Pagano Andrea, Kunz Laura, Dittmann Antje, Araújo Susana De Sousa, Macovei Anca, Shridhar Gaonkar Shraddha, Sincinelli Federico, Wazeer Hisham, Balestrazzi Alma
Department of Biology and Biotechnology 'L. Spallanzani', University of Pavia, Pavia, Italy.
Functional Genomics Center Zurich (FGCZ), University of Zurich/Eidgenossische Technische Hochschule (ETH) Zurich, Zurich, Switzerland.
Front Plant Sci. 2023 Jun 13;14:1188546. doi: 10.3389/fpls.2023.1188546. eCollection 2023.
Several molecular aspects underlying the seed response to priming and the resulting vigor profile are still poorly understood. Mechanisms involved in genome maintenance deserve attention since the balance between stimulation of germination and DNA damage accumulation versus active repair is a key determinant for designing successful seed priming protocols.
Changes in the Medicago truncatula seed proteome were investigated in this study, using discovery mass spectrometry and label-free quantification, along the rehydration-dehydration cycle of a standard vigorization treatment (hydropriming plus dry-back), and during post-priming imbibition.
From 2056 to 2190 proteins were detected in each pairwise comparison, among which six were differentially accumulated and 36 were detected only in one condition. The following proteins were selected for further investigation: MtDRP2B (DYNAMIN-RELATED PROTEIN), MtTRXm4 (THIOREDOXIN m4), and MtASPG1 (ASPARTIC PROTEASE IN GUARD CELL 1) showing changes in seeds under dehydration stress; MtITPA (INOSINE TRIPHOSPHATE PYROPHOSPHORYLASE), MtABA2 (ABSCISIC ACID DEFICIENT 2), MtRS2Z32 (SERINE/ARGININE-RICH SPLICING FACTOR RS2Z32), and MtAQR (RNA HELICASE AQUARIUS) that were differentially regulated during post-priming imbibition. Changes in the corresponding transcript levels were assessed by qRT-PCR. In animal cells, ITPA hydrolyses 2'-deoxyinosine triphosphate and other inosine nucleotides, preventing genotoxic damage. A proof of concept was performed by imbibing primed and control M. truncatula seeds in presence/absence of 20 mM 2'-deoxyinosine (dI). Results from comet assay highlighted the ability of primed seeds to cope with dI-induced genotoxic damage. The seed repair response was assessed by monitoring the expression profiles of MtAAG (ALKYL-ADENINE DNA GLYCOSILASE) and MtEndoV (ENDONUCLEASE V) genes that participate in the repair of the mismatched I:T pair in BER (base excision repair) and AER (alternative excision repair) pathways, respectively.
种子对引发处理的响应以及由此产生的活力特征背后的几个分子层面仍未得到充分理解。涉及基因组维持的机制值得关注,因为发芽刺激与DNA损伤积累和主动修复之间的平衡是设计成功的种子引发方案的关键决定因素。
在本研究中,使用发现质谱和无标记定量法,沿着标准活力处理(水引发加回干)的复水-脱水循环以及引发后吸胀过程,研究了蒺藜苜蓿种子蛋白质组的变化。
在每次成对比较中检测到2056至2190种蛋白质,其中6种差异积累,36种仅在一种条件下被检测到。选择以下蛋白质进行进一步研究:在脱水胁迫下种子中表现出变化的MtDRP2B(动力相关蛋白)、MtTRXm4(硫氧还蛋白m4)和MtASPG1(保卫细胞中的天冬氨酸蛋白酶1);在引发后吸胀过程中差异调节的MtITPA(肌苷三磷酸焦磷酸化酶)、MtABA2(脱落酸缺陷2)、MtRS2Z32(富含丝氨酸/精氨酸的剪接因子RS2Z32)和MtAQR(RNA解旋酶水瓶座)。通过qRT-PCR评估相应转录水平的变化。在动物细胞中,ITPA水解2'-脱氧肌苷三磷酸和其他肌苷核苷酸,防止遗传毒性损伤。通过在存在/不存在20 mM 2'-脱氧肌苷(dI)的情况下浸泡引发的和对照蒺藜苜蓿种子进行了概念验证。彗星试验结果突出了引发种子应对dI诱导的遗传毒性损伤的能力。通过监测分别参与碱基切除修复(BER)和替代切除修复(AER)途径中错配的I:T对修复的MtAAG(烷基腺嘌呤DNA糖苷酶)和MtEndoV(核酸内切酶V)基因的表达谱来评估种子修复反应。
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