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Phosphoproteome analysis of the human mitotic spindle

机译:人类有丝分裂纺锤体的磷酸化蛋白质组学分析

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During cell division, the mitotic spindle segregates the sister chromatids into two nascent cells, such that each daughter cell inherits one complete set of chromosomes. Errors in spindle formation can result in both chromosome missegregation and cytokinesis defects and hence lead to genomic instability. To ensure the correct function of the spindle, the activity and localization of spindle associated proteins has to be tightly regulated in time and space. Reversible phosphorylation has been shown to be one of the key regulatory mechanisms for the organization of the mitotic spindle. The relatively low number of identified in vivo phosphorylation sites of spindle components, however, has hampered functional analysis of regulatory spindle networks. A more complete inventory of the phosphorylation sites of spindle-associated proteins would therefore constitute an important advance. Here, we describe the mass spectrometry-based identification of in vivo phosphorylation sites from purified human mitotic spindles. In total, 736 phosphorylation sites were identified, of which 312 could be attributed to known spindle proteins. Among these are phosphorylation sites that were previously shown to be important for the regulation of spindle-associated proteins. Importantly, this data set also comprises 279 novel phosphorylation sites of known spindle proteins for future functional studies. This inventory of spindle phosphorylation sites should thus make an important contribution to a better understanding of the molecular mechanisms that regulate the formation, function, and integrity of the mitotic spindle.
机译:在细胞分裂过程中,有丝分裂纺锤体将姐妹染色单体分离为两个新生细胞,这样每个子细胞都可以继承一套完整的染色体。纺锤体形成中的错误会导致染色体错聚和胞质分裂缺陷,从而导致基因组不稳定。为了确保纺锤体的正确功能,必须在时间和空间上严格调节纺锤体相关蛋白的活性和位置。可逆磷酸化已被证明是有丝分裂纺锤体组织的关键调控机制之一。然而,纺锤体成分的鉴定出的体内磷酸化位点的数量相对较少,阻碍了调节纺锤体网络的功能分析。因此,纺锤体相关蛋白的磷酸化位点的更完整清单将构成重要的进步。在这里,我们描述了基于质谱的鉴定从纯化的人类有丝分裂纺锤体体内磷酸化位点。总共鉴定出736个磷酸化位点,其中312个可归因于已知的纺锤体蛋白。其中有磷酸化位点,以前显示对调节纺锤体相关蛋白很重要。重要的是,该数据集还包含279种已知纺锤体蛋白的新磷酸化位点,以用于将来的功能研究。因此,对主轴磷酸化位点的这种库存应有助于更好地理解调节有丝分裂纺锤体的形成,功能和完整性的分子机制。

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