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甘蓝型油菜中 BnaA02.TOP1α 和 BnaC02.TOP1α 参与真叶生物量积累的功能特征

Functional characterisation of BnaA02.TOP1α and BnaC02.TOP1α involved in true leaf biomass accumulation in Brassica napus L.

机构信息

State Key Laboratory for Crop Stress Resistance and High-Efficiency Production, National Yangling Agricultural Biotechnology & Breeding Center, Shaanxi Key Laboratory of Crop Heterosis, and College of Agronomy, Northwest A&F University, Yangling, 712100, Shaanxi, China.

出版信息

Plant J. 2024 Nov;120(4):1358-1376. doi: 10.1111/tpj.17054. Epub 2024 Sep 30.

Abstract

Leaves, as primary photosynthetic organs essential for high crop yield and quality, have attracted significant attention. The functions of DNA topoisomerase 1α (TOP1α) in various biological processes, including leaf development, in Brassica napus remain unknown. Here, four paralogs of BnaTOP1α, namely BnaA01.TOP1α, BnaA02.TOP1α, BnaC01.TOP1α and BnaC02.TOP1α, were identified and cloned in the B. napus inbred line 'K407'. Expression pattern analysis revealed that BnaA02.TOP1α and BnaC02.TOP1α, but not BnaA01.TOP1α and BnaC01.TOP1α, were persistently and highly expressed in B. napus true leaves. Preliminary analysis in Arabidopsis thaliana revealed that BnaA02.TOP1α and BnaC02.TOP1α paralogs, but not BnaA01.TOP1α and BnaC01.TOP1α, performed biological functions. Targeted mutations of four BnaTOP1α paralogs in B. napus using the CRISPR-Cas9 system revealed that BnaA02.TOP1α and BnaC02.TOP1α served as functional paralogs and redundantly promoted true leaf number and size, thereby promoting true leaf biomass accumulation. Moreover, BnaA02.TOP1α modulated the levels of endogenous gibberellins, cytokinins and auxins by indirectly regulating several genes related to their metabolism processes. BnaA02.TOP1α directly activated BnaA03.CCS52A2 and BnaC09.AN3 by facilitating the recruitment of RNA polymerase II and modulating H3K27me3, H3K36me2 and H3K36me3 levels at these loci and indirectly activated the BnaA08.PARL1 expression, thereby positively controlling the true leaf size in B. napus. Additionally, BnaA02.TOP1α indirectly activated the BnaA07.PIN1 expression to positively regulate the true leaf number. These results reveal the important functions of BnaTOP1α and provide insights into the regulatory network controlling true leaf biomass accumulation in B. napus.

摘要

叶片是作物高产、优质的重要光合器官,受到广泛关注。在甘蓝型油菜中,DNA 拓扑异构酶 1α(TOP1α)在各种生物过程中的功能,包括叶片发育,仍然未知。本研究在甘蓝型油菜自交系‘K407’中鉴定并克隆了四个 TOP1α 同源基因,分别为 BnaA01.TOP1α、BnaA02.TOP1α、BnaC01.TOP1α 和 BnaC02.TOP1α。表达模式分析表明,BnaA02.TOP1α 和 BnaC02.TOP1α在甘蓝型油菜真叶中持续且高度表达,而 BnaA01.TOP1α和 BnaC01.TOP1α则没有。在拟南芥中的初步分析表明,BnaA02.TOP1α 和 BnaC02.TOP1α 同源基因,而不是 BnaA01.TOP1α 和 BnaC01.TOP1α,具有生物学功能。利用 CRISPR-Cas9 系统靶向敲除甘蓝型油菜的四个 BnaTOP1α 同源基因,结果表明 BnaA02.TOP1α 和 BnaC02.TOP1α 是功能同源基因,它们冗余地促进真叶数量和大小,从而促进真叶生物量积累。此外,BnaA02.TOP1α 通过间接调节与代谢过程相关的几个基因来调节内源赤霉素、细胞分裂素和生长素的水平。BnaA02.TOP1α 通过促进 RNA 聚合酶 II 的募集并调节这些基因座处的 H3K27me3、H3K36me2 和 H3K36me3 水平,直接激活 BnaA03.CCS52A2 和 BnaC09.AN3,并间接激活 BnaA08.PARL1 的表达,从而正向调控甘蓝型油菜的真叶大小。此外,BnaA02.TOP1α 间接激活 BnaA07.PIN1 的表达,正向调控真叶数量。这些结果揭示了 BnaTOP1α 的重要功能,并为调控甘蓝型油菜真叶生物量积累的调控网络提供了新的见解。

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