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Characterizing the functions of the protein kinase genes MAP3Kepsilon1 and MAP3Kepsilon2 in Arabidopsis thaliana growth and development.

机译:表征蛋白激酶基因MAP3Kepsilon1和MAP3Kepsilon2在拟南芥生长和发育中的功能。

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摘要

I have used reverse-genetic analysis to investigate the function of MAP3K&egr;1 and MAP3K&egr;2, a pair of closely-related Arabidopsis thaliana genes that encode protein kinases. Plants homozygous for insertional mutations of either map3k&egr;1 or map3k&egr;2 displayed no apparent mutant phenotype, whereas the double-mutant combination caused pollen lethality. Through the use of transmission electron microscopy it was determined that double-mutant pollen grains develop plasma membrane irregularities following pollen mitosis I. Use of confocal microscopy and biochemical fractionation indicated that MAP3K&egr;1 protein is localized to the plasma membrane.;Analysis of the expression of a YFP-MAP3K&egr;1 fusion protein revealed strong expression in actively dividing tissues, lateral roots, and embryos. In order to investigate the function of these kinases in the sporophyte, we used a conditional-rescue strategy based on an ethanol-inducible system to construct map3k&egr;1-/- map3k&egr;2-/- double-mutant plants. The conditionally-rescued double-mutants had decreased cell expansion and proliferation, and their embryo development was delayed and arrested. By contrast, MAP3K&egr;1 over-expression caused ectopic cell division in dark-grown hypocotyls, increased cell expansion in light-grown hypocotyls, stimulated auxin-responsive gene expression, and supported auxin-independent growth of suspension cells. My work has indicated that MAP3K&egr;1 and MAP3K&egr;2 regulate cell division and cell expansion via auxin signal transduction in Arabidopsis, and that this pair of genes is required for embryo development. Future studies will investigate the precise mechanisms by which MAP3K&egr;1 and MAP3K&egr;2 regulate cell division, expansion, and auxin signaling.
机译:我已经使用反向基因分析来研究MAP3K&egr; 1和MAP3K&egr; 2(编码蛋白激酶的一对紧密相关的拟南芥基因)的功能。 map3k&egr; 1或map3k&egr; 2的插入突变纯合的植物未显示明显的突变表型,而双突变体组合则导致花粉致死率。通过透射电子显微镜确定花粉有丝分裂I后双突变体的花粉粒发展出质膜不规则性。共聚焦显微镜和生化分离表明MAP3K&egr; 1蛋白定位于质膜。 YFP-MAP3K&egr; 1融合蛋白的表达揭示了在活跃分裂的组织,侧根和胚胎中的强表达。为了研究这些激酶在孢子体中的功能,我们使用了基于乙醇诱导系统的条件拯救策略来构建map3k&egr; 1-/-map3k&egr; 2-/-双突变植物。有条件救援的双突变体减少了细胞的扩增和增殖,并且其胚胎发育被延迟并被阻止。相比之下,MAP3K&egr; 1的过表达导致暗生长的下胚轴中的异位细胞分裂,浅生长的下胚轴中的细胞扩增增加,刺激了生长素响应基因的表达,并支持了生长素非依赖性的悬浮细胞生长。我的工作表明,拟南芥中的MAP3K&egr; 1和MAP3K&egr; 2通过生长素信号转导来调节细胞分裂和细胞扩增,而这对基因是胚胎发育所必需的。未来的研究将研究MAP3K&egr; 1和MAP3K&egr; 2调控细胞分裂,扩增和生长素信号传导的精确机制。

著录项

  • 作者

    Chaiwongsar, Suraphon.;

  • 作者单位

    The University of Wisconsin - Madison.;

  • 授予单位 The University of Wisconsin - Madison.;
  • 学科 Biology Molecular.;Biology Genetics.
  • 学位 Ph.D.
  • 年度 2007
  • 页码 242 p.
  • 总页数 242
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

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