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Mechanistic Origin of Microtubule Dynamic Instability and Its Modulation by EB Proteins

机译:MicroTubule动态稳定性的机械起源及其EB蛋白的调节

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摘要

Microtubule (MT) dynamic instability is driven by GTP hydrolysis and regulated by microtubule-associated proteins, including the plus-end tracking end-binding protein (EB) family. We report six cryo-electron microscopy (cryo-EM) structures of MTs, at 3.5 angstrom or better resolution, bound to GMPCPP, GTP gamma S, or GDP, either decorated with kinesin motor domain after polymerization or copolymerized with EB3. Subtle changes around the E-site nucleotide during hydrolysis trigger conformational changes in alpha-tubulin around an "anchor point,'' leading to global lattice rearrangements and strain generation. Unlike the extended lattice of the GMPCPP-MT, the EB3-bound GTP gamma S-MT has a compacted lattice that differs in lattice twist from that of the also compacted GDP-MT. These results and the observation that EB3 promotes rapid hydrolysis of GMPCPP suggest that EB proteins modulate structural transitions at growing MT ends by recognizing and promoting an intermediate state generated during GTP hydrolysis. Our findings explain both EBs end-tracking behavior and their effect on microtubule dynamics.
机译:Microotubule(MT)动态不稳定性由GTP水解驱动,并由微管相关蛋白调节,包括加端跟踪端结合蛋白(EB)家族。我们向3.5埃或更好的分辨率报告MTS的六种冷冻电子显微镜(Cryo-EM)结构,与GMPCPP,GTPγS或GDP结合,在聚合或与EB3共聚合后用Kinesin Motor结构域装饰。在水解过程中围绕e-核苷酸的微妙变化触发α-微管蛋白的构象变化,围绕着“锚点”,导致全球晶格重排和应变产生。与GMPCPP-MT的延伸格子不同,EB3结合的GTP伽玛S-MT具有压实的晶格,其不同的晶格扭曲来自也是压实的GDP-MT。这些结果和EB3促进GMPCPP的快速水解的观察结果表明EB蛋白通过识别和促进MT的生长MT而调节结构过渡GTP水解期间产生的中间状态。我们的研究结果解释了EBS结束跟踪行为及其对微管动态的影响。

著录项

  • 来源
    《Cell》 |2015年第4期|共11页
  • 作者单位

    Univ Calif Berkeley Lawrence Berkeley Natl Lab Life Sci Div Berkeley CA 94720 USA;

    Univ Calif Berkeley Biophys Grad Program Berkeley CA 94720 USA;

    MRC Mol Biol Lab Cambridge CB2 0QH England;

    Univ Calif Berkeley Lawrence Berkeley Natl Lab Life Sci Div Berkeley CA 94720 USA;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 细胞生物学;
  • 关键词

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