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Polyamines contribute to salinity tolerance in the symbiosis Medicago truncatula-Sinorhizobium meliloti by preventing oxidative damage
Accepted Manuscript Polyamines contribute to salinity tolerance in the symbiosis Medicago truncatulaSinorhizobium meliloti by preventing oxidative damage Miguel López-Gómez, Javier Hidalgo-Castellanos, J. Rubén Muñoz-Sánchez, Agustín J. Marín-Peña, Carmen Lluch, José A. Herrera-Cervera PII:
S0981-9428(17)30146-8
DOI:
10.1016/j.plaphy.2017.04.024
Reference:
PLAPHY 4870
To appear in:
Plant Physiology and Biochemistry
Received Date: 24 January 2017 Revised Date:
24 April 2017
Accepted Date: 25 April 2017
Please cite this article as: M. López-Gómez, J. Hidalgo-Castellanos, J.Rubé. Muñoz-Sánchez, Agustí.J. Marín-Peña, C. Lluch, José.A. Herrera-Cervera, Polyamines contribute to salinity tolerance in the symbiosis Medicago truncatula-Sinorhizobium meliloti by preventing oxidative damage, Plant Physiology et Biochemistry (2017), doi: 10.1016/j.plaphy.2017.04.024. 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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Title
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Polyamines contribute to salinity tolerance in the symbiosis Medicago truncatula-
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Sinorhizobium meliloti by preventing oxidative damage.
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Authors
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Miguel López-Gómez, Javier Hidalgo-Castellanos, J. Rubén Muñoz-Sánchez,
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Agustín J. Marín-Peña, Carmen Lluch, José A. Herrera-Cervera
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Departamento de Fisiología Vegetal, Facultad de Ciencias, Universidad de
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Granada, Campus de Fuentenueva s/n, 18071 Granada, Spain.
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Corresponding Author
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Miguel López-Gómez
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e-mail: [email protected]
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Departamento de Fisiología Vegetal, Facultad de Ciencias, Universidad de
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Granada, Campus de Fuentenueva s/n, 18071 Granada, Spain
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ACCEPTED MANUSCRIPT Abstract
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Polyamines (PAs) such as spermidine (Spd) and spermine (Spm) are small ubiquitous
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polycationic compounds that contribute to plant adaptation to salt stress. The positive
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effect of PAs has been associated to a cross-talk with other anti-stress hormones such as
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brassinoesteroids (BRs), also involved in anti-stress responses in plants. In this work we
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have studied the effects of exogenous Spd and Spm pre-treatments in the response to
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salt stress of the symbiotic interaction between Medicago truncatula and Sinorhizobium
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meliloti by analyzing parameters related to nitrogen fixation, oxidative damage and
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cross-talk with BRs in the response to salinity.
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Exogenous PAs treatments incremented the foliar and nodular Spd and Spm content
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which correlated with an increment of the nodule biomass and nitrogenase activity.
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Exogenous Spm treatment partially prevented proline accumulation which suggests that
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this polyamine could replace the role of this amino acid in the salt stress response.
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Additionally, Spd and Spm pre-treatments reduced the levels of H2O2 and lipid
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peroxidation under salt stress. PAs induced the expression of genes involved in the BRs
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biosynthesis which support a cross-talk between PAs and BRs in the salt stress response
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of the M. truncatula-S. meliloti symbiosis
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In conclusion, exogenous PAs improved the response to salinity of the M. truncatula-S.
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meliloti symbiosis by reducing the oxidative damage induced under salt stress
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conditions. In addition, in this work we provide evidences of the cross-talk between PAs
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and BRs in the adaptive responses to salinity.
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Keywords
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Polyamines, brassinosteroids, salt stress, symbiosis, Medicago truncatula.
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Abbreviations
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PAs, polyamines; BRs, brassinosteroids; Put, putrescine; Spd, spermidine; Spm,
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spermine; Cad, cadaverine; Homspd, homospermidine; MDA, malondialdehyde; Pro,
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proline; NFR, nitrogen fixation rate; NFW, nodule fresh weight.
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1. Introduction The diamine putrescine (Put) and the polyamines (PAs) spermidine (Spd) and spermine
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(Spm) are small ubiquitous polycations involved in numerous processes in all living
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organisms [1]. In plants, PAs are involved in cell division, embryogenesis, senescence,
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floral development and fruit ripening [2]. In addition, PAs play an important role in the
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response of plants to adverse environmental conditions due to their polycationic nature
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[3] [4]. Among these adverse conditions, soil salinity is one of the most important
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abiotic factors limiting crop productivity all over the world, especially in arid and
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semiarid regions, and is predicted to get worse under climate change conditions [5]. Salt
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stress adversely affects plant development and productivity by generating ion toxicity,
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osmotic stress, water deficits and oxidative damage through the production of reactive
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oxygen species (ROS) including hydrogen peroxide (H2O2) among others [6].
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Legumes are classified as salt-sensitive crop species and their productivity is
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particularly affected by soil salinity because nodular nitrogenase activity, responsible
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for the nitrogen supply to the plant in symbiosis with soil bacteria known as rhizobia,
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markedly decreases upon exposure to saline conditions [7] [8]. Root nodules of legumes
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have been found to contain a high variety and concentration of PAs, some of them of
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bacteroidal origin [9], however, little is known about the role of PAs within the root
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nodules. A cross-talk between PAs and other plant growth regulators such as
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brassinosteroids (BRs), has been described in the response to abiotic stresses [10], [11],
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[12]. BRs biosynthesis is regulated at the transcriptional level of the biosynthetic genes
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by other plant hormones such as auxin [13] and in addition, BRs have been shown to be
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involved in the systemic regulation of the root nodule formation in soybean [14] by a
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modification of the PAs levels in leaves [15].
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to salinity. There is a large body of evidence suggesting that exogenous application of
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PAs could preserve plant cell membrane integrity, minimize growth inhibition caused
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by stress, reduce superoxide radical and H2O2 contents and increase activities of
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antioxidant enzymes (reviewed by [2]).
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In this work we have studied the effects of exogenous Spd and Spm in the adaptation to
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salt stress of the symbiosis M. truncatula-S.meliloti by analyzing parameters related to
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nitrogen fixation, oxidative damage and cross-talk with BRs in the response to salinity.
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2. Material and Methods
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2.1 Biological material and growth conditions
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Medicago truncatula (var. Jemalong) seeds were scarified by immersion in concentrated
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H2SO4 for 5 min, washed with sterile water, surface sterilized by immersion in NaClO
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50% (v/v) plus Tween-20 for 10 min and germinated onto 1.0% water-agar plates at 25
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ºC in the darkness. After 3 days, Medicago seedlings were transferred to sterile
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vermiculite:perlite (3:1) and watered with a modified nitrogen free [16] nutrient
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solution. Two days later, M. truncatula seedlings were inoculated with S. meliloti 1021
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strain (c. 109 cell ml-1) grown in a TY medium.Plants, in individual pots of about 200
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ml, were grown in a controlled environmental chamber with a 16/8 h light-dark cycle,
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23/18ºC day night temperature, relative humidity 55/65% and photosynthetic photon
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flux density (400-700 nm) of 450 µmol m-2 s-1 supplied by combined fluorescent and
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incandescent lamps. Six weeks after sowing plants were subjected to Spd and Spm
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treatments by the addition of 0.1 mM of each polyamine to the nutrient solution.
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Control plants were watered with the same nutrient solution without polyamines. Salt
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nutrient solution. Control plants were watered with a NaCl-free nutrient solution. Plants
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were harvested 10 weeks after sowing with polyamines and NaCl treatments lasting 4
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and 2 weeks, respectively. Nodules and leaves were frozen at -80 ºC for further
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analyses. Samples of leaves, stems and roots were dried at 70 ºC for 24 h and their dry
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weight determined.
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2.2 Nitrogen fixation
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Nitrogenase activity (E.C. 1.7.9.92) was measured as the representative H2-evolution in
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an open-flow system [17] using an electrochemical H2 sensor (Qubit System Inc.,
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Canada). H2 production was recorded in intact nodulated roots of plants. Apparent
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nitrogenase activity (ANA, rate of H2 production in air) was determined under N2:O2
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(80%:20%) with a total flow of 0.4 l min-1. After reaching steady-state conditions total
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nitrogenase activity (TNA) was determined under Ar:O2 (79%:21%). Nitrogen fixation
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rate (NFR) was calculated as (TNA-ANA)/3. Standards of high purity H2 were used to
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calibrate the detector.
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2.3 Determination of free polyamines in leaves and nodules
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Nodule and leaves extracts were prepared from 0.2 g of fresh tissue with 0.6 ml of 5%
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(v/v) cold perchloric acid (PCA) and incubated 24 h at 4 ºC. The homogenate was
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centrifuged (3,000xg, 5 min, 4 ºC) and 0.2 ml aliquots of the supernatant were
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dansylated as described below. The analysis of free PAs was performed with HPLC
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(Agilent Technologies 1260) equipped with a reverse phase column (4.6 x 250 mm
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ACCEPTED MANUSCRIPT C18) after derivatization with dansyl chloride (Sigma). Derivatization was performed by
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mixing 0.2 ml aliquots of the extracts prepared as described above with 0.4 ml of dansyl
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chloride (prepared fresh in acetone, 10 mg/ ml) and 0.2 ml of saturated sodium
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carbonate. After brief vortexing, the mixture was incubated in darkness at room
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temperature overnight. Excess dansyl reagent was removed by reaction with 0.1 ml (100
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mg/ml) of added proline, and incubation for 30 min. Dansylpolyamines were extracted
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in 0.5 ml toluene. The organic phase was collected and evaporated to dryness under a
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stream of nitrogen, and redissolved in 0.1 ml acetonitrile.
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Column flow was 1.5 ml min-1 and the elution gradient was prepared with eluent A
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(water) and eluent B (acetonitrile). The column was equilibrated with 70% B and 30%
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A before injecting 0.01 ml samples. This was followed by a linear gradient ending with
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100% B after 9 min. The final step was held for 4 min before regenerating the column.
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Detection was done with a fluorometer using excitation and emission wavelengths of
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415 and 510 nm, respectively, according to [18]. A relative calibration procedure was
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used to determine the PAs in the samples, using 1,7- diaminoheptane (HTD) as internal
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standard and PAs standards amounts ranging from 0.3 to 1.5 nmol purchased from
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Sigma. Results were expressed as nmol g-1 fresh weight.
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2.4 Proline determination
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Proline was determined by the ninhydrine method [19]. Briefly, 250 mg of plant
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material was homogenized in 3 ml of 95% (v/v) ethanol at room temperature and
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centrifuged at 2,000 x g for 5 min. 300 µl of distilled water and 2 ml of ninhydrine
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reagent were added to an aliquot of 200 µl of extract. The mixture was boiled for 60
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min, and the reaction was stopped in an ice bath. The chromophore obtained was 7
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extracted with 6 ml of toluene by vigorous shaking for 20 s. Absorbance of the resulting
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organic layer was measured at 520 nm with Varian UV-VIS spectrophotometer.
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Calibration was made using L-Pro as a standard.
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2.5 Lipid peroxidation
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Lipid peroxidation was measured by the level of malondialdehyde (MDA), a product of
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lipid peroxidation, using a reaction with thiobarbituric acid (TBA) as described by [20].
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Fresh samples (100 mg) were ground in a mixture of 1 ml trichloroacetic acid (TCA)
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(20% w/v) and 0.2 ml of 4% (w/v) butylatedhidroxytoluene in ethanol, at 4 ºC. After
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centrifugation (10,000 x g for 15 min), 0.25 ml aliquots of the supernatant were mixed
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with 0.75 ml of 0.5% (w/v) thiobarbituric acid in 20% TCA and the mixture was
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incubated at 94 ºC for 30 min. The reaction was stopped by cooling in an ice bath for 15
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min. Reaction tubes were centrifuged at 10,000 x g for 15 min and supernatants were
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used to determine the absorbance at 532 nm. The value for non-specific absorption at
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600 nm was subtracted.
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2.6 Histochemical and quantitative detection of H2O2 in leaves
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The histochemical analysis of H2O2 was performed in leaves of two weeks old plants
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grown axenically in glass test tubes. Plants were pretreated with Spm 0.1 mM 24 h
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before treatment with NaCl to a final concentration of 150 mM for 24h. The H2O2 was
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localized histochemically by staining leaves with 1% 3,3-diaminobenzidine (DAB)
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solution. Leaves were immersed in such solution until brown spots appeared due to the
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boiling ethanol to see the spots.
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Quantitative analysis of H2O2 was performed spectrophotometrically after reaction with
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KI [22]. The reaction mixture consisted of 0.5 ml 0.1% trichloroacetic acid (TCA) leaf
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extract supernatant, 0.5 mL of 100 mM K-phosphate buffer and 2 mL reagent (1 M KI
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w/v in fresh double-distilled water H2O). The blank probe consisted of 0.1% TCA in the
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absence of leaf extract. The reaction was developed for 1 h in darkness and absorbance
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measured at 390 nm. The amount of H2O2 was calculated using a standard curve
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prepared with known concentrations of H2O2.
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2.7 Gene expression analysis in leaves
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For gene expression analysis, plants were grown axenically onto filter paper in glass test
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tubes containing 10 ml of nutrient solution [23]. Two weeks after sowing, plants were
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pre-treated with Spd and Spm to a final concentration of 0.1 mM for 24h and then, NaCl
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to a final concentration of 150 mM was added. After 48h and 24h of PAs and NaCl
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treatments, respectively, plants were harvested and frozen at -80 ºC. A total of 6 plants
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per repetition and treatment were used for RNA preparation.
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Total RNA was extracted using an RNeasy plant mini kit (Macherey-Nagel, Germany)
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followed by treatment with DNaseI (Ambion, Texas, USA) for genomic DNA removal.
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First-strand cDNA was reverse transcribed from 1.5 µg of DNase-treated total RNA. All
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DNase-treated total RNA samples were denatured at 65 ºC for 5 min followed by quick
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chill on ice in 12 µl of reaction mixture containing 0.5 µg oligo-dT adapter primers and
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1 µl of 10 Mm deoxy-nucleotide triphosphate.
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inhibitor and 2 µl of 0.1 M dithiothreitol (DTT), the reaction was preheated at 37 ºC for
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3 min before the addition of 1 µl (200 U) of iScript reverse transcriptase (Bio-Rad,
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California, USA). The reaction mixture was incubated at 42 ºC for 50 min, followed by
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heat inactivation at 70 ºC for 15 min. The resulted first strand cDNA was amplified
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using gene specific primers (Table 1) designed from the transcribed region of each gene
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by using the Clone Manager Professional Suite software. The actin gene was used as
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loading control.
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PCR amplifications were performed in 20 µl reactions mixture as follows: one cycle of
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2 min at 94 ºC, 35 cycles of 30 s at 94 ºC, 30 s at 56 ºC and 1 min at 72 ºC and a final
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extension at 72 ºC for 10 min. PCR products were electrophoretically separated in 1%
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(w/v) agarose gels. Real-time PCR (qPCR) was performed using a SYBR Green PCR
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Master kit containing the Platinum Taq DNA polymerase (Invitrogen) on an iCycler IQ
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thermocycler (Bio-Rad). PCR amplification mixtures contained 10 ng of template
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cDNA and 0.5 U of polymerase. The cycling conditions were chosen according to the
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manufacturer. They comprised 10 min polymerase activation at 95 ºC and 35 cycles at
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95 ºC for 15 s, 55 ºC for 30 s and 72 ºC for 20 s. Results were quantified with the DDCt
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method [24]. Transcript levels were normalised to actin gene expression. The primer
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sequences for qPCR analysis are provided in Table 1.
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2.8 Statistical analysis
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Experiments were arranged in a completely randomized design with totally 60 plants
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per treatment. The data were subjected to an analysis of two-way ANOVA with
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exogenous polyamines as one factor and salt treatment as the other using the 10
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significant differences between treatments were determined by LSD (P ≤ 0.05).
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Experiments were performed three times in triplicate. Mean values ± SE error bars are
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3. Results
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3.1 Exogenous PAs induce plant growth
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Exogenous addition of Spd and Spm increased plant biomass about 43% with the same
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effect in shoots and roots (Fig. 1). Under salt stress conditions, the effect of PAs
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treatment was similar on the SDW and higher on RDW which incremented by 57%. Salt
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treatment provoked a plant growth inhibition more significant in roots than in shoots
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with a 40% and 20% reduction, respectively. Pre-treatments with PAs did not modify
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the response to salinity in shoots and roots.
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3.2 Nitrogenase activity is increased by exogenous PAs
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Nitrogen fixation rate (NFR), evaluated through the nitrogenase activity and the nodule
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fresh weight (NFW) is shown in Fig. 2. In general, NFR was highly increased by the
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Spd treatment with 2.6 fold increment. Additionally, under salt stress conditions the
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effect of both PAs was even greater, which led to a reduction of the salinity inhibitory
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effect from 11 to 10 and 3 times with Spd and Spm, respectively. Nodule biomass was
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also induced by the Spd and Spm treatments with 44% and 32% increment,
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respectively. This effect was even higher under salt stress with double nodule biomass
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in plants co-treated with PAs and NaCl. Salinity provoked a NFW reduction of 40%
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while this effect was reduced to 20% with Spd and 4% with Spm.
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3.3 Nodule specific PAs accumulate under salt stress
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Content of PAs in leaves and nodules were analyzed in order to compare the effect of
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exogenous Spd and Spm in both tissues under salt stress as shown in Fig. 3. In general,
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the levels of PAs were higher in nodules, which also display a more complex PA profile
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because they contain nodule-specific PAs such as cadaverine (Cad) and
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homospermidine (Homspd). Exogenous Spd and Spm treatments provoked an
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increment of both PAs of about 50% in leaves. Under salt stress conditions, Spm was
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the only polyamine that accumulated in leaves, with 30% and 46% increment in control
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and Spm treated plants. Put levels did not show differences by PAs treatment in leaves
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but NaCl provoked a reduction that ranged from 50% to 2.7 fold. Spd showed a similar
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response to salt stress while Spm was the only polyamine that accumulated in salt-
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stressed leaves. A similar result was detected for Spm in nodules, although in addition
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to this polyamine, Cad doubled its concentration under salinity, independently of the co-
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treatment with exogenous Spd and Spm. Homspd was the most abundant polyamine in
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nodules and under salt stress increased between 37% and 16% depending on the
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exogenous polyamine treatment. Put and Spd responses to salinity in nodules were
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similar to the observed in leaves with significant reductions under salt stress conditions.
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3.4 Proline accumulation is partially prevented by exogenous Spm
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the PAs metabolism and the synthesis of this amino acid. Salt stress induced a dramatic
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increase in the Pro levels in leaves with 3.6 fold higher concentration in such conditions
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(Fig. 4). However, the co-treatment with Spm partially inhibited the accumulation of
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Pro, which only showed a 76% induction by the salinity compared with the 3.6 fold
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induction observed in the absence of the PAs co-treatment. On the contrary, Spd did not
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induce any effect on the Pro accumulation by the salinity.
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3.5 Lipid peroxidation is inhibited by exogenous PAs
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Lipid peroxidation, estimated as the malondialdehyde (MDA) concentration in leaves
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(Fig. 5), was prevented by the exogenous treatment with Spd and Spm. Salt stress
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provoked a 2.5 fold increment in the MDA levels, however, with the exogenous Spd
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and Spm treatment this increment was 25% and 43%, respectively. In control
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conditions, no differences in the MDA levels were induced by the exogenous treatments
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with PAs.
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3.6 H2O2 production is reduced by exogenous PAs under salt stress
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H2O2 content in leaves was evaluated in a quantitative and in a semi-quantitative way in
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leaves as shown in Fig. 6A, B. The quantitative assay revealed that the level of H2O2
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was incremented by 3 times under salt stress conditions. However, pre-treatments with
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PAs reduced this increment to 30% with Spd and it was even completely abolished with
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Spm. Interestingly, the treatment with Spd and Spm produced an induction of H2O2 of
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40% and 2.5 times, respectively. The histochemical assay showed similar results to the
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quantitative assay with an increment of H2O2 in the salt stressed leaves and a slight
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reduction of this effect by the pretreatment with Spd.
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3.7 Exogenous PAs induce the synthesis of Brassinosteroids
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Expression level of genes involved in the synthesis of BRs DET2 (De-etiolated 2),
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DWF4 (Dwarf 4) and CYP85 were analyzed in leaves in order to determine a possible
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interaction between PAs and BRs metabolism (Fig. 7). Additionally, the expression of
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PAO1 (Polyamine oxidase 1) responsible of the Spd and Spm catabolism was analyzed.
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In general, all genes implicated in the synthesis of BRs were induced under salt stress
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conditions with 2 to 5 fold increment in the expression level. Exogenous treatments
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with PAs also induced the transcription level of the BRs biosynthetic genes to a higher
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extend with Spm which incremented 8 to 17 times the expression of the three genes
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analyzed. Nevertheless, the positive effect of Spd on the expression levels was
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completely abolished by salt stress and partially by the Spm treatment, except for
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DWF4 that did not show a significant difference. PAO1 transcription level was induced
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by Spd and Spm as well, while no significant differences were induced by the salt
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treatment.
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4. Discussion
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Exogenous application of PAs has been extensively shown to enhance tolerance to
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salinity stress in plants by scavenging free radicals, stabilizing membrane and cellular
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structures and modulating ion channels among other effects [25]; [3]; [26]. The positive
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effect of PAs has been associated to a cross-talk with other anti-stress hormones such as
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ACCEPTED MANUSCRIPT abcisic acid [27]; [28] salicylic acid [29], ethylene [30] or BRs [10, 12]. Indeed, the
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establishment of symbiosis between legumes and rhizobium has been shown to be
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influenced by the regulation of the PAs levels by a systemic effect of BRs on root
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nodule formation [15]. Those previous discoveries led us to study the effect of
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exogenous PAs (Spd and Spm) on the response to salinity of M. truncatula-S. meliloti
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symbiosis and its possible interaction with the BRs biosynthetic genes.
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Treatments with Spd and Spm increased plant growth, having similar effects on SDW
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and RDW (Fig. 1). This effect of exogenous PAs would be related with their growth
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regulatory capacity which includes DNA replication, cell division and root growth [3]
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Together with the increment in plant biomass, exogenous PAs incremented also nodule
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nitrogenase activity (Fig. 2).This could be also involved in the plant growth promotion
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due to a higher nitrogen supply to the plant. In that sense, a linear correlation between
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the concentration of PAs in nodules and nitrogenase activity has been shown [31].The
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increment of nitrogenase activity was accompanied by an increment of the nodule fresh
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weight as previously shown in Galega orientalis-Rhizobium galegae symbiosis [32].
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This effect could be related to a regulatory role of PAs in the nodulation process, as
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suggested by [33] in Lotus japonicus, where the expression of PAs biosynthetic genes
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(Spds and Spms) was maximal at early stages of nodule development.
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Under salt stress conditions Put and Spd levels were lower in leaves independently of
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the exogenous addition of PAs, while Spm augmented 32% in control plants and 46% in
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Spm treated plants (Fig. 3). In general, an increment in the (Spd+Spm)/Put ratio has
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been reported to be related with salinity tolerance in most cases [34]. In addition, Spm
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seems to participate on membrane modulation of permeability and stability [35]
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reducing radical generation under oxidative stress [36]. In that sense, Spm accumulation
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has been considered a general feature of plant response to salinity [37]. Exogenous Spd
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which indicates a transport of these PAs from the root to the shoot. Nodule PAs analysis
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revealed the presence of uncommon PAs such as Cad and Homspd, characteristics of
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nodules of legumes such as M. truncatula [38] or Phaseolus vulgaris [9]. In addition,
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the levels of all PAs were higher in nodules than in leaves, as described by [39], with
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Homspd as the most abundant PA synthesized by the bacteroids [38]. Similarly to
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leaves, exogenous Spd and Spm treatments incremented the nodular content of both
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PAs which correlated with an increment of the nodule biomass (NFW) and nitrogenase
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activity (NFR), suggesting the implication of Spd and Spm in the improvement of the
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symbiosis effectiveness. Nevertheless, Cad and Homspd levels declined by the
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exogenous addition of the common PAs (Spd and Spm), which might be due to the
337
replacement of these uncommon PAs by Spd and Spm, since the exact structure of these
338
compounds has been shown not to be critical for their function [40]. Interestingly, the
339
concentration of nodule specific PAs (Cad and Homspd) augmented under salt stress
340
due to the implication of Homspd in the stress tolerance of fast-growing rhizobia [41].
341
Proline accumulation is considered one of the most commonly adaptive responses of
342
plants to salinity due to its antioxidant and osmo-compatible properties [42].
343
Additionally, polyamine metabolism exerts a direct or indirect action on proline
344
metabolism through PAs degradation, which could contribute to proline accumulation,
345
or by the competition of both metabolites by glutamate as common precursor [43]. In
346
this context, salt stress strongly induced proline accumulation in M. truncatula leaves
347
(Fig 4) which suggest prevalence of this amino acid over PAs in the response to salinity
348
as previously described in Medicago sativa nodules [43]. Nevertheless, exogenous Spm
349
treatment partially prevented proline accumulation which together to the Spm
350
accumulation under salinity suggests that in such conditions, this polyamine could
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ACCEPTED MANUSCRIPT replace the role of proline without requiring its accumulation. This result is supported
352
by [44] who reported that exogenous PAs decreased Pro accumulation in salinity
353
exposed Phaseolus vulgaris plants.
354
In addition to the primary effects, salinity leads to oxidative stress through an increase
355
of reactive oxygen species (ROS) such as hydrogen peroxide (H2O2), which cause lipid
356
peroxidation and disturb cellular membrane functioning. The H2O2 level increased
357
significantly upon salt stress exposure (Fig. 6A), which indicated higher oxidative stress
358
in these plants. MDA, a lipid peroxidation product, served as the indicator of the extent
359
oxidative damage in salt stressed plants in this study (Fig. 5). Spd and Spm pre-
360
treatments reduced the levels of H2O2 and MDA during salt stress. These results agree
361
with previous studies [25]; [45] and suggest that PAs serve as efficient ROS scavenger
362
and membrane stabilizers by the MDA reduction under salt stress. However, at low
363
concentrations, H2O2 is known to prevent oxidative damage by up-regulating
364
antioxidative defence enzymes and by restoring redox homeostasis [46] which make
365
vital to keep the level of H2O2 rather than removing it. In that sense, visual
366
identification of H2O2 detected by histochemical staining (Fig. 6B) as well as the
367
quantitative analysis reflected a moderate increment of H2O2 in Spd and Spm treated
368
plants.
369
The beneficial effects of PAs in the response to salinity have been associated to a cross-
370
talk with other plant growth regulators such as BRs [47]. Indeed, in a previous study we
371
found that the salt stress ameliorative effect of 24-epibrassinolide in the M. truncatula-
372
S. meliloti symbiosis was mediated by PAs [10]. In that sense, we found that exogenous
373
PAs induced the expression of genes involved in the BRs biosynthesis (Fig. 7) which
374
support a cross-talk between PAs and BRs in the salt stress response of the M.
375
truncatula-S. meliloti symbiosis.
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ACCEPTED MANUSCRIPT In conclusion, exogenous PAs improved the response to salinity of the M. truncatula-S.
377
meliloti symbiosis by reducing the nitrogenase inhibition as well as the oxidative
378
damage induced under salt stress conditions. Additionally, in this work we provide
379
evidences of the cross-talk between PAs and BRs in the adaptive responses to salinity.
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380
Aknowledgements
382
This work has been supported by the Andalusian Research Program (AGR-139) and the
383
Spanish Ministry of Science and Technology (Grant: AGL2013-42778-P).
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ACCEPTED MANUSCRIPT Figure legends
397
Figure 1
398
Effect of exogenous Spd and Spm on shoot dry weight (SDW) and root dry weight
399
(RDW) of M. truncatula plants inoculated with S. meliloti under control (white bars)
400
and salt stress conditions (grey bars). Data are means + SE (n=10). Mean values
401
followed by the same letter do not differ (p<0.05) using the LSD test.
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Figure 2
404
Effect of exogenous Spd and Spm on nitrogen fixation rate (NFR) and nodule fresh
405
weight (NFW) of M. truncatula plants inoculated with S. meliloti under control (white
406
bars) and salt stress conditions (grey bars). Data are means + SE (n=10). Mean values
407
followed by the same letter do not differ (p<0.05) using the LSD test.
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Figure 3
410
Effect of exogenous Spd and Spm on polyamines content (Put, putrescine; Spd,
411
spermidine; Spm, spermine; Cad, cadaverine; Homspd, homospermidine) in M.
412
truncatula leaves (L) and nodules (N) inoculated with S. meliloti under control (white
413
bars) and salt stress conditions (grey bars). Data are means + SE (n=4). Mean values
414
followed by the same letter do not differ (p<0.05) using the LSD test.
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Figure 4
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ACCEPTED MANUSCRIPT Effect of exogenous Spd and Spm on proline content (Pro) in leaves of M. truncatula
418
inoculated with S. meliloti under control (white bars) and salt stress conditions (grey
419
bars). Data are means + SE (n=4). Mean values followed by the same letter do not differ
420
(p<0.05) using the LSD test.
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Figure 5
423
Effect of exogenous Spd and Spm on malondialdehyde content (MDA) in leaves of M.
424
truncatula inoculated with S. meliloti under control (white bars) and salt stress
425
conditions (grey bars). Data are means + SE (n=4). Mean values followed by the same
426
letter do not differ (p<0.05) using the LSD test.
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427
Figure 6
429
Effect of exogenous Spd and Spm on (A) H2O2 content in leaves of M. truncatula
430
inoculated with S. meliloti under control (white bars) and salt stress conditions (grey
431
bars). Data are means + SE (n=4). Mean values followed by the same letter do not differ
432
(p<0.05) using the LSD test. (B) DAB staining of H2O2 in leaves of M. truncatula
433
inoculated with S. meliloti and treated or not with NaCl and Spd.
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Figure 7
436
Effect of exogenous Spd and Spm on expression level of DET2, DWF4, CYP85 and
437
PAO1 genes in leaves of M. truncatula inoculated with S. meliloti under control (white
20
ACCEPTED MANUSCRIPT 438
bars) and salt stress conditions (grey bars). Data are means + SE (n=4). Mean values
439
followed by the same letter do not differ (p<0.05) using the LSD test.
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[1] A. Bouchereau, A. Aziz, F. Larher, J. Martin-Tanguy, Polyamines and environmental challenges: recent development, Plant Science, 140 (1999) 103-125. [2] S.S. Hussain, M. Ali, M. Ahmad, K.H.M. Siddique, Polyamines: Natural and engineered abiotic and biotic stress tolerance in plants, Biotechnol. Adv., 29 (2011) 300-311. [3] R. Alcazar, T. Altabella, F. Marco, C. Bortolotti, M. Reymond, C. Koncz, P. Carrasco, A.F. Tiburcio, Polyamines: molecules with regulatory functions in plant abiotic stress tolerance, Planta, 231 (2010) 1237-1249. [4] J.H. Liu, H. Kitashiba, J. Wang, Y. Ban, T. Moriguchi, Polyamines and their ability to provide environmental stress tolerance to plants, Plant Biotechnology, 24 (2007) 117-126. [5] J. Rozema, T. Flowers, Ecology: Crops for a salinized world, Science, 322 (2008) 14781480. [6] R. Munns, M. Tester, Mechanisms of Salinity Tolerance, Annu. Rev. Plant Biol., 59 (2008) 651-681. [7] M. López, J.A. Herrera-Cervera, C. Iribarne, N.A. Tejera, C. Lluch, Growth and nitrogen fixation in Lotus japonicus and Medicago truncatula under NaCl stress: Nodule carbon metabolism, J. Plant Physiol., 165 (2008) 641-650. [8] I. Aranjuelo, C. Arrese-Igor, G. Molero, Nodule performance within a changing environmental context, J. Plant Physiol., 171 (2014) 1076-1090. [9] M. López-Gómez, L. Cobos-Porras, J. Hidalgo-Castellanos, C. Lluch, Occurrence of polyamines in root nodules of Phaseolus vulgaris in symbiosis with Rhizobium tropici in response to salt stress, Phytochemistry, 107 (2014) 32-41. [10] M. López-Gómez, J. Hidalgo-Castellanos, C. Lluch, J.A. Herrera-Cervera, 24Epibrassinolide ameliorates salt stress effects in the symbiosis Medicago truncatulaSinorhizobium meliloti and regulates the nodulation in cross-talk with polyamines, Plant Physiology and Biochemistry, 108 (2016) 212-221. [11] S.P. Choudhary, H.V. Oral, R. Bhardwaj, J.Q. Yu, L.S.P. Tran, Interaction of brassinosteroids and polyamines enhances copper stress tolerance in raphanus sativus, J. Exp. Bot., 63 (2012) 5659-5675. [12] Q. Zheng, J. Liu, R. Liu, H. Wu, C. Jiang, C. Wang, Y. Guan, Temporal and spatial distributions of sodium and polyamines regulated by brassinosteroids in enhancing tomato salt resistance, Plant Soil, 400 (2016) 147-164. [13] Y. Chung, P.M. Maharjan, O. Lee, S. Fujioka, S. Jang, B. Kim, S. Takatsuto, M. Tsujimoto, H. Kim, S. Cho, T. Park, H. Cho, I. Hwang, S. Choe, Auxin stimulates DWARF4 expression and brassinosteroid biosynthesis in Arabidopsis, Plant J., 66 (2011) 564-578. [14] J. Terakado, T. Yoneyama, S. Fujihara, Shoot-applied polyamines suppress nodule formation in soybean (Glycine max), J. Plant Physiol., 163 (2006) 497-505. [15] J. Terakado-Tonooka, S. Fujihara, Involvement of polyamines in the root nodule regulation of soybeans (Glycine max), Plant Root, 2 (2008) 46-53. [16] A. Puppo, J. Rigaud, Indole-3-acetic-acid (IAA) oxidation by leghemoglobin from soybean nodules, Physiol. Plantarum, 35 (1975) 181-185. [17] J.F. Witty, F.R. Minchin, Hydrogen measurements provide direct evidence for a variable physical barrier to gas diffusion in legume nodules, J. Exp. Bot., 49 (1998) 1015-1020. [18] H.E. Flores, A.W. Galston, Analysis of Polyamines in Higher Plants by High Performance Liquid Chromatography, Plant Physiol., 69 (1982) 701-706. [19] W. Troll, J. Lindsley, A photometric method for the determination of proline, J. Biol. Chem., 215 (1955) 655-660. [20] D.M. Hodges, J.M. DeLong, C.F. Forney, R.K. Prange, Improving the thiobarbituric acidreactive-substances assay for estimating lipid peroxidation in plant tissues containing anthocyanin and other interfering compounds, Planta, 207 (1999) 604-611.
AC C
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M AN U
SC
RI PT
442
22
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
[21] M.C. Romero-Puertas, M. Rodríguez-Serrano, F.J. Corpas, M. Gómez, L.A. Del Río, L.M. Sandalio, Cadmium-induced subcellular accumulation of O2.- and H2O2 in pea leaves, Plant Cell Environ., 27 (2004) 1122-1134. [22] V. Alexieva, I. Sergiev, S. Mapelli, E. Karanov, The effect of drought and ultraviolet radiation on growth and stress markers in pea and wheat, Plant Cell Environ., 24 (2001) 1337-1344. [23] J. Rigaud, A. Puppo, Indole-3-acetic-acid catabolism by soybean bacteroids, J. Gen. Microbiol., 88 (1975) 223-228. [24] K.J. Livak, T.D. Schmittgen, Analysis of relative gene expression data using real-time quantitative PCR and the 2(T)(-Delta Delta C) method, Methods, 25 (2001) 402-408. [25] S. Li, H. Jin, Q. Zhang, The effect of exogenous spermidine concentration on polyamine metabolism and salt tolerance in zoysiagrass (Zoysia japonica steud) subjected to short-term salinity stress, Frontiers in Plant Science, 7 (2016). [26] W. Tang, R.J. Newton, Polyamines reduce salt-induced oxidative damage by increasing the activities of antioxidant enzymes and decreasing lipid peroxidation in Virginia pine, Plant Growth Regulation, 46 (2005) 31-43. [27] F. Palma, M. López-Gómez, N.A. Tejera, C. Lluch, Involvement of abscisic acid in the response of Medicago sativa plants in symbiosis with Sinorhizobium meliloti to salinity, Plant Science, 223 (2014) 16-24. [28] R. Radhakrishnan, I.-J. Lee, Ameliorative effects of spermine against osmotic stress through antioxidants and abscisic acid changes in soybean pods and seeds, Acta Physiol. Plant., 35 (2013) 263-269. [29] F. Palma, M. López-Gómez, N.A. Tejera, C. Lluch, Salicylic acid improves the salinity tolerance of Medicago sativa in symbiosis with Sinorhizobium meliloti by preventing nitrogen fixation inhibition, Plant Science, 208 (2013) 75-82. [30] A.W. Galston, R. Kaur-Sawhney, T. Altabella, A.F. Tiburcio, Plant polyamines in reproductive activity and response to abiotic stress, Botanica acta, 110 (1997) 197-207. [31] K. Lahiri, S. Chattopadhyay, B. Ghosh, Correlation of endogenous free polyamine levels with root nodule senescence in different genotypes in Vigna mungo L, J. Plant Physiol., 161 (2004) 563-571. [32] V. Vassileva, G. Ignatov, Polyamine-induced changes in symbiotic parameters of the Galega orientalis-Rhizobium galegae nitrogen-fixing system, Plant Soil, 210 (1999) 83-91. [33] R.C. Efrose, E. Flemetakis, L. Sfichi, C. Stedel, E.D. Kouri, M.K. Udvardi, K. Kotzabasis, P. Katinakis, Characterization of spermidine and spermine synthases in Lotus japonicus: induction and spatial organization of polyamine biosynthesis in nitrogen fixing nodules, Planta, 228 (2008) 37-49. [34] P.J. Zapata, M. Serrano, M.T. Pretel, A. Amorós, M.A. Botella, Polyamines and ethylene changes during germination of different plant species under salinity, Plant Science, 167 (2004) 781-788. [35] P. Roy, K. Niyogi, D.N. SenGupta, B. Ghosh, Spermidine treatment to rice seedlings recovers salinity stress-induced damage of plasma membrane and PM-bound H+-ATPase in salt-tolerant and salt-sensitive rice cultivars, Plant Science, 168 (2005) 583-591. [36] J.C. Cuevas, D.H. Sánchez, M. Marina, O.A. Ruiz, Do polyamines modulate the Lotus glaber NADPH oxidation activity induced by the herbicide methyl viologen?, Functional Plant Biology, 31 (2004) 921-928. [37] D.H. Sanchez, J.C. Cuevas, M.A. Chiesa, O.A. Ruiz, Free spermidine and spermine content in Lotus glaber under long-term salt stress, Plant Science, 168 (2005) 541-546. [38] M. López-Gómez, L. Cobos-Porras, J. Prell, C. Lluch, Homospermidine synthase contributes to salt tolerance in free-living Rhizobium tropici and in symbiosis with Phaseolus vulgaris, Plant Soil, 404 (2016) 413-425.
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[39] S. Fujihara, H. Abe, Y. Minakawa, S. Akao, T. Yoneyama, Polyamines in nodules from various plant-microbe symbiotic associations, Plant and Cell Physiology, 35 (1994) 11271134. [40] F.L. Shaw, K.A. Elliott, L.N. Kinch, C. Fuell, M.A. Phillips, A.J. Michael, Evolution and Multifarious Horizontal Transfer of an Alternative Biosynthetic Pathway for the Alternative Polyamine sym-Homospermidine, J. Biol. Chem., 285 (2010) 14711-14723. [41] S. Fujihara, Biogenic Amines in Rhizobia and Legume Root Nodules, Microbes and Environments, 24 (2009) 1-13. [42] A. Aziz, J. Martin-Tanguy, F. Larher, Salt stress-induced proline accumulation and changes in tyramine and polyamine levels are linked to ionic adjustment in tomato leaf discs, Plant Science, 145 (1999) 83-91. [43] M. Lopez-Gomez, J. Hidalgo-Castellanos, C. Iribarne, C. Lluch, Proline accumulation has prevalence over polyamines in nodules of Medicago sativa in symbiosis with Sinorhizobium meliloti during the initial response to salinity, Plant Soil, 374 (2014) 149-159. [44] J.F. Jimenez-Bremont, A. Becerra-Flora, E. Hernandez-Lucero, M. Rodriguez-Kessler, J.A. Acosta-Gallegos, J.G. Ramirez-Pimentel, Proline accumulation in two bean cultivars under salt stress and the effect of polyamines and ornithine, Biol. Plantarum, 50 (2006) 763-766. [45] K. Nahar, M. Hasanuzzaman, A. Rahman, M. Alam, J.A. Mahmud, T. Suzuki, M. Fujita, Polyamines confer salt tolerance in mung bean (Vigna Radiata l.) by reducing sodium uptake, improving nutrient homeostasis, antioxidant defense, and Methylglyoxal detoxification systems, Frontiers in Plant Science, 7 (2016). [46] S. Bhattacharjee, An inductive pulse of hydrogen peroxide pretreatment restores redoxhomeostasis and oxidative membrane damage under extremes of temperature in two rice cultivars, Plant Growth Regulation, 68 (2012) 395-410. [47] Q. Fariduddin, B.A. Mir, M. Yusuf, A. Ahmad, Comparative roles of brassinosteroids and polyamines in salt stress tolerance, Acta Physiol. Plant., 35 (2013) 2037-2053.
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ACCEPTED MANUSCRIPT 578 Table 1. Primer sequences of Medicago truncatula genes used for qRT-PCR. Oligonucleotide sequence
Product size
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Gene
Fw 5´-GTCGCGGTGGTTTGAATTCC-3´ Mt DET2
154 bp
SC
Rv 5´-AGTCCCAAATTCGGCATACC-3´
Fw 5´-TTCCATGTGGGTGGAAAGTC-3´ Mt DWF4
171 bp
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Rv 5´-GATCCTGCGCATAATCTTGG-3´
Fw 5´-CTGTGAAGTACCTCCATGAC-3´ Mt CYP85
162 bp
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Rv 5´-GTGGCCAATCTAGTTGTCTC-3´
Fw 5´-GGCCTGACGTAGAACTTATG-3´
Mt PAO1
312 bp
EP
Rv 5´-GCACGTAGCTTGTCATACAC-3´
Fw 5´-ATGGGGCAGAAGGATGCGTATG-3´ 115 bp
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Mt Actin
Rv 5´-AGCCTTCATAGATGGGGACCGT-3´
579
580
581
582
25
ACCEPTED MANUSCRIPT 583
Figure 1
584 0,30
SDW PSPA aa
587
aa
0,20
g plant-1
586
0,15
ab
bb
ab
c
b 0,06
0,10 0,05 0,00
0,00 Spd
Spm
C
M AN U
590 591
598
EP AC C
597
TE D
592
596
b
SC
C
595
a b
c
0,03
589
594
a
0,09
588
593
RDW PSR
0,12
RI PT
0,25
g plant-1
585
0,15
599 600 601
26
Spd
Spm
ACCEPTED MANUSCRIPT 602
Figure 2
603
NFR
b b
607 c
c
610
616 617
EP
615
AC C
614
25
c
C
Spm
TE D
611
613
b
b
M AN U
Spd
609
612
b b
0 C
a
c
0
608
50
RI PT
a
100
50
NFW mg plant-1
606
µmol N g-1 NFW h-1
605
75
150
SC
604
618 619 620
27
Spd
Spm
ACCEPTED MANUSCRIPT 621
Figure 3
622 623
5
AB
1,0
B
a a
a C
ab
0,5
b
C
C
b
4
a
0,0
b
2
SPM
Spd Spm
D
F E
C
638
C
Spd Spm
N
B C D E F
0,0 C
Spd Spm
L
nmols g-1 FW
AC C
HOMSPD A B C
6
D
D E
4 2 0 Spd Spm
L
C
Spd Spm
N
28
C
Spd Spm
N
10 8
A
CAD
0,5
N
C
639
Spd Spm
1,0
Spd Spm
EP
C
C
TE D
cd d
nmols g-1 FW
b c
L
637
D
b
L
B
a
1,0
0,0
636
E
A
1,5
632
635
C
N
0,5
634
C
1,5
d
633
Spd Spm
2,0
nmols g-1 FW
631
C
L
629 630
Spd Spm
b
M AN U
C
B
b
b
0
628
B
3
1
627
A
SPD
RI PT
626
PUT
SC
625
6 A
nmols g-1 FW
624
nmols g-1 FW
1,5
ACCEPTED MANUSCRIPT 640
Figure 4
641 642
PRO
643
645
a
a 1000
b 500
c
c
646 C
647 648
652 653 654 655
EP
651
AC C
650
Spd
TE D
649
c
M AN U
0
SC
644
nmol gFW -1
1500
RI PT
2000
656 657 658
29
Spm
ACCEPTED MANUSCRIPT 659
Figure 5
660 661
800
b 400
c
c
200
664
0
665 666 667
673 674
EP
672
AC C
671
TE D
668
670
Spd
c
Spm
M AN U
C
669
c
SC
µmol MDA gFW-1
663
600
RI PT
MDA
a 662
675 676 677
30
ACCEPTED MANUSCRIPT 678
Figure 6
679
A 680
20
µmol gFW -1
15
682
a b
10
5
684
0
d
685
B
TE D
687
689
Spd
692 693
AC C
691
NaCl
EP
Control 690
Spm
M AN U
C
688
bc
c
683
686
b
SC
681
RI PT
H2O2
Spd + NaCl
Spd
694 695 696
31
ACCEPTED MANUSCRIPT 697
Figure 7
698
25
25
DET2 20
10
c
5
Spd
CYP85
20 15
20
a
10
b
5
c
TE D
Fol change
C
a
b
c
Spd
Spm
25
707
b
b
0
Spd
b
Spm
AC C
EP
C
712
Spm
Fol change
705
b c
SC
C
25
711
10
0
704
710
a
5
0
703
709
15
d
d
708
Fol change
b
15
DWF4
20
c
702
706
a
M AN U
701
Fol change
700
RI PT
699
713
32
PAO1
15 10
a a
a
5
b b
b
0 C
Spd
Spm
ACCEPTED MANUSCRIPT Highlights 1. Exogenous polyamines increment nodule biomass and nitrogenase activity in the symbiosis Medicago truncatula-Sinorhizobium meliloti.
peroxidation under salt stress.
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2. Spermidine and spermine pre-treatments reduce the levels of H2O2 and lipid
3. Polyamines induce the expression of genes involved in brassinosteroids biosynthesis.
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4. Exogenous polyamines improve the response to salinity of the M.
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truncatula-S. meliloti symbiosis by reducing the oxidative damage.
ACCEPTED MANUSCRIPT Contribution
Miguel López Gómez: conceived and designed the experiments and wrote the
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manuscript. Javier Hidalgo-Castellanos: performed the experiments and analyzed the data.
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J. Rubén Muñoz-Sánchez: performed some of the experiments
Carmen Lluch Plá: Project leader
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Agustín J. Marín-Peña: performed some of the experiments
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José A. Herrera-Cervera: Project leader
S0981-9428(17)30146-8
DOI:
10.1016/j.plaphy.2017.04.024
Reference:
PLAPHY 4870
To appear in:
Plant Physiology and Biochemistry
Received Date: 24 January 2017 Revised Date:
24 April 2017
Accepted Date: 25 April 2017
Please cite this article as: M. López-Gómez, J. Hidalgo-Castellanos, J.Rubé. Muñoz-Sánchez, Agustí.J. Marín-Peña, C. Lluch, José.A. Herrera-Cervera, Polyamines contribute to salinity tolerance in the symbiosis Medicago truncatula-Sinorhizobium meliloti by preventing oxidative damage, Plant Physiology et Biochemistry (2017), doi: 10.1016/j.plaphy.2017.04.024. 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.
ACCEPTED MANUSCRIPT 1
Title
2
Polyamines contribute to salinity tolerance in the symbiosis Medicago truncatula-
3
Sinorhizobium meliloti by preventing oxidative damage.
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Authors
6
Miguel López-Gómez, Javier Hidalgo-Castellanos, J. Rubén Muñoz-Sánchez,
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Agustín J. Marín-Peña, Carmen Lluch, José A. Herrera-Cervera
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Departamento de Fisiología Vegetal, Facultad de Ciencias, Universidad de
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Granada, Campus de Fuentenueva s/n, 18071 Granada, Spain.
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Corresponding Author
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Miguel López-Gómez
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e-mail: [email protected]
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Departamento de Fisiología Vegetal, Facultad de Ciencias, Universidad de
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Granada, Campus de Fuentenueva s/n, 18071 Granada, Spain
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ACCEPTED MANUSCRIPT Abstract
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Polyamines (PAs) such as spermidine (Spd) and spermine (Spm) are small ubiquitous
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polycationic compounds that contribute to plant adaptation to salt stress. The positive
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effect of PAs has been associated to a cross-talk with other anti-stress hormones such as
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brassinoesteroids (BRs), also involved in anti-stress responses in plants. In this work we
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have studied the effects of exogenous Spd and Spm pre-treatments in the response to
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salt stress of the symbiotic interaction between Medicago truncatula and Sinorhizobium
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meliloti by analyzing parameters related to nitrogen fixation, oxidative damage and
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cross-talk with BRs in the response to salinity.
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Exogenous PAs treatments incremented the foliar and nodular Spd and Spm content
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which correlated with an increment of the nodule biomass and nitrogenase activity.
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Exogenous Spm treatment partially prevented proline accumulation which suggests that
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this polyamine could replace the role of this amino acid in the salt stress response.
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Additionally, Spd and Spm pre-treatments reduced the levels of H2O2 and lipid
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peroxidation under salt stress. PAs induced the expression of genes involved in the BRs
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biosynthesis which support a cross-talk between PAs and BRs in the salt stress response
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of the M. truncatula-S. meliloti symbiosis
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In conclusion, exogenous PAs improved the response to salinity of the M. truncatula-S.
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meliloti symbiosis by reducing the oxidative damage induced under salt stress
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conditions. In addition, in this work we provide evidences of the cross-talk between PAs
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and BRs in the adaptive responses to salinity.
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Keywords
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Polyamines, brassinosteroids, salt stress, symbiosis, Medicago truncatula.
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Abbreviations
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PAs, polyamines; BRs, brassinosteroids; Put, putrescine; Spd, spermidine; Spm,
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spermine; Cad, cadaverine; Homspd, homospermidine; MDA, malondialdehyde; Pro,
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proline; NFR, nitrogen fixation rate; NFW, nodule fresh weight.
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1. Introduction The diamine putrescine (Put) and the polyamines (PAs) spermidine (Spd) and spermine
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(Spm) are small ubiquitous polycations involved in numerous processes in all living
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organisms [1]. In plants, PAs are involved in cell division, embryogenesis, senescence,
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floral development and fruit ripening [2]. In addition, PAs play an important role in the
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response of plants to adverse environmental conditions due to their polycationic nature
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[3] [4]. Among these adverse conditions, soil salinity is one of the most important
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abiotic factors limiting crop productivity all over the world, especially in arid and
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semiarid regions, and is predicted to get worse under climate change conditions [5]. Salt
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stress adversely affects plant development and productivity by generating ion toxicity,
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osmotic stress, water deficits and oxidative damage through the production of reactive
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oxygen species (ROS) including hydrogen peroxide (H2O2) among others [6].
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Legumes are classified as salt-sensitive crop species and their productivity is
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particularly affected by soil salinity because nodular nitrogenase activity, responsible
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for the nitrogen supply to the plant in symbiosis with soil bacteria known as rhizobia,
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markedly decreases upon exposure to saline conditions [7] [8]. Root nodules of legumes
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have been found to contain a high variety and concentration of PAs, some of them of
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bacteroidal origin [9], however, little is known about the role of PAs within the root
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nodules. A cross-talk between PAs and other plant growth regulators such as
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brassinosteroids (BRs), has been described in the response to abiotic stresses [10], [11],
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[12]. BRs biosynthesis is regulated at the transcriptional level of the biosynthetic genes
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by other plant hormones such as auxin [13] and in addition, BRs have been shown to be
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involved in the systemic regulation of the root nodule formation in soybean [14] by a
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modification of the PAs levels in leaves [15].
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ACCEPTED MANUSCRIPT Exogenous addition of PAs has been extensively used as a strategy to enhance tolerance
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to salinity. There is a large body of evidence suggesting that exogenous application of
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PAs could preserve plant cell membrane integrity, minimize growth inhibition caused
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by stress, reduce superoxide radical and H2O2 contents and increase activities of
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antioxidant enzymes (reviewed by [2]).
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In this work we have studied the effects of exogenous Spd and Spm in the adaptation to
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salt stress of the symbiosis M. truncatula-S.meliloti by analyzing parameters related to
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nitrogen fixation, oxidative damage and cross-talk with BRs in the response to salinity.
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2. Material and Methods
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2.1 Biological material and growth conditions
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Medicago truncatula (var. Jemalong) seeds were scarified by immersion in concentrated
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H2SO4 for 5 min, washed with sterile water, surface sterilized by immersion in NaClO
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50% (v/v) plus Tween-20 for 10 min and germinated onto 1.0% water-agar plates at 25
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ºC in the darkness. After 3 days, Medicago seedlings were transferred to sterile
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vermiculite:perlite (3:1) and watered with a modified nitrogen free [16] nutrient
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solution. Two days later, M. truncatula seedlings were inoculated with S. meliloti 1021
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strain (c. 109 cell ml-1) grown in a TY medium.Plants, in individual pots of about 200
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ml, were grown in a controlled environmental chamber with a 16/8 h light-dark cycle,
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23/18ºC day night temperature, relative humidity 55/65% and photosynthetic photon
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flux density (400-700 nm) of 450 µmol m-2 s-1 supplied by combined fluorescent and
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incandescent lamps. Six weeks after sowing plants were subjected to Spd and Spm
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treatments by the addition of 0.1 mM of each polyamine to the nutrient solution.
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Control plants were watered with the same nutrient solution without polyamines. Salt
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nutrient solution. Control plants were watered with a NaCl-free nutrient solution. Plants
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were harvested 10 weeks after sowing with polyamines and NaCl treatments lasting 4
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and 2 weeks, respectively. Nodules and leaves were frozen at -80 ºC for further
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analyses. Samples of leaves, stems and roots were dried at 70 ºC for 24 h and their dry
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weight determined.
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2.2 Nitrogen fixation
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Nitrogenase activity (E.C. 1.7.9.92) was measured as the representative H2-evolution in
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an open-flow system [17] using an electrochemical H2 sensor (Qubit System Inc.,
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Canada). H2 production was recorded in intact nodulated roots of plants. Apparent
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nitrogenase activity (ANA, rate of H2 production in air) was determined under N2:O2
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(80%:20%) with a total flow of 0.4 l min-1. After reaching steady-state conditions total
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nitrogenase activity (TNA) was determined under Ar:O2 (79%:21%). Nitrogen fixation
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rate (NFR) was calculated as (TNA-ANA)/3. Standards of high purity H2 were used to
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calibrate the detector.
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2.3 Determination of free polyamines in leaves and nodules
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Nodule and leaves extracts were prepared from 0.2 g of fresh tissue with 0.6 ml of 5%
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(v/v) cold perchloric acid (PCA) and incubated 24 h at 4 ºC. The homogenate was
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centrifuged (3,000xg, 5 min, 4 ºC) and 0.2 ml aliquots of the supernatant were
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dansylated as described below. The analysis of free PAs was performed with HPLC
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(Agilent Technologies 1260) equipped with a reverse phase column (4.6 x 250 mm
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ACCEPTED MANUSCRIPT C18) after derivatization with dansyl chloride (Sigma). Derivatization was performed by
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mixing 0.2 ml aliquots of the extracts prepared as described above with 0.4 ml of dansyl
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chloride (prepared fresh in acetone, 10 mg/ ml) and 0.2 ml of saturated sodium
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carbonate. After brief vortexing, the mixture was incubated in darkness at room
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temperature overnight. Excess dansyl reagent was removed by reaction with 0.1 ml (100
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mg/ml) of added proline, and incubation for 30 min. Dansylpolyamines were extracted
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in 0.5 ml toluene. The organic phase was collected and evaporated to dryness under a
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stream of nitrogen, and redissolved in 0.1 ml acetonitrile.
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Column flow was 1.5 ml min-1 and the elution gradient was prepared with eluent A
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(water) and eluent B (acetonitrile). The column was equilibrated with 70% B and 30%
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A before injecting 0.01 ml samples. This was followed by a linear gradient ending with
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100% B after 9 min. The final step was held for 4 min before regenerating the column.
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Detection was done with a fluorometer using excitation and emission wavelengths of
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415 and 510 nm, respectively, according to [18]. A relative calibration procedure was
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used to determine the PAs in the samples, using 1,7- diaminoheptane (HTD) as internal
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standard and PAs standards amounts ranging from 0.3 to 1.5 nmol purchased from
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Sigma. Results were expressed as nmol g-1 fresh weight.
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2.4 Proline determination
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Proline was determined by the ninhydrine method [19]. Briefly, 250 mg of plant
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material was homogenized in 3 ml of 95% (v/v) ethanol at room temperature and
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centrifuged at 2,000 x g for 5 min. 300 µl of distilled water and 2 ml of ninhydrine
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reagent were added to an aliquot of 200 µl of extract. The mixture was boiled for 60
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min, and the reaction was stopped in an ice bath. The chromophore obtained was 7
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extracted with 6 ml of toluene by vigorous shaking for 20 s. Absorbance of the resulting
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organic layer was measured at 520 nm with Varian UV-VIS spectrophotometer.
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Calibration was made using L-Pro as a standard.
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2.5 Lipid peroxidation
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Lipid peroxidation was measured by the level of malondialdehyde (MDA), a product of
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lipid peroxidation, using a reaction with thiobarbituric acid (TBA) as described by [20].
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Fresh samples (100 mg) were ground in a mixture of 1 ml trichloroacetic acid (TCA)
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(20% w/v) and 0.2 ml of 4% (w/v) butylatedhidroxytoluene in ethanol, at 4 ºC. After
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centrifugation (10,000 x g for 15 min), 0.25 ml aliquots of the supernatant were mixed
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with 0.75 ml of 0.5% (w/v) thiobarbituric acid in 20% TCA and the mixture was
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incubated at 94 ºC for 30 min. The reaction was stopped by cooling in an ice bath for 15
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min. Reaction tubes were centrifuged at 10,000 x g for 15 min and supernatants were
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used to determine the absorbance at 532 nm. The value for non-specific absorption at
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600 nm was subtracted.
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2.6 Histochemical and quantitative detection of H2O2 in leaves
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The histochemical analysis of H2O2 was performed in leaves of two weeks old plants
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grown axenically in glass test tubes. Plants were pretreated with Spm 0.1 mM 24 h
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before treatment with NaCl to a final concentration of 150 mM for 24h. The H2O2 was
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localized histochemically by staining leaves with 1% 3,3-diaminobenzidine (DAB)
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solution. Leaves were immersed in such solution until brown spots appeared due to the
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boiling ethanol to see the spots.
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Quantitative analysis of H2O2 was performed spectrophotometrically after reaction with
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KI [22]. The reaction mixture consisted of 0.5 ml 0.1% trichloroacetic acid (TCA) leaf
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extract supernatant, 0.5 mL of 100 mM K-phosphate buffer and 2 mL reagent (1 M KI
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w/v in fresh double-distilled water H2O). The blank probe consisted of 0.1% TCA in the
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absence of leaf extract. The reaction was developed for 1 h in darkness and absorbance
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measured at 390 nm. The amount of H2O2 was calculated using a standard curve
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prepared with known concentrations of H2O2.
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2.7 Gene expression analysis in leaves
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For gene expression analysis, plants were grown axenically onto filter paper in glass test
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tubes containing 10 ml of nutrient solution [23]. Two weeks after sowing, plants were
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pre-treated with Spd and Spm to a final concentration of 0.1 mM for 24h and then, NaCl
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to a final concentration of 150 mM was added. After 48h and 24h of PAs and NaCl
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treatments, respectively, plants were harvested and frozen at -80 ºC. A total of 6 plants
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per repetition and treatment were used for RNA preparation.
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Total RNA was extracted using an RNeasy plant mini kit (Macherey-Nagel, Germany)
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followed by treatment with DNaseI (Ambion, Texas, USA) for genomic DNA removal.
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First-strand cDNA was reverse transcribed from 1.5 µg of DNase-treated total RNA. All
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DNase-treated total RNA samples were denatured at 65 ºC for 5 min followed by quick
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chill on ice in 12 µl of reaction mixture containing 0.5 µg oligo-dT adapter primers and
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1 µl of 10 Mm deoxy-nucleotide triphosphate.
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inhibitor and 2 µl of 0.1 M dithiothreitol (DTT), the reaction was preheated at 37 ºC for
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3 min before the addition of 1 µl (200 U) of iScript reverse transcriptase (Bio-Rad,
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California, USA). The reaction mixture was incubated at 42 ºC for 50 min, followed by
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heat inactivation at 70 ºC for 15 min. The resulted first strand cDNA was amplified
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using gene specific primers (Table 1) designed from the transcribed region of each gene
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by using the Clone Manager Professional Suite software. The actin gene was used as
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loading control.
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PCR amplifications were performed in 20 µl reactions mixture as follows: one cycle of
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2 min at 94 ºC, 35 cycles of 30 s at 94 ºC, 30 s at 56 ºC and 1 min at 72 ºC and a final
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extension at 72 ºC for 10 min. PCR products were electrophoretically separated in 1%
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(w/v) agarose gels. Real-time PCR (qPCR) was performed using a SYBR Green PCR
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Master kit containing the Platinum Taq DNA polymerase (Invitrogen) on an iCycler IQ
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thermocycler (Bio-Rad). PCR amplification mixtures contained 10 ng of template
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cDNA and 0.5 U of polymerase. The cycling conditions were chosen according to the
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manufacturer. They comprised 10 min polymerase activation at 95 ºC and 35 cycles at
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95 ºC for 15 s, 55 ºC for 30 s and 72 ºC for 20 s. Results were quantified with the DDCt
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method [24]. Transcript levels were normalised to actin gene expression. The primer
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sequences for qPCR analysis are provided in Table 1.
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2.8 Statistical analysis
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Experiments were arranged in a completely randomized design with totally 60 plants
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per treatment. The data were subjected to an analysis of two-way ANOVA with
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exogenous polyamines as one factor and salt treatment as the other using the 10
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significant differences between treatments were determined by LSD (P ≤ 0.05).
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Experiments were performed three times in triplicate. Mean values ± SE error bars are
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3. Results
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3.1 Exogenous PAs induce plant growth
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Exogenous addition of Spd and Spm increased plant biomass about 43% with the same
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effect in shoots and roots (Fig. 1). Under salt stress conditions, the effect of PAs
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treatment was similar on the SDW and higher on RDW which incremented by 57%. Salt
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treatment provoked a plant growth inhibition more significant in roots than in shoots
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with a 40% and 20% reduction, respectively. Pre-treatments with PAs did not modify
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the response to salinity in shoots and roots.
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3.2 Nitrogenase activity is increased by exogenous PAs
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Nitrogen fixation rate (NFR), evaluated through the nitrogenase activity and the nodule
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fresh weight (NFW) is shown in Fig. 2. In general, NFR was highly increased by the
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Spd treatment with 2.6 fold increment. Additionally, under salt stress conditions the
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effect of both PAs was even greater, which led to a reduction of the salinity inhibitory
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effect from 11 to 10 and 3 times with Spd and Spm, respectively. Nodule biomass was
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also induced by the Spd and Spm treatments with 44% and 32% increment,
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respectively. This effect was even higher under salt stress with double nodule biomass
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in plants co-treated with PAs and NaCl. Salinity provoked a NFW reduction of 40%
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while this effect was reduced to 20% with Spd and 4% with Spm.
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3.3 Nodule specific PAs accumulate under salt stress
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Content of PAs in leaves and nodules were analyzed in order to compare the effect of
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exogenous Spd and Spm in both tissues under salt stress as shown in Fig. 3. In general,
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the levels of PAs were higher in nodules, which also display a more complex PA profile
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because they contain nodule-specific PAs such as cadaverine (Cad) and
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homospermidine (Homspd). Exogenous Spd and Spm treatments provoked an
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increment of both PAs of about 50% in leaves. Under salt stress conditions, Spm was
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the only polyamine that accumulated in leaves, with 30% and 46% increment in control
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and Spm treated plants. Put levels did not show differences by PAs treatment in leaves
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but NaCl provoked a reduction that ranged from 50% to 2.7 fold. Spd showed a similar
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response to salt stress while Spm was the only polyamine that accumulated in salt-
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stressed leaves. A similar result was detected for Spm in nodules, although in addition
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to this polyamine, Cad doubled its concentration under salinity, independently of the co-
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treatment with exogenous Spd and Spm. Homspd was the most abundant polyamine in
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nodules and under salt stress increased between 37% and 16% depending on the
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exogenous polyamine treatment. Put and Spd responses to salinity in nodules were
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similar to the observed in leaves with significant reductions under salt stress conditions.
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3.4 Proline accumulation is partially prevented by exogenous Spm
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the PAs metabolism and the synthesis of this amino acid. Salt stress induced a dramatic
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increase in the Pro levels in leaves with 3.6 fold higher concentration in such conditions
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(Fig. 4). However, the co-treatment with Spm partially inhibited the accumulation of
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Pro, which only showed a 76% induction by the salinity compared with the 3.6 fold
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induction observed in the absence of the PAs co-treatment. On the contrary, Spd did not
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induce any effect on the Pro accumulation by the salinity.
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3.5 Lipid peroxidation is inhibited by exogenous PAs
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Lipid peroxidation, estimated as the malondialdehyde (MDA) concentration in leaves
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(Fig. 5), was prevented by the exogenous treatment with Spd and Spm. Salt stress
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provoked a 2.5 fold increment in the MDA levels, however, with the exogenous Spd
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and Spm treatment this increment was 25% and 43%, respectively. In control
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conditions, no differences in the MDA levels were induced by the exogenous treatments
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with PAs.
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3.6 H2O2 production is reduced by exogenous PAs under salt stress
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H2O2 content in leaves was evaluated in a quantitative and in a semi-quantitative way in
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leaves as shown in Fig. 6A, B. The quantitative assay revealed that the level of H2O2
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was incremented by 3 times under salt stress conditions. However, pre-treatments with
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PAs reduced this increment to 30% with Spd and it was even completely abolished with
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Spm. Interestingly, the treatment with Spd and Spm produced an induction of H2O2 of
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40% and 2.5 times, respectively. The histochemical assay showed similar results to the
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quantitative assay with an increment of H2O2 in the salt stressed leaves and a slight
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reduction of this effect by the pretreatment with Spd.
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3.7 Exogenous PAs induce the synthesis of Brassinosteroids
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Expression level of genes involved in the synthesis of BRs DET2 (De-etiolated 2),
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DWF4 (Dwarf 4) and CYP85 were analyzed in leaves in order to determine a possible
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interaction between PAs and BRs metabolism (Fig. 7). Additionally, the expression of
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PAO1 (Polyamine oxidase 1) responsible of the Spd and Spm catabolism was analyzed.
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In general, all genes implicated in the synthesis of BRs were induced under salt stress
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conditions with 2 to 5 fold increment in the expression level. Exogenous treatments
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with PAs also induced the transcription level of the BRs biosynthetic genes to a higher
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extend with Spm which incremented 8 to 17 times the expression of the three genes
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analyzed. Nevertheless, the positive effect of Spd on the expression levels was
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completely abolished by salt stress and partially by the Spm treatment, except for
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DWF4 that did not show a significant difference. PAO1 transcription level was induced
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by Spd and Spm as well, while no significant differences were induced by the salt
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treatment.
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4. Discussion
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Exogenous application of PAs has been extensively shown to enhance tolerance to
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salinity stress in plants by scavenging free radicals, stabilizing membrane and cellular
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structures and modulating ion channels among other effects [25]; [3]; [26]. The positive
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effect of PAs has been associated to a cross-talk with other anti-stress hormones such as
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ACCEPTED MANUSCRIPT abcisic acid [27]; [28] salicylic acid [29], ethylene [30] or BRs [10, 12]. Indeed, the
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establishment of symbiosis between legumes and rhizobium has been shown to be
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influenced by the regulation of the PAs levels by a systemic effect of BRs on root
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nodule formation [15]. Those previous discoveries led us to study the effect of
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exogenous PAs (Spd and Spm) on the response to salinity of M. truncatula-S. meliloti
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symbiosis and its possible interaction with the BRs biosynthetic genes.
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Treatments with Spd and Spm increased plant growth, having similar effects on SDW
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and RDW (Fig. 1). This effect of exogenous PAs would be related with their growth
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regulatory capacity which includes DNA replication, cell division and root growth [3]
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Together with the increment in plant biomass, exogenous PAs incremented also nodule
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nitrogenase activity (Fig. 2).This could be also involved in the plant growth promotion
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due to a higher nitrogen supply to the plant. In that sense, a linear correlation between
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the concentration of PAs in nodules and nitrogenase activity has been shown [31].The
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increment of nitrogenase activity was accompanied by an increment of the nodule fresh
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weight as previously shown in Galega orientalis-Rhizobium galegae symbiosis [32].
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This effect could be related to a regulatory role of PAs in the nodulation process, as
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suggested by [33] in Lotus japonicus, where the expression of PAs biosynthetic genes
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(Spds and Spms) was maximal at early stages of nodule development.
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Under salt stress conditions Put and Spd levels were lower in leaves independently of
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the exogenous addition of PAs, while Spm augmented 32% in control plants and 46% in
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Spm treated plants (Fig. 3). In general, an increment in the (Spd+Spm)/Put ratio has
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been reported to be related with salinity tolerance in most cases [34]. In addition, Spm
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seems to participate on membrane modulation of permeability and stability [35]
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reducing radical generation under oxidative stress [36]. In that sense, Spm accumulation
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has been considered a general feature of plant response to salinity [37]. Exogenous Spd
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ACCEPTED MANUSCRIPT and Spm treatments increased foliar Spd and Spm levels by 50% and 70%, respectively,
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which indicates a transport of these PAs from the root to the shoot. Nodule PAs analysis
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revealed the presence of uncommon PAs such as Cad and Homspd, characteristics of
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nodules of legumes such as M. truncatula [38] or Phaseolus vulgaris [9]. In addition,
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the levels of all PAs were higher in nodules than in leaves, as described by [39], with
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Homspd as the most abundant PA synthesized by the bacteroids [38]. Similarly to
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leaves, exogenous Spd and Spm treatments incremented the nodular content of both
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PAs which correlated with an increment of the nodule biomass (NFW) and nitrogenase
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activity (NFR), suggesting the implication of Spd and Spm in the improvement of the
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symbiosis effectiveness. Nevertheless, Cad and Homspd levels declined by the
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exogenous addition of the common PAs (Spd and Spm), which might be due to the
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replacement of these uncommon PAs by Spd and Spm, since the exact structure of these
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compounds has been shown not to be critical for their function [40]. Interestingly, the
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concentration of nodule specific PAs (Cad and Homspd) augmented under salt stress
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due to the implication of Homspd in the stress tolerance of fast-growing rhizobia [41].
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Proline accumulation is considered one of the most commonly adaptive responses of
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plants to salinity due to its antioxidant and osmo-compatible properties [42].
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Additionally, polyamine metabolism exerts a direct or indirect action on proline
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metabolism through PAs degradation, which could contribute to proline accumulation,
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or by the competition of both metabolites by glutamate as common precursor [43]. In
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this context, salt stress strongly induced proline accumulation in M. truncatula leaves
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(Fig 4) which suggest prevalence of this amino acid over PAs in the response to salinity
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as previously described in Medicago sativa nodules [43]. Nevertheless, exogenous Spm
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treatment partially prevented proline accumulation which together to the Spm
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accumulation under salinity suggests that in such conditions, this polyamine could
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by [44] who reported that exogenous PAs decreased Pro accumulation in salinity
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exposed Phaseolus vulgaris plants.
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In addition to the primary effects, salinity leads to oxidative stress through an increase
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of reactive oxygen species (ROS) such as hydrogen peroxide (H2O2), which cause lipid
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peroxidation and disturb cellular membrane functioning. The H2O2 level increased
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significantly upon salt stress exposure (Fig. 6A), which indicated higher oxidative stress
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in these plants. MDA, a lipid peroxidation product, served as the indicator of the extent
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oxidative damage in salt stressed plants in this study (Fig. 5). Spd and Spm pre-
360
treatments reduced the levels of H2O2 and MDA during salt stress. These results agree
361
with previous studies [25]; [45] and suggest that PAs serve as efficient ROS scavenger
362
and membrane stabilizers by the MDA reduction under salt stress. However, at low
363
concentrations, H2O2 is known to prevent oxidative damage by up-regulating
364
antioxidative defence enzymes and by restoring redox homeostasis [46] which make
365
vital to keep the level of H2O2 rather than removing it. In that sense, visual
366
identification of H2O2 detected by histochemical staining (Fig. 6B) as well as the
367
quantitative analysis reflected a moderate increment of H2O2 in Spd and Spm treated
368
plants.
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The beneficial effects of PAs in the response to salinity have been associated to a cross-
370
talk with other plant growth regulators such as BRs [47]. Indeed, in a previous study we
371
found that the salt stress ameliorative effect of 24-epibrassinolide in the M. truncatula-
372
S. meliloti symbiosis was mediated by PAs [10]. In that sense, we found that exogenous
373
PAs induced the expression of genes involved in the BRs biosynthesis (Fig. 7) which
374
support a cross-talk between PAs and BRs in the salt stress response of the M.
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truncatula-S. meliloti symbiosis.
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ACCEPTED MANUSCRIPT In conclusion, exogenous PAs improved the response to salinity of the M. truncatula-S.
377
meliloti symbiosis by reducing the nitrogenase inhibition as well as the oxidative
378
damage induced under salt stress conditions. Additionally, in this work we provide
379
evidences of the cross-talk between PAs and BRs in the adaptive responses to salinity.
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380
Aknowledgements
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This work has been supported by the Andalusian Research Program (AGR-139) and the
383
Spanish Ministry of Science and Technology (Grant: AGL2013-42778-P).
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ACCEPTED MANUSCRIPT Figure legends
397
Figure 1
398
Effect of exogenous Spd and Spm on shoot dry weight (SDW) and root dry weight
399
(RDW) of M. truncatula plants inoculated with S. meliloti under control (white bars)
400
and salt stress conditions (grey bars). Data are means + SE (n=10). Mean values
401
followed by the same letter do not differ (p<0.05) using the LSD test.
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Figure 2
404
Effect of exogenous Spd and Spm on nitrogen fixation rate (NFR) and nodule fresh
405
weight (NFW) of M. truncatula plants inoculated with S. meliloti under control (white
406
bars) and salt stress conditions (grey bars). Data are means + SE (n=10). Mean values
407
followed by the same letter do not differ (p<0.05) using the LSD test.
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Figure 3
410
Effect of exogenous Spd and Spm on polyamines content (Put, putrescine; Spd,
411
spermidine; Spm, spermine; Cad, cadaverine; Homspd, homospermidine) in M.
412
truncatula leaves (L) and nodules (N) inoculated with S. meliloti under control (white
413
bars) and salt stress conditions (grey bars). Data are means + SE (n=4). Mean values
414
followed by the same letter do not differ (p<0.05) using the LSD test.
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Figure 4
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ACCEPTED MANUSCRIPT Effect of exogenous Spd and Spm on proline content (Pro) in leaves of M. truncatula
418
inoculated with S. meliloti under control (white bars) and salt stress conditions (grey
419
bars). Data are means + SE (n=4). Mean values followed by the same letter do not differ
420
(p<0.05) using the LSD test.
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Figure 5
423
Effect of exogenous Spd and Spm on malondialdehyde content (MDA) in leaves of M.
424
truncatula inoculated with S. meliloti under control (white bars) and salt stress
425
conditions (grey bars). Data are means + SE (n=4). Mean values followed by the same
426
letter do not differ (p<0.05) using the LSD test.
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Figure 6
429
Effect of exogenous Spd and Spm on (A) H2O2 content in leaves of M. truncatula
430
inoculated with S. meliloti under control (white bars) and salt stress conditions (grey
431
bars). Data are means + SE (n=4). Mean values followed by the same letter do not differ
432
(p<0.05) using the LSD test. (B) DAB staining of H2O2 in leaves of M. truncatula
433
inoculated with S. meliloti and treated or not with NaCl and Spd.
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Figure 7
436
Effect of exogenous Spd and Spm on expression level of DET2, DWF4, CYP85 and
437
PAO1 genes in leaves of M. truncatula inoculated with S. meliloti under control (white
20
ACCEPTED MANUSCRIPT 438
bars) and salt stress conditions (grey bars). Data are means + SE (n=4). Mean values
439
followed by the same letter do not differ (p<0.05) using the LSD test.
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ACCEPTED MANUSCRIPT References
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[1] A. Bouchereau, A. Aziz, F. Larher, J. Martin-Tanguy, Polyamines and environmental challenges: recent development, Plant Science, 140 (1999) 103-125. [2] S.S. Hussain, M. Ali, M. Ahmad, K.H.M. Siddique, Polyamines: Natural and engineered abiotic and biotic stress tolerance in plants, Biotechnol. Adv., 29 (2011) 300-311. [3] R. Alcazar, T. Altabella, F. Marco, C. Bortolotti, M. Reymond, C. Koncz, P. Carrasco, A.F. Tiburcio, Polyamines: molecules with regulatory functions in plant abiotic stress tolerance, Planta, 231 (2010) 1237-1249. [4] J.H. Liu, H. Kitashiba, J. Wang, Y. Ban, T. Moriguchi, Polyamines and their ability to provide environmental stress tolerance to plants, Plant Biotechnology, 24 (2007) 117-126. [5] J. Rozema, T. Flowers, Ecology: Crops for a salinized world, Science, 322 (2008) 14781480. [6] R. Munns, M. Tester, Mechanisms of Salinity Tolerance, Annu. Rev. Plant Biol., 59 (2008) 651-681. [7] M. López, J.A. Herrera-Cervera, C. Iribarne, N.A. Tejera, C. Lluch, Growth and nitrogen fixation in Lotus japonicus and Medicago truncatula under NaCl stress: Nodule carbon metabolism, J. Plant Physiol., 165 (2008) 641-650. [8] I. Aranjuelo, C. Arrese-Igor, G. Molero, Nodule performance within a changing environmental context, J. Plant Physiol., 171 (2014) 1076-1090. [9] M. López-Gómez, L. Cobos-Porras, J. Hidalgo-Castellanos, C. Lluch, Occurrence of polyamines in root nodules of Phaseolus vulgaris in symbiosis with Rhizobium tropici in response to salt stress, Phytochemistry, 107 (2014) 32-41. [10] M. López-Gómez, J. Hidalgo-Castellanos, C. Lluch, J.A. Herrera-Cervera, 24Epibrassinolide ameliorates salt stress effects in the symbiosis Medicago truncatulaSinorhizobium meliloti and regulates the nodulation in cross-talk with polyamines, Plant Physiology and Biochemistry, 108 (2016) 212-221. [11] S.P. Choudhary, H.V. Oral, R. Bhardwaj, J.Q. Yu, L.S.P. Tran, Interaction of brassinosteroids and polyamines enhances copper stress tolerance in raphanus sativus, J. Exp. Bot., 63 (2012) 5659-5675. [12] Q. Zheng, J. Liu, R. Liu, H. Wu, C. Jiang, C. Wang, Y. Guan, Temporal and spatial distributions of sodium and polyamines regulated by brassinosteroids in enhancing tomato salt resistance, Plant Soil, 400 (2016) 147-164. [13] Y. Chung, P.M. Maharjan, O. Lee, S. Fujioka, S. Jang, B. Kim, S. Takatsuto, M. Tsujimoto, H. Kim, S. Cho, T. Park, H. Cho, I. Hwang, S. Choe, Auxin stimulates DWARF4 expression and brassinosteroid biosynthesis in Arabidopsis, Plant J., 66 (2011) 564-578. [14] J. Terakado, T. Yoneyama, S. Fujihara, Shoot-applied polyamines suppress nodule formation in soybean (Glycine max), J. Plant Physiol., 163 (2006) 497-505. [15] J. Terakado-Tonooka, S. Fujihara, Involvement of polyamines in the root nodule regulation of soybeans (Glycine max), Plant Root, 2 (2008) 46-53. [16] A. Puppo, J. Rigaud, Indole-3-acetic-acid (IAA) oxidation by leghemoglobin from soybean nodules, Physiol. Plantarum, 35 (1975) 181-185. [17] J.F. Witty, F.R. Minchin, Hydrogen measurements provide direct evidence for a variable physical barrier to gas diffusion in legume nodules, J. Exp. Bot., 49 (1998) 1015-1020. [18] H.E. Flores, A.W. Galston, Analysis of Polyamines in Higher Plants by High Performance Liquid Chromatography, Plant Physiol., 69 (1982) 701-706. [19] W. Troll, J. Lindsley, A photometric method for the determination of proline, J. Biol. Chem., 215 (1955) 655-660. [20] D.M. Hodges, J.M. DeLong, C.F. Forney, R.K. Prange, Improving the thiobarbituric acidreactive-substances assay for estimating lipid peroxidation in plant tissues containing anthocyanin and other interfering compounds, Planta, 207 (1999) 604-611.
AC C
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M AN U
SC
RI PT
442
22
ACCEPTED MANUSCRIPT
EP
TE D
M AN U
SC
RI PT
[21] M.C. Romero-Puertas, M. Rodríguez-Serrano, F.J. Corpas, M. Gómez, L.A. Del Río, L.M. Sandalio, Cadmium-induced subcellular accumulation of O2.- and H2O2 in pea leaves, Plant Cell Environ., 27 (2004) 1122-1134. [22] V. Alexieva, I. Sergiev, S. Mapelli, E. Karanov, The effect of drought and ultraviolet radiation on growth and stress markers in pea and wheat, Plant Cell Environ., 24 (2001) 1337-1344. [23] J. Rigaud, A. Puppo, Indole-3-acetic-acid catabolism by soybean bacteroids, J. Gen. Microbiol., 88 (1975) 223-228. [24] K.J. Livak, T.D. Schmittgen, Analysis of relative gene expression data using real-time quantitative PCR and the 2(T)(-Delta Delta C) method, Methods, 25 (2001) 402-408. [25] S. Li, H. Jin, Q. Zhang, The effect of exogenous spermidine concentration on polyamine metabolism and salt tolerance in zoysiagrass (Zoysia japonica steud) subjected to short-term salinity stress, Frontiers in Plant Science, 7 (2016). [26] W. Tang, R.J. Newton, Polyamines reduce salt-induced oxidative damage by increasing the activities of antioxidant enzymes and decreasing lipid peroxidation in Virginia pine, Plant Growth Regulation, 46 (2005) 31-43. [27] F. Palma, M. López-Gómez, N.A. Tejera, C. Lluch, Involvement of abscisic acid in the response of Medicago sativa plants in symbiosis with Sinorhizobium meliloti to salinity, Plant Science, 223 (2014) 16-24. [28] R. Radhakrishnan, I.-J. Lee, Ameliorative effects of spermine against osmotic stress through antioxidants and abscisic acid changes in soybean pods and seeds, Acta Physiol. Plant., 35 (2013) 263-269. [29] F. Palma, M. López-Gómez, N.A. Tejera, C. Lluch, Salicylic acid improves the salinity tolerance of Medicago sativa in symbiosis with Sinorhizobium meliloti by preventing nitrogen fixation inhibition, Plant Science, 208 (2013) 75-82. [30] A.W. Galston, R. Kaur-Sawhney, T. Altabella, A.F. Tiburcio, Plant polyamines in reproductive activity and response to abiotic stress, Botanica acta, 110 (1997) 197-207. [31] K. Lahiri, S. Chattopadhyay, B. Ghosh, Correlation of endogenous free polyamine levels with root nodule senescence in different genotypes in Vigna mungo L, J. Plant Physiol., 161 (2004) 563-571. [32] V. Vassileva, G. Ignatov, Polyamine-induced changes in symbiotic parameters of the Galega orientalis-Rhizobium galegae nitrogen-fixing system, Plant Soil, 210 (1999) 83-91. [33] R.C. Efrose, E. Flemetakis, L. Sfichi, C. Stedel, E.D. Kouri, M.K. Udvardi, K. Kotzabasis, P. Katinakis, Characterization of spermidine and spermine synthases in Lotus japonicus: induction and spatial organization of polyamine biosynthesis in nitrogen fixing nodules, Planta, 228 (2008) 37-49. [34] P.J. Zapata, M. Serrano, M.T. Pretel, A. Amorós, M.A. Botella, Polyamines and ethylene changes during germination of different plant species under salinity, Plant Science, 167 (2004) 781-788. [35] P. Roy, K. Niyogi, D.N. SenGupta, B. Ghosh, Spermidine treatment to rice seedlings recovers salinity stress-induced damage of plasma membrane and PM-bound H+-ATPase in salt-tolerant and salt-sensitive rice cultivars, Plant Science, 168 (2005) 583-591. [36] J.C. Cuevas, D.H. Sánchez, M. Marina, O.A. Ruiz, Do polyamines modulate the Lotus glaber NADPH oxidation activity induced by the herbicide methyl viologen?, Functional Plant Biology, 31 (2004) 921-928. [37] D.H. Sanchez, J.C. Cuevas, M.A. Chiesa, O.A. Ruiz, Free spermidine and spermine content in Lotus glaber under long-term salt stress, Plant Science, 168 (2005) 541-546. [38] M. López-Gómez, L. Cobos-Porras, J. Prell, C. Lluch, Homospermidine synthase contributes to salt tolerance in free-living Rhizobium tropici and in symbiosis with Phaseolus vulgaris, Plant Soil, 404 (2016) 413-425.
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[39] S. Fujihara, H. Abe, Y. Minakawa, S. Akao, T. Yoneyama, Polyamines in nodules from various plant-microbe symbiotic associations, Plant and Cell Physiology, 35 (1994) 11271134. [40] F.L. Shaw, K.A. Elliott, L.N. Kinch, C. Fuell, M.A. Phillips, A.J. Michael, Evolution and Multifarious Horizontal Transfer of an Alternative Biosynthetic Pathway for the Alternative Polyamine sym-Homospermidine, J. Biol. Chem., 285 (2010) 14711-14723. [41] S. Fujihara, Biogenic Amines in Rhizobia and Legume Root Nodules, Microbes and Environments, 24 (2009) 1-13. [42] A. Aziz, J. Martin-Tanguy, F. Larher, Salt stress-induced proline accumulation and changes in tyramine and polyamine levels are linked to ionic adjustment in tomato leaf discs, Plant Science, 145 (1999) 83-91. [43] M. Lopez-Gomez, J. Hidalgo-Castellanos, C. Iribarne, C. Lluch, Proline accumulation has prevalence over polyamines in nodules of Medicago sativa in symbiosis with Sinorhizobium meliloti during the initial response to salinity, Plant Soil, 374 (2014) 149-159. [44] J.F. Jimenez-Bremont, A. Becerra-Flora, E. Hernandez-Lucero, M. Rodriguez-Kessler, J.A. Acosta-Gallegos, J.G. Ramirez-Pimentel, Proline accumulation in two bean cultivars under salt stress and the effect of polyamines and ornithine, Biol. Plantarum, 50 (2006) 763-766. [45] K. Nahar, M. Hasanuzzaman, A. Rahman, M. Alam, J.A. Mahmud, T. Suzuki, M. Fujita, Polyamines confer salt tolerance in mung bean (Vigna Radiata l.) by reducing sodium uptake, improving nutrient homeostasis, antioxidant defense, and Methylglyoxal detoxification systems, Frontiers in Plant Science, 7 (2016). [46] S. Bhattacharjee, An inductive pulse of hydrogen peroxide pretreatment restores redoxhomeostasis and oxidative membrane damage under extremes of temperature in two rice cultivars, Plant Growth Regulation, 68 (2012) 395-410. [47] Q. Fariduddin, B.A. Mir, M. Yusuf, A. Ahmad, Comparative roles of brassinosteroids and polyamines in salt stress tolerance, Acta Physiol. Plant., 35 (2013) 2037-2053.
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ACCEPTED MANUSCRIPT 578 Table 1. Primer sequences of Medicago truncatula genes used for qRT-PCR. Oligonucleotide sequence
Product size
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Gene
Fw 5´-GTCGCGGTGGTTTGAATTCC-3´ Mt DET2
154 bp
SC
Rv 5´-AGTCCCAAATTCGGCATACC-3´
Fw 5´-TTCCATGTGGGTGGAAAGTC-3´ Mt DWF4
171 bp
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Rv 5´-GATCCTGCGCATAATCTTGG-3´
Fw 5´-CTGTGAAGTACCTCCATGAC-3´ Mt CYP85
162 bp
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Rv 5´-GTGGCCAATCTAGTTGTCTC-3´
Fw 5´-GGCCTGACGTAGAACTTATG-3´
Mt PAO1
312 bp
EP
Rv 5´-GCACGTAGCTTGTCATACAC-3´
Fw 5´-ATGGGGCAGAAGGATGCGTATG-3´ 115 bp
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Mt Actin
Rv 5´-AGCCTTCATAGATGGGGACCGT-3´
579
580
581
582
25
ACCEPTED MANUSCRIPT 583
Figure 1
584 0,30
SDW PSPA aa
587
aa
0,20
g plant-1
586
0,15
ab
bb
ab
c
b 0,06
0,10 0,05 0,00
0,00 Spd
Spm
C
M AN U
590 591
598
EP AC C
597
TE D
592
596
b
SC
C
595
a b
c
0,03
589
594
a
0,09
588
593
RDW PSR
0,12
RI PT
0,25
g plant-1
585
0,15
599 600 601
26
Spd
Spm
ACCEPTED MANUSCRIPT 602
Figure 2
603
NFR
b b
607 c
c
610
616 617
EP
615
AC C
614
25
c
C
Spm
TE D
611
613
b
b
M AN U
Spd
609
612
b b
0 C
a
c
0
608
50
RI PT
a
100
50
NFW mg plant-1
606
µmol N g-1 NFW h-1
605
75
150
SC
604
618 619 620
27
Spd
Spm
ACCEPTED MANUSCRIPT 621
Figure 3
622 623
5
AB
1,0
B
a a
a C
ab
0,5
b
C
C
b
4
a
0,0
b
2
SPM
Spd Spm
D
F E
C
638
C
Spd Spm
N
B C D E F
0,0 C
Spd Spm
L
nmols g-1 FW
AC C
HOMSPD A B C
6
D
D E
4 2 0 Spd Spm
L
C
Spd Spm
N
28
C
Spd Spm
N
10 8
A
CAD
0,5
N
C
639
Spd Spm
1,0
Spd Spm
EP
C
C
TE D
cd d
nmols g-1 FW
b c
L
637
D
b
L
B
a
1,0
0,0
636
E
A
1,5
632
635
C
N
0,5
634
C
1,5
d
633
Spd Spm
2,0
nmols g-1 FW
631
C
L
629 630
Spd Spm
b
M AN U
C
B
b
b
0
628
B
3
1
627
A
SPD
RI PT
626
PUT
SC
625
6 A
nmols g-1 FW
624
nmols g-1 FW
1,5
ACCEPTED MANUSCRIPT 640
Figure 4
641 642
PRO
643
645
a
a 1000
b 500
c
c
646 C
647 648
652 653 654 655
EP
651
AC C
650
Spd
TE D
649
c
M AN U
0
SC
644
nmol gFW -1
1500
RI PT
2000
656 657 658
29
Spm
ACCEPTED MANUSCRIPT 659
Figure 5
660 661
800
b 400
c
c
200
664
0
665 666 667
673 674
EP
672
AC C
671
TE D
668
670
Spd
c
Spm
M AN U
C
669
c
SC
µmol MDA gFW-1
663
600
RI PT
MDA
a 662
675 676 677
30
ACCEPTED MANUSCRIPT 678
Figure 6
679
A 680
20
µmol gFW -1
15
682
a b
10
5
684
0
d
685
B
TE D
687
689
Spd
692 693
AC C
691
NaCl
EP
Control 690
Spm
M AN U
C
688
bc
c
683
686
b
SC
681
RI PT
H2O2
Spd + NaCl
Spd
694 695 696
31
ACCEPTED MANUSCRIPT 697
Figure 7
698
25
25
DET2 20
10
c
5
Spd
CYP85
20 15
20
a
10
b
5
c
TE D
Fol change
C
a
b
c
Spd
Spm
25
707
b
b
0
Spd
b
Spm
AC C
EP
C
712
Spm
Fol change
705
b c
SC
C
25
711
10
0
704
710
a
5
0
703
709
15
d
d
708
Fol change
b
15
DWF4
20
c
702
706
a
M AN U
701
Fol change
700
RI PT
699
713
32
PAO1
15 10
a a
a
5
b b
b
0 C
Spd
Spm
ACCEPTED MANUSCRIPT Highlights 1. Exogenous polyamines increment nodule biomass and nitrogenase activity in the symbiosis Medicago truncatula-Sinorhizobium meliloti.
peroxidation under salt stress.
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2. Spermidine and spermine pre-treatments reduce the levels of H2O2 and lipid
3. Polyamines induce the expression of genes involved in brassinosteroids biosynthesis.
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4. Exogenous polyamines improve the response to salinity of the M.
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truncatula-S. meliloti symbiosis by reducing the oxidative damage.
ACCEPTED MANUSCRIPT Contribution
Miguel López Gómez: conceived and designed the experiments and wrote the
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manuscript. Javier Hidalgo-Castellanos: performed the experiments and analyzed the data.
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J. Rubén Muñoz-Sánchez: performed some of the experiments
Carmen Lluch Plá: Project leader
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Agustín J. Marín-Peña: performed some of the experiments
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José A. Herrera-Cervera: Project leader