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水稻减数分裂过程中,OsPRD2对双链断裂形成至关重要,但对纺锤体组装并非必需。

OsPRD2 is essential for double-strand break formation, but not spindle assembly during rice meiosis.

作者信息

Wang Chong, Qu Shuying, Zhang Jie, Fu Ming, Chen Xiaofei, Liang Wanqi

机构信息

Joint International Research Laboratory of Metabolic & Developmental Sciences, State Key Laboratory of Hybrid Rice, School of Life Sciences and Biotechnology, Shanghai Jiao Tong University, Shanghai, China.

Development Center of Plant Germplasm Resources, Shanghai Key Laboratory of Plant Molecular Sciences, College of Life Sciences, Shanghai Normal University, Shanghai, China.

出版信息

Front Plant Sci. 2023 Jan 13;13:1122202. doi: 10.3389/fpls.2022.1122202. eCollection 2022.

Abstract

Meiotic recombination starts with the programmed formation of double-strand breaks (DSB) in DNA, which are catalyzed by SPO11, a type II topoisomerase that is evolutionarily conserved, and several other accessary proteins. Homologs of MEIOSIS INHIBITOR 4 (MEI4/REC24/PRD2) are proteins that are also essential for the generation of meiotic DSBs in budding yeast, mice and Arabidopsis thaliana. In Arabidopsis, the protein ARABIDOPSIS THALIANA PUTATIVE RECOMBINATION INITIATION DEFECTS 2/MULTIPOLAR SPINDLE 1 (AtPRD2/MPS1) has been shown to have additional roles in spindle assembly, indicating a functional diversification. Here we characterize the role of the rice MEI4/PRD2 homolog in meiosis. The mutant was completely male and female sterile. In male meiocytes of , no γH2AX foci were detected and twenty-four univalents were produced at diakinesis, suggesting that OsPRD2 is essential for DSB generation. OsPRD2 showed a dynamic localization during meiosis. For instance, OsPRD2 foci first appeared as discrete signals across chromosome at leptotene, and then became confined to the centromeres during zygotene, suggesting that they might be involved in assembly of the spindle. However we did not observe any obvious aberrant morphologies in neither the organization of the bipolar spindle nor in the orientation of the kinetochore in the mutant. These findings suggest that in rice PRD2 might not be required for spindle assembly and organization, as it does in Arabidopsis. Taken together our results indicate that plant MEI4/PRD2 homologs do play a conserved role in the formation of meiotic DSBs in DNA, but that their involvement in bipolar spindle assembly is rather species-specific.

摘要

减数分裂重组始于DNA中双链断裂(DSB)的程序性形成,这是由进化上保守的II型拓扑异构酶SPO11以及其他几种辅助蛋白催化的。减数分裂抑制剂4(MEI4/REC24/PRD2)的同源物是在芽殖酵母、小鼠和拟南芥中产生减数分裂DSB所必需的蛋白质。在拟南芥中,蛋白质拟南芥假定重组起始缺陷2/多极纺锤体1(AtPRD2/MPS1)已被证明在纺锤体组装中具有额外作用,表明其功能具有多样性。在这里,我们描述了水稻MEI4/PRD2同源物在减数分裂中的作用。该突变体完全雄性和雌性不育。在该突变体的雄性减数分裂细胞中,未检测到γH2AX焦点,并且在终变期产生了24个单价体,这表明OsPRD2对于DSB的产生至关重要。OsPRD2在减数分裂过程中表现出动态定位。例如,OsPRD2焦点在细线期首先作为染色体上离散的信号出现,然后在偶线期局限于着丝粒,这表明它们可能参与纺锤体的组装。然而,我们在突变体中既未观察到双极纺锤体组织的任何明显异常形态,也未观察到动粒方向的明显异常。这些发现表明,在水稻中,PRD2可能不像在拟南芥中那样是纺锤体组装和组织所必需的。综合我们的结果表明,植物MEI4/PRD2同源物在DNA减数分裂DSB的形成中确实发挥保守作用,但它们在双极纺锤体组装中的参与具有物种特异性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7b61/9880466/57c7fda5c3e1/fpls-13-1122202-g001.jpg

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