in both wild-type and lip1 mutant, so that the
371
stomatal aperture of wild-type and lip1 decreased to 2.9 and 3.5 µm in response to ABA treatment.
372
Therefore, neither cop1-4 nor lip1 appear impaired in the ABA-induced stomatal closure (Fig. 6B). Our
373
findings suggested that COP1 can play an essential role in regulating the stomatal movements in both
374
Arabidopsis and pea.
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Fig.6. lip1 mutant and wild-type
376
stomatal behaviour. (A) lip1 mutant
377
and wild-type stomatal behaviour in
378
response to short-term dehydration as
379
evidenced by leaf water loss assay.
380
Water loss rate is expressed as the
381
percentage of initial fresh weight.
382
Each data point is presented as the
383
mean ± SD (n=3). (B) The lip1 mutant
384
and wild-type stomata response to the
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leaf treatment with 10 µmol ABA. (C)
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387
after 2 and 4 days of drought stress.
388
Data are the average stomatal aperture
389
of 200 stomata. Means followed by
390
the same letter(s) are not significantly
391
different at 0.05 level of probability
392
(DMRT).
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Furthermore, drought treatment was applied on the soil-grown pea lip1 mutant and wild-type by water
399
withholding and the stomatal behaviour surveyed after 2 and 4 days of soil drought stress. Interestingly,
400
we observed that lip1 stomatal aperture decreased in response to soil water shortage as wild-type (Fig.
401
6C). As Fig. 6C showed, the average of stomatal aperture reduced to 4.3 µm and 2.8 µm from 6.1 µm and
402
4.3 µm in lip1 mutant and wild-type, respectively, after 4 days of drought stress.
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Evaluation of main physiological parameters related to drought stress in cop1-4
405 406
RWC content
407
RWC is an important index of plant water status and reflects the balance between the water supply and
408
transpiration rate. Hence, in order to estimate the whole plant transpiration under drought stress, we
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examined the RWC level of wild-type and cop1-4 plants after two and four days of the cessation of
410
irrigation. Based on the results, there was no difference between wild-type and cop1-4 mutant in the RWC
411
content during drought treatment, the RWC of both wild-type and cop1-4 plants significantly diminished
412
after two days of drought stress (Fig. 7A). The similarity in the level of RWC under soil water shortage
413
conditions further support that in contrast to cop1-4 detached leaves, the cop1-4 whole plant could limit
414
the transpirational water loss via the stomatal closure and maintain the RWC as wild-type plants.
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415 Proline content
417
It is well documented that proline has an important role in protecting plants under drought stress. To
418
evaluate this hypothesis and to determine the effects of cop1 mutation on drought-induced proline
419
accumulation, proline level was measured in wild-type, cop1-4, and abi1-1 mutants under normal and
420
long-term drought stress conditions. Interestingly, we found that proline content in cop1-4 mutant leaves
421
was about 4.5 fold higher than that of the wild-type under normal growth conditions (Fig. 7B). As shown
422
in Fig. 7B, soil water deficiency resulted in proline accumulation in wild-type and abi1-1 mutant leaves
423
while the level of this compatible solute remained relatively constant until the fourth day of drought
424
treatment, when significantly increased when compared to well-watered conditions. However, the cop-1-4
425
leaves exhibited the lowest proline content while abi1-1 and col had the highest proline level at the end of
426
drought treatment.
427
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H2O2 and MDA content
429
Since the increased ROS production is one of the major effects of a drought stress on plants and can
430
induce lipid peroxidation, the levels of H2O2 (the main ROS in plants) and MDA (the key by-product of
431
lipid peroxidation) were measured to survey the oxidative damage level during drought stress. As
432
illustrated in Figs. 7C and 7D, the H2O2 and MDA content showed no significant difference between
433
wild-type and mutant plants under normal growth conditions. However, H2O2 level was increased 2- and
434
6-fold in wild-type and abi1-1 mutant leaves, respectively, after four days of water withholding as
435
compared with the control conditions. Interestingly, no significant change in the H2O2 content was
436
observed in the cop1-4 leaves in these conditions (Fig. 7C). Regarding MDA content, in contrast to wild-
437
type and abi1-1 mutant, the MDA content was not significantly altered in the cop1-4 leaves during soil
438
water deficient treatment. However, the highest MDA content was obtained from wild-type and abi1-1
439
mutant plants after four days of stopping irrigation (Fig. 7D). Based on the results, cop1-4 mutant
440
suffered from the lower level of drought-induced oxidative damage than wild-type under our
441
experimental conditions.
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442 443
Fig.7. RWC (A), Proline (B), H2O2 (C) and MDA (D) levels in cop1-4, abi1-1 mutants as well as wild-
444
type leave in response to soil water shortage conditions. Data represent the mean ± SD (n = 3). Means
445
followed by the same letter(s) are not significantly different at 0.05 level of probability (DMRT).
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446 Antioxidant activities level
448
ROS level is modulated by a well-defined detoxification system, involving a number of antioxidants that
449
reduce the reactive oxygen species content and minimize their deleterious effects. Here, the activity of
450
two main antioxidant enzymes, SOD and CAT were surveyed to monitor enzymatic ROS detoxification
451
in the plants under drought stress. Based on our results, there was no significant difference in SOD and
452
CAT activities among wild-type and the two mutants, cop1-4 and abi1-1 leaves under normal growth
453
conditions (Fig. 8A). While the CAT activity tends to be increased during drought treatment in wild-type
454
and reached to its highest activity (2.4 fold) at the end of experiment, cop1-4 exhibited no significant
455
change in the enzyme activity. The CAT activity was enhanced after two days of drought stress in abi1-1
456
leaves, and then significantly deceased after four days of water shortage in this mutant (Fig. 8A). In the
457
case of SOD activity, wild-type and abi1-1 leaves elevated SOD activity by 1.6 and 2.2 fold after four
458
days of drought treatment as compared to the control growth conditions whereas no alternation in the
459
enzyme activity was observed in drought-stressed cop1-4 mutant leaves (Fig. 8B).
460
Furthermore, anthocyanins are a large class of water-soluble pigments in the flavonoid group found in all
461
plant tissues, which can decrease leaf osmotic potential and operate as antioxidant in plants under abiotic
462
stresses (Rossel et al., 2007). Hence, to examine the effects of water deficiency on this non-enzymatic
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antioxidant level, especially in the cop1-4, anthocyanin content in wild-type and two mutants, cop1-4 and
464
abi1-1 leaves was measured. As shown in Fig. 8C, there was no significant difference in anthocyanin
465
content among wild-type, cop1-4, and abi1-1 plants under normal growth conditions, while soil water
466
deficiency gave rise to an excess production of anthocyanin in all plants. The anthocyanin level was
467
elevated by about 2.5 times in wild-type and cop1-4 leaves and 4 times in abi1-1 at the end of experiment
468
(fourth day of treatment). The more anthocyanin accumulation in abi1-1 leaves may implicate the severe
469
dehydration stress in the mutant.
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Fig.8. Enzymatic antioxidant activities
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472
level of CAT (A) and SOD (B) as well
473
as the non-enzymatic antioxidant level,
474
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anthocyanin (C) content, in cop1-4,
475
abi1-1 mutants, and wild-type leaves in
476
response to soil water stress. Data
477
represent the mean ± SD (n = 3). Means
478
followed by the same letter(s) are not
479
significantly different at 0.05 level of
480
484 485 486 487 488 489 490 491
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probability (DMRT).
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Gene expression analysis in cop1-4
493
Plant drought response is a complex biological process that needs to be surveyed at both physiological
494
and molecular levels. Here, to explore the effects of cop1 mutation on drought tolerance at the molecular
495
level, the expression profiling of several key stress-responsive genes, including MYB60, P5CS1, RD22,
496
KIN2, NCED3, and ABI1 was evaluated by qRT-PCR analysis in the wild-type and the two mutants’
16
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leaves, cop1-4 and abi1-1 under controlled and drought treatment conditions. Also, the COP1 expression
498
pattern was assessed in the plants under control, drought, salt and cold treatments as well as in the
499
presence and the absence of light. Furthermore, considering the fact that the cop1-4 stomata are
500
constitutively open in darkness (Mao et al., 2005) and AtMYB61 plays a major role in dark-induced
501
stomatal closure (Liang et al., 2005), the expression pattern of AtMYB61 was monitored in wild-type and
502
cop1-4 under light and darkness.
503
Based on the expression analysis of AtMYB60 gene, the transcript level of AtMYB60 was significantly
504
decreased after two days of drought treatment in the wild-type and cop1-4 leaves. The reduced gene
505
expression pattern was retained until the fourth day of treatment, when wild-type and cop1-4 leaves
506
accumulated the lowest level of AtMYB60 transcript, so that there was about 4 folds reduction in gene
507
expression at this time. As compared with wild-type and cop1-4 mutant, the gene expression was
508
diminished with a delay of two days, after four days of desiccation in abi1-1 mutant (Fig. 9A). Given that
509
the AtMYB60 function in the drought-induced stomatal closure, our results are consistent with the
510
stomatal behaviour at the stressed plants and illustrated that cop1-4 whole plant can lessen their stomatal
511
aperture via the reduced AtMYB60 transcript level in response to soil water limiting conditions.
512
In regards to stress-responsive genes, the wild-type as well as the mutants, cop1-4 and abi1-1 exhibited
513
elevated levels of KIN2, RD22, and P5CS1 under dehydration treatment compared with normal growth
514
conditions. But, interestingly, the up-regulation level of the genes was significantly lower in cop1-4
515
leaves than wild-type under drought treatment compared to normal growth conditions as illustrated in
516
Figs. 9B-9D
517
As ABA plays a fundamental role in the stress signalling pathway, leading to plant adaptation to adverse
518
growth conditions, the mRNA level of NCED3 and ABI1 genes involved in ABA biosynthesis and signal
519
transduction pathways, respectively, were assessed during drought treatment. As presented in Figs.9E and
520
9F, the transcripts abundance had no difference between wild-type and cop1-4 mutant under normal
521
growth conditions. However, the enhanced transcript level of NCED3 and ABI1 were observed in wild-
522
type, cop1-4 and abi1-1 after two days of desiccation. The induction of these genes in cop1-4 mutant can
523
suggest that this mutant is not deficient in ABA-related pathways.
525 526
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Fig. 9. Relative expression level of MYB60, KIN2, RD22, P5C1, NCED3 and ABI1 (A-F) in cop1-4, abi1-
529
1 mutants and wild-type leaves in response to soil water limiting conditions. Data represent the mean ±
530
SD (n = 3). Means followed by the same letter(s) are not significantly different at 0.05 level of probability
531
(DMRT).
532
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To elucidate the potential involvement of COP1 gene in plant abiotic stresses response, we evaluated its
534
expression under drought, salinity, and cold stresses. Our results, surprisingly demonstrated that COP1
535
expression was strongly induced by the applied stresses in wild-type and abi1-1 leaves, but not
536
significantly in the cop1-4 (Fig. 10). As illustrated in Fig. 10, in contrast to cop1-4 mutant, the COP1
537
transcript was accumulated in wild-type and abi1-1 leaves after two days of drought treatment until the
538
end of experiment (Fig. 10). Similarly, the same trend was detected in response to salt and cold stresses
539
(Fig. 10). As Fig. 10 displays, wild-type and abi1-1 mutant exhibited the elevated COP1 transcript level
540
after one day salinity treatment until five days of treatment while cop1-4 mutant accumulated this
541
transcript after three days of salt stress, however, the transcript abundance in cop1-4 leaves was
542
significantly lower than wild-type (Fig. 10). In the case of cold stress, while the COP1 transcript level
543
was notably increased in the wild-type and abi1-1 mutant at 4°C and -7°C, the transcript abundance was
544
approximately remained constant in cop1-4 leaves (Fig. 10).
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546 547
Fig. 10. Relative expression level of COP1 in cop1-4, abi1-1 mutants and wild-type leaves in response to
548
drought, salt, and cold stresses. Data represent the mean ± SD (n = 3). Means followed by the same
549
letter(s) are not significantly different at 0.05 level of probability (DMRT).
550
Earlier studies revealed that the stomatal aperture of cop1-4 mutant was much larger than wild-type and
552
our findings determined that the mutant was extremely sensitive to leaf detachment-imposed dehydration
553
(Fig. 1). With this information in mind, we assessed the expression level of NCED3 and COP1 genes in
554
detached leaves of wild-type and cop1-4 mutant at 10, 20, and 30 minutes after leaf detachment. As
555
shown in Figs. 11A and 11B, NCED3 and COP1 transcript accumulation were significantly induced in
556
both wild-type and cop1-4 leaves within 20 and 30 min after leaf detachment, respectively, implicating
557
that similar to NCED3, the COP1 could be an early-responsive gene. This broad responsiveness of COP1
558
to various types of abiotic stresses suggests it may be a component of plant abiotic stress response.
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566 567
Fig. 11. Relative expression levels of
568
NCED3 (A) and (B) COP1 (B) in
569
cop1-4
570
response to short-term dehydration
571
imposed by leaf detachment. Data
572
represent the mean ± SD (n = 3).
573
Means followed by the same letter(s)
574
are not significantly different at 0.05
575
level of probability (DMRT).
wild-type
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and
576
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577 578 579 580 581 582
We also investigated the probable effect of cop1 mutation on the steady-state mRNA level of AtMYB61 in
584
the presence and absence of light. Surprisingly, wild-type and cop1-4 plants showed the opposite
585
expression pattern. As Fig. 12A illustrates, in contrast to cop1-4, the transcript abundance of AtMYB61 is
586
significantly higher in the darkness than the light presence in wild-type plants. Similarly, the expression
587
analysis of COP1 demonstrated that both wild-type and cop1-4 displayed the decreased transcript
588
abundance in darkness when compared to the presence of light, but the reduction level was much higher
589
(11 folds) in cop1-4 than wild-type in darkness (Fig. 12B). Our results can infer that COP1 expression in
590
darkness is required for the expression of AtMYB61 that is essential for dark-induced stomatal closure.
592 593 594 595
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597 Fig.12. Relative expression levels of
599
MYB61 (A) and COP1 (B) in cop1-4
600
and wild-type leaves in the presence
601
and absence of light. Data represent
602
the mean ± SD (n = 3). Means
603
followed by the same letter(s) are not
604
significantly different at 0.05 level of
605
probability (DMRT).
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608 609 610 611 612 613 614 Promoter analysis
616
The gene expression induction or suppression under various developmental and environmental conditions
617
is mainly regulated via gene promoters and their cis-acting elements (Hernandez-Garcia and Finer, 2014).
618
In the current study, the altered expression pattern of COP1 gene in response to various abiotic stresses
619
prompted us to survey its promoter region for the probable stress-related cis-acting elements and the
620
corresponding transcription factors. The survey of 1 kb upstream sequences from translational initiation
621
codon of COP1 revealed the presence of multiple stress-associated cis-acting elements, including 3
622
abscisic acid-responsive elements (ABRE), 16 ABRE-like sequence required for etiolation-induced
623
expression of ERD1 (early response to dehydration 1) and 2 dehydration response element (DRE) in the
624
promoter region (Supplementary file S1). In addition, one salt-tolerance zinc finger protein binding site,
625
12 MYB recognition sites, one binding site for cold-regulated protein 15a (COR15a), and 20 heat shock
626
transcription factor (HSF) binding sites were detected in the COP1 promoter. The results implied that
627
COP1 is an abiotic stress-responsive gene that whose expression regulated in both ABA-dependent and
628
ABA-independent pathways. It is consistent with the altered COP1 expression level in response to
629
drought, salt, and cold stresses in both wild-type and abi1 mutant. Furthermore, in order to get insight into
630
the function of associated transcription factors (TFs) to COP1 promoter, all identified TFs were subjected
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to singular enrichment analysis embedded in AgriGO. Based on the analysis, several gene ontology (GO)
632
terms related to abiotic stresses including, response to stress (GO:0006950), response to abiotic stimulus
633
(GO:0009628), response to water deprivation (GO:0009414), response to abscisic acid stimulus
634
(GO:0009737), abscisic acid mediated signaling pathway (GO:0009738), response to salt stress
635
(GO:0009651), response to cold (GO:0009409), cellular response to heat (GO:0034605), response to
636
osmotic stress (GO:0006970), response to hydrogen peroxide (GO:0042542), and hyperosmotic salinity
637
response (GO:0042538) were significantly enriched (FDR < 0.01), which further support the COP1
638
function under various stresses. The complete list of significantly enriched GO term is presented in
639
Supplementary file S2.
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640 641 Discussion
643
Understanding the drought signal transduction pathway and the consequent plant response to reduce the
644
detrimental effects of water scarcity has continued to be one of the main objectives for scientists
645
(Obidiegwu et al., 2015; Pinheiro and Chaves, 2010). Drought stress response was extensively studied
646
in various plants, especially in Arabidopsis (Oh et al., 2005; Todaka et al., 2015; Wang et al., 2008). The
647
current study as the first attempt to uncover the different attributes of cop1-4 as well as lip1 mutants in
648
response to drought stress added the novel and main player, COP1, to drought signalling pathway. The
649
COP1 importance in plant drought response is related to its pivotal roles in developing stomata and
650
regulating stomatal movements (Mao et al., 2005). Stomatal closure is an early and rapid plant reaction to
651
water deficiency that is regulated through a complex network of signalling pathways (Merilo et al., 2015).
652
Here, we found that the lip1 stomatal apertures, like cop1-4, are significantly larger than wild-type under
653
normal growth conditions. It suggests that the COP1 function in the regulation of stomatal pore size is
654
conserved during evolution, in both Arabidopsis and pea. Interestingly, we discovered that contrary to
655
wild-type, the cop1-4 and lip1 detached leaves failed to decrease their stomatal aperture in response to
656
leaf detachment imposed dehydration, accounting for up to 50% of water loss during only 30 and 90
657
minutes after leaf excising in cop1-4 and lip1, respectively. It suggested that the COP1 plays a prominent
658
role in the sense and the rapid stomata response to short-term dehydration in the detached leaves in both
659
Arabidopsis and pea.
660
Guard cell ABA signaling is important for regulating basal stomatal openness and rapid stomatal
661
responses to environmental stimuli (Merilo et al., 2015). However, the appropriate hormone functioning
662
relies on the proper level of biologically active ABA, correlating with several processes including, ABA
663
biosynthesis, catabolism, conjugation, deconjugation, transport, and perception (Daszkowska-Golec and
664
Szarejko, 2013). Here, the sensitivity of cop1-4 detached leaves to exogenous ABA treatment after 120
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minutes, not after 40 minutes, implied that cop1-4 stomata is less sensitive to ABA than wild-type.
666
Similarly, Khanna et al (2014) reported that the stomata of GFP–TUA6,cop1-4 line resulted from
667
crossing GFP–TUA6 line with the cop1-4 mutant did not respond to 40 minutes treatment with 10 µM
668
ABA (Khanna et al., 2014). Although, ABA-mediated stomatal closure is not defective in the cop1-4
669
mutant, the delay in stomatal response to ABA may be long enough to induce rapid wilting in detached
670
leaves.
671
In Arabidopsis, ABA was synthesized mainly in leaves via the induction of NCED3 expression (Merilo et
672
al., 2015). NCED3 is considered to be the main regulatory enzyme, which its transcript up-regulated
673
within 15–30 min after leaf detachment or dehydration (Behnam et al., 2013; Xiong and Zhu, 2003).
674
Although, we could clearly detect the enhanced level of NCED3 transcript level within 20 minutes in both
675
wild-type and cop1-4 detached leaves, the cop1-4 stomata remained open, unlike wild-type. It can
676
propose that the accumulation of NCED3 transcript and the subsequent ABA biosynthesis appear to occur
677
normally in cop1-4 mutant; however, it is not sufficient for rapid stomatal closure in response to short-
678
term dehydration.
679
Unexpectedly, cop1-4 and lip1 whole plants were not as sensitive as the detached leaves to drought
680
treatment as they exhibited the decreased stomatal apertures accompanied by the similar level of RWC
681
between the mutant and wild-type during soil water deficient. This discrepancy highlights the root-shoot
682
signalling role in plant stress response. Contrary to detached leaves, as stress was imposed gradually on
683
the intact plants and the root-shoot signalling precede the ABA-induced stomatal closure, the ABA
684
concentration and time is enough to induce stomatal closure in the mutants as wild-type. Christmann et al
685
(2007) reported soil water stress generates a hydraulic signal in the shoot, which acts upstream of ABA
686
signalling and stomatal closure; however, both hydraulic signal and ABA is required for stomatal closure
687
in response to water stress. Another study by Pantin et al (2013) showed that ABA has two effects on
688
stomata: a direct biochemical effect on the guard cells and an indirect hydraulic impact by reducing leaf
689
water permeability triggered within vascular tissues. Under drought stress, ABA concentration rises in the
690
vascular parenchyma as a result of importing root-derived ABA and locally synthesized ABA. ABA
691
signalling in the bundle sheath by inactivating bundle sheath aquaporins (PIP) resulted in the reduced leaf
692
hydraulic conductance. Vascular ABA then transfers to the guard cells and promotes stomatal closure
693
(Pantin et al., 2013). Overall, our findings can suggest that the COP1 plays an important but a transient
694
role in initiating the rapid stomatal response to short-term dehydration and this role was evolutionary
695
conserved in both Arabidopsis and Pea.
696
Moreover, surveying the adaxial and abaxial stomatal density of wild-type and cop1-4 mutant under
697
control growth conditions and soil drought treatment revealed that there is no significant difference in
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stomatal density between wild-type and mutant. The similar results reported by previous studies
699
(Balcerowicz et al., 2014; Kang et al., 2009).
700
Although the stomatal aperture of cop1-4 was much wider than wild-type, both wild-type and cop1-4
701
displayed the similar level of RWC under normal growth conditions. As RWC implies the balance
702
between transpiration rate and water reservation, it indicated that cop1-4 mutant is able to conserve leaf
703
water probably via an efficient osmo-regulation system. It has been shown that proline accumulation
704
resulted in lowered cell osmotic potential and facilitated the cell turgor pressure maintenance (Hayat et
705
al., 2012). In line with this report, we found that cop1-4 leaves significantly contained more proline level
706
than wild-type under well-watered conditions. Therefore, the proline accumulation may be the essential
707
factor for compensating the increased water loss via the wide stomatal aperture and maintaining relative
708
leaf water content in cop1-4 mutants as wild-type plants.
709
The enhanced proline content as a common phenomenon in the stressed plants has also been widely
710
described; it is important not only for osmoregulation, but also for protecting cells by enhancing the
711
protein and cell membrane stability (Bhaskara et al., 2015; Estrada-Melo et al., 2015; Szabados and
712
Savouré, 2010). In the present study, while the increased content of proline was detected in wild-type and
713
abi1-1 after two days of drought stress, cop1-4 significantly accumulated this osmolyte after four days of
714
desiccation. It appears that the high constitutive levels of proline in cop1-4 can protect cell against the
715
detrimental effects of stress without additional proline enhancement until mutant exposed to longer
716
treatment periods or more severe stress, leading to further proline accumulation. The similar situation has
717
been also described in a drought-tolerant citrus genotype (Zandalinas et al., 2016).
718
Plants suffering from various stresses, including water deficiency often exhibit oxidative stress symptoms
719
as evidenced by the elevated reactive oxygen species and MDA levels (Das and Roychoudhury, 2014).
720
Compared with other ROS, H2O2 is a relatively long-lived molecule that is able to diffuse across cell
721
membranes. This characteristic is compatible with its role as a signalling molecule during growth and
722
stress plant response (Sharma et al., 2012). However, the high concentration of H2O2 can be a sign of
723
undesirable situation and extremely harmful for organism survival. Here, H2O2 and MDA content were
724
presented the positive association as also described by previous studies (Murshed et al., 2013; Ren et al.,
725
2016). In contrast to cop1-4 leaves, both H2O2 and MDA level were significantly incremented in wild-
726
type and abi1-1 under drought treatment. It implicated that cop1-4 mutant did not undergo the detectable
727
oxidative damage resulting from applied drought stress.
728
Enzymatic and non-enzymatic antioxidants are considered as an efficient defence system to cope with
729
excessive ROS and ameliorate the oxidative damage level. Among the enzymatic antioxidants, SOD acts
730
as one of the central and preliminary antioxidants by converting O2.− into H2O2 and maintaining the
731
intracellular O2.− within normal range (Das and Roychoudhury, 2014). In consistent with previous studies
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in Arabidopsis (Jung, 2004) and rubber tree (Wang, 2014), SOD activity was enhanced in wild-type and
733
abi1-1 leaves during drought stress while no significant change was detected in cop1-4 mutants, it is
734
probably due to either superoxide radical levels was not as high as for SOD activation in the mutant or the
735
non-enzymatic antioxidants such as anthocyanin play a main role in these conditions. Similarly, the lack
736
of significant CAT activity enhancement in cop1-4 can refer to the low level of H2O2 in the mutant as
737
reported that catalase breaks down high concentration of H2O2 because of its low affinity (high Km) for
738
this substrate (Mhamdi et al., 2010). It has been demonstrated that environmental stresses cause either
739
enhancement or depletion of CAT activity, depending on the intensity, duration, and type of the stress
740
(Janiak et al., 2015). Therefore, the drought-induced reductions in CAT activities in abi1-1 leaves may be
741
as a result of sever oxidative stress as also evidenced by the increased H2O2 and MDA levels. Overall, the
742
antioxidants activity was in accordance to H2O2 and MDA content during drought stress and may confirm
743
that oxidative damage level in cop1-4 and abi1-1 leaves is lower and higher than wild-type leaves,
744
respectively.
745
Many drought-inducible genes with various functions respond to water deficiency at the transcriptional
746
level. K1N2, RD22, and COR15a are of key stress-responsive genes encode the variety of LEA and like-
747
LEA proteins that are able to act as chaperones to stabilize proteins and membrane structure in the
748
stressed plants to confer cellular tolerance to dehydration (Goyal et al., 2005; Janiak et al., 2015). Based
749
on our results, the expression of these genes were induced in leaves of wild-type and two mutants, cop1-4
750
and abi1-1 in response to water deficiency; however, their expression levels in cop1-4 leaves were not as
751
high as wild-type, hence the improved drought tolerance of cop1-4 whole plant might not be correlated
752
with these genes. The expression of stress-inducible genes is regulated by the ABA-dependent and ABA-
753
independent pathways (Joshi et al., 2016). A similar expression pattern of the above-mentioned genes in
754
abi1-1 mutant in our study indicated that their induction is ABA-independent, as previous studies have
755
been also reported (Jensen et al., 1996).
756
There are two closely related P5CS genes in Arabidopsis that mainly P5CS1 expression is promoted by
757
drought and salt stresses (Ben Rejeb et al., 2015; Székely et al., 2008). In agreement with previous
758
researches, the increased steady state level of P5CS1 mRNA was detected in the drought stressed plants.
759
While the proline content of cop1-4 leaves was significantly higher than wild-type under normal growth
760
conditions, the P5CS1 transcript accumulation had not been followed the same pattern. It can refer to the
761
proline feedback inhibition effect as previous studies was also reported that proline biosynthesis in plants
762
primarily regulated at the transcriptional level by end product (Porcel et al., 2004; Sharma and Verslues,
763
2010). Although the role of ABA in regulating proline accumulation requires further examination due to
764
contradictory data obtained in various species by different researchers (Guan et al., 2014; Verslues and
765
Bray, 2005), we could clearly observed the enhanced P5CS1 transcript and proline levels in abi1-1
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mutant leaves, suggesting that no ABA involvement is required for proline accumulation or drought-
767
induced P5CS1 is regulated by both ABA-dependent and ABA-independent pathways.
768
In Arabidopsis genome, at least nine genes are identified to code NCED that among them NCED3 showed
769
higher expression in both roots and shoots in response to drought stress (Rasheed et al., 2016). Similarly,
770
we found the elevated NCED3 expression in wild-type and two mutants, cop1-4 and abi1-1 leaves under
771
water limiting conditions. Hence, the mutation in COP1 gene does not interfere with ABA biosynthesis
772
pathway at least at the transcription level. Further, Barrero et al revealed that there is a positive
773
correlation between the enhanced NCED3 transcript level and ABA content (Barrero et al., 2006). Thus,
774
the cop1-4 mutant can produce enough ABA, which facilitates the stomatal closure as evidenced by the
775
reduced stomatal pores in cop1-4 whole plant in response to soil water deficiency. Besides the
776
environmental signals, Arabidopsis stomatal aperture was modulated by several transcription factors,
777
including AtMYB60 and AtMYB61. Here, we found that the steady-state level of AtMYB60 was reduced in
778
wild-type, cop1-4, and abi1-1 leaves. The AtMYB60 response in abi1-1 refers to the presence of cis-acting
779
elements responsible for down-regulating gene expression in response to dehydration in an ABA-
780
independent manner (Rusconi et al., 2013). However, abi1-1 could not able to close their stomata in
781
response to water shortage conditions, it may propose that the ABA-independent pathway mediated
782
AtMYB60 down-regulation is not enough for drought-induced stomatal closure. The down-regulated
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AtMYB60 was in line with decreased stomatal pore in wild-type as reported by previous report (Cominelli
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et al., 2005) as well as cop1-4 leaves in response to soil water deficiency. Consequently, the diminished
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stomatal aperture in the stressed cop1-4 whole plant could be resulted from the reduced AtMYB60
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transcript level.
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AtMYB61 is a pleiotropic regulator of plant stomatal aperture, lateral root formation, and xylem cell
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differentiation. It has suggested that this gene has an active role for stomatal opening inhibition in
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darkness (Baldoni et al., 2015). Here, we figured out cop1-4 leaves accumulated AtMYB61 and COP1 in
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much lower than wild-type in darkness. Considering that stomatal closure was impaired in the cop1-4
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leaves in darkness and COP1 expression can complement the constitutive stomatal opening phenotype in
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this mutant (Mao et al., 2005), our findings can uncover that the expression of both COP1 and AtMYB61
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may essential for the reduced stomatal pores in darkness and AtMYB61 might play a key role on the
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downstream of COP1 for promoting darkness-induced stomatal closure.
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Additionally, we deciphered that COP1 expression pattern can undergo by various abiotic stresses
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(drought, salinity, and cold), offering the COP1 could be a stress-responsive gene. While COP1 transcript
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abundance remained relatively constant in cop1-4 mutant, it was significantly up-regulated in wild-type
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and abi1-1 mutant during abiotic stresses. The COP1 expression in abi1-1 mutant revealed that its
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expression is regulated through both ABA-dependent and ABA-independent pathways in response to
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unfavourable conditions as also evidenced by the presence of both ABRE and DRE cis-acting elements in
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the COP1 promoter region. Similarly, the existence of several enriched ABA- and stress-related GO terms
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among the biological functions of transcription factors associated to the COP1 promoter could further
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confirm the altered gene expression pattern in response to applied various abiotic treatments.
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Taken together, COP1 can act as a central regulator of abiotic stresses response pathway with diverse
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roles in detached leaves and whole plant levels. The conserved function of COP1 in both Arabidopsis and
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pea during evolution can emphasis its crucial importance. Our study adds a new level of complexity to the
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overall understanding of main effectors required for stomatal closure as well as the root-shoot signalling
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pathway under drought stress. Further efforts are needed to resolve exactly how COP1 mediates plant
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response to both short-term and long-term dehydration.
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Acknowledgements
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We are grateful to Prof. Xing-Wang Deng for providing cop1-4 seeds as well as Dr. William Thompson
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and Dr. Shannon Frances for providing lip1 seeds.
815 816 References
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Supporting information
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Supplementary file 2. List of significantly enriched GO terms associated with all transcriptions factors
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bind to COP1 promoter region.
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Supplementary file 1. List of stress-related cis-acting elements in COP1 promoter region.
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Highlights
2. COP1 is an abiotic stress-responsive gene in Arabidopsis.
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1. COP1 plays a fundamental role in the regulation of stomatal movements in response to dehydration in both Arabidopsis and Pea.
3. cop1-4 mutant stomata respond to short-term and long-term dehydration in a different manner in
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Arabidopsis.
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Author contributions M.M.J, S.GH, and S.M.S designed the research. M.M.J and S.GH carried out the experiment and analyzed the data. M.M.J wrote the manuscript. S.M.S and V.N supervised the project. All authors read
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and approved the manuscript.