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Insights into EB1 structure and the role of its C-terminal domain for discriminating microtubule tips from the lattice

机译:洞悉EB1结构及其C末端结构域从晶格中区分微管尖端的作用

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End-binding proteins (EBs) comprise a conserved family of microtubule plus end–tracking proteins. The concerted action of calponin homology (CH), linker, and C-terminal domains of EBs is important for their autonomous microtubule tip tracking, regulation of microtubule dynamics, and recruitment of numerous partners to microtubule ends. Here we report the detailed structural and biochemical analysis of mammalian EBs. Small-angle X-ray scattering, electron microscopy, and chemical cross-linking in combination with mass spectrometry indicate that EBs are elongated molecules with two interacting CH domains, an arrangement reminiscent of that seen in other microtubule- and actin-binding proteins. Removal of the negatively charged C-terminal tail did not affect the overall conformation of EBs; however, it increased the dwell times of EBs on the microtubule lattice in microtubule tip–tracking reconstitution experiments. An even more stable association with the microtubule lattice was observed when the entire negatively charged C-terminal domain of EBs was replaced by a neutral coiled-coil motif. In contrast, the interaction of EBs with growing microtubule tips was not significantly affected by these C-terminal domain mutations. Our data indicate that long-range electrostatic repulsive interactions between the C-terminus and the microtubule lattice drive the specificity of EBs for growing microtubule ends.
机译:末端结合蛋白(EB)包含一个保守的微管家族和末端追踪蛋白。钙蛋白的同源性(CH),接头和EB的C端结构域的协同作用对于其自主的微管尖端跟踪,微管动力学调节以及向微管末端募集大量伴侣至关重要。在这里,我们报告哺乳动物EB的详细结构和生化分析。小角X射线散射,电子显微镜和化学交联与质谱的结合表明EB是具有两个相互作用的CH域的细长分子,这种排列让人联想到其他微管和肌动蛋白结合蛋白中的排列。去除带负电的C末端尾巴不会影响EB的整体构象;然而,在微管尖端追踪重建实验中,它增加了EB在微管晶格上的停留时间。当EBs的整个带负电的C末端结构域被中性的卷曲螺旋基序取代时,与微管晶格的结合更加稳定。相反,这些C末端域突变并未显着影响EB与生长中的微管末端的相互作用。我们的数据表明,C末端和微管晶格之间的远距离静电排斥相互作用驱动了EBs增长微管末端的特异性。

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