Effect of Vitis vinifera zygotic embryo cryopreservation and post-cryopreservation on the gene expression of DNA demethylases

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2024-08-14 DOI:10.1016/j.cryobiol.2024.104947
Juan Luis García-Vázquez , Mariana Quijada-Rivera , Miguel Ángel Hernández-Oñate , Martín Ernesto Tiznado-Hernández , María Fernanda Lazo-Javalera , Miguel Ángel Martínez-Téllez , Karen Rosalinda Astorga-Cienfuegos , Marisela Rivera-Domínguez
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Abstract

Grapevine (Vitis vinifera L.) crops are continuously exposed to biotic and abiotic stresses, which can cause genetic and epigenetic alterations. To determine the possible effects of grapevine cryopreservation on the regulation of DNA demethylase genes, this work studied the expression of DNA demethylase genes in cryopreserved and post-cryopreserved grapevine tissues. V. vinifera DNA demethylases were characterized by in silico analysis, and gene expression quantification was conducted by RT‒qPCR. Three DNA demethylase sequences were found: VIT_13s0074g00450 (VvDMT), VIT_08s0007g03920 (VvROS1), and VIT_06s0061g01270 (VvDML3). Phylogenetic analysis revealed that the sequences from V. vinifera and A. thaliana had a common ancestry. In the promoters of responsive elements to transcription factors such as AP-2, Myb, bZIP, TBP, and GATA, the conserved domains RRM DME and Perm CXXC were detected. These responsive elements play roles in the response to abiotic stress and the regulation of cell growth. These data helped us characterize the V. vinifera DNA demethylase genes. Gene expression analysis indicated that plant vitrification solution 2 (PVS2) treatment does not alter the expression of DNA demethylase genes. The expression levels of VvDMT and VvROS1 increased in response to cryopreservation by vitrification. Furthermore, in post-cryopreservation, VvROS1 was highly induced, and VvDML3 was repressed in all the treatment groups. Gene expression differences between different treatments and tissues may play roles in controlling methylation patterns during gene regulation in tissues stressed by cryopreservation procedures and in the post-cryopreservation period during plant growth and development.

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葡萄子代胚胎冷冻保存和冷冻保存后对 DNA 去甲基化酶基因表达的影响。
葡萄(Vitis vinifera L.)作物不断受到生物和非生物胁迫,这些胁迫可导致遗传和表观遗传改变。为了确定葡萄低温保存对 DNA 去甲基化酶基因调控可能产生的影响,这项工作研究了低温保存和低温保存后葡萄组织中 DNA 去甲基化酶基因的表达。通过硅学分析对葡萄藤 DNA 去甲基化酶进行了表征,并通过 RT-qPCR 对基因表达进行了定量。发现了三种 DNA 去甲基化酶序列:VIT_13s0074g00450(VvDMT)、VIT_08s0007g03920(VvROS1)和 VIT_06s0061g01270(VvDML3)。系统进化分析表明,来自葡萄和大连的序列具有共同的祖先。在AP-2、Myb、bZIP、TBP和GATA等转录因子的反应元件启动子中,发现了RRM DME和Perm CXXC保守结构域。这些反应元件在非生物胁迫反应和细胞生长调控中发挥作用。这些数据帮助我们确定了葡萄属 DNA 去甲基化酶基因的特征。基因表达分析表明,植物玻璃化溶液 2(PVS2)处理不会改变 DNA 去甲基化酶基因的表达。VvDMT 和 VvROS1 的表达水平在玻璃化冷冻保存后有所增加。此外,在冷冻保存后的所有处理组中,VvROS1 被高度诱导,VvDML3 被抑制。不同处理和组织之间的基因表达差异可能在植物生长和发育过程中,在受冷冻保存程序胁迫的组织和冷冻保存后组织的基因调控过程中起着控制甲基化模式的作用。
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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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