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通过高通量筛选和基因编辑对水稻花粉萌发关键基因进行全基因组鉴定。

Global identification of key genes for pollen germination in rice through high-throughput screening and gene editing.

作者信息

Kim Eui-Jung, Hong Woo-Jong, Kim Yu-Jin, Kim Eun Young, Yun Sang Dae, Moon Sunok, Lee Su-Kyoung, Park Soon Ki, Jung Ki-Hong

机构信息

Graduate School of Green-Bio Science & Crop Biotech Institute, Kyung Hee University, Yongin, 17104, Korea.

Research Center for Plant Plasticity, Seoul National University, Seoul, 08826, Korea.

出版信息

J Integr Plant Biol. 2025 Jun;67(6):1665-1684. doi: 10.1111/jipb.13900. Epub 2025 Apr 1.

Abstract

Successful reproduction depends on the stable germination and growth of the pollen tubes (PT). However, the molecular mechanisms involved in rice PT growth and development remain largely unknown. In a previous study, microarray transcriptome analysis identified 627 genes preferentially expressed in the tricellular and germinating pollen of rice (i.e., Oryza sativa ssp. japonica). To elucidate key genes involved in the gene transfer process facilitated by male gametophytes, we systematically screened T-DNA lines containing disrupted sequences that corresponded to these 627 genes and analyzed the genotypes of heterozygote progeny from 107 T-DNA-indexed lines covering 105 genes. We found that 42 lines exhibited a distorted segregation ratio among the wild-type (WT), heterozygote (HT), and homozygote (HM) genotypes, which deviated from the expected Mendelian ratio of 1:2:1 (WT:HT:HM). Further characterization using CRISPR/Cas9 mutants revealed that knockout mutants of certain genes that exhibited segregation distortion in the T-DNA insertion region were completely sterile. Moreover, even when T-DNA insertion lines followed Mendelian segregation patterns, sterility could be induced by simultaneously mutating functionally redundant genes, thereby overcoming genetic compensation. Interestingly, although some T-DNA insertion lines exhibited segregation ratios approximating 1:1:0, the corresponding CRISPR/Cas9 mutants produced homozygous seeds and showed partial sterility. Partial sterility suggests that despite mutant pollen grains being less competitive than WT pollen, they retain their fertilization potential under relaxed competition from WT pollen. Beyond mutant-based analysis, transcriptomic profiling of sterile mutant lines provided additional insight into the regulatory relationship between key germination regulators and the 105 target genes studied here. Overall, this study demonstrates the effectiveness of a multi-pronged strategy to accelerate the identification of defective phenotypes using mutant studies and provides valuable genetic resources for inducing novel male sterility in rice.

摘要

成功繁殖依赖于花粉管(PT)的稳定萌发和生长。然而,水稻花粉管生长发育所涉及的分子机制仍 largely 未知。在先前的一项研究中,微阵列转录组分析鉴定出 627 个在水稻(即粳稻)三细胞和萌发花粉中优先表达的基因。为了阐明雄配子体促进基因转移过程中涉及的关键基因,我们系统地筛选了包含与这 627 个基因相对应的 disrupted 序列的 T-DNA 系,并分析了来自涵盖 105 个基因的 107 个 T-DNA 索引系的杂合子后代的基因型。我们发现 42 个系在野生型(WT)、杂合子(HT)和纯合子(HM)基因型之间表现出扭曲的分离比,偏离了预期的孟德尔比例 1:2:1(WT:HT:HM)。使用 CRISPR/Cas9 突变体的进一步表征表明,在 T-DNA 插入区域表现出分离扭曲的某些基因的敲除突变体完全不育。此外,即使 T-DNA 插入系遵循孟德尔分离模式,通过同时突变功能冗余基因也可诱导不育,从而克服遗传补偿。有趣的是,尽管一些 T-DNA 插入系表现出接近 1:1:0 的分离比,但相应的 CRISPR/Cas9 突变体产生了纯合种子并表现出部分不育。部分不育表明,尽管突变花粉粒的竞争力不如野生型花粉,但在野生型花粉竞争宽松的情况下,它们仍保留受精潜力。除了基于突变体的分析外,不育突变体系的转录组分析为关键萌发调节因子与本文研究的 105 个靶基因之间的调控关系提供了额外的见解。总体而言,本研究证明了使用突变体研究加速鉴定缺陷表型的多管齐下策略的有效性,并为诱导水稻新型雄性不育提供了宝贵的遗传资源。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c2cf/12131703/edff8f8f7345/JIPB-67-1665-g001.jpg

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