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Analysis of membrane proteins localizing to the inner nuclear envelope in living cells

机译:膜蛋白定位于活细胞内核包膜的膜蛋白

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Understanding the protein composition of the inner nuclear membrane (INM) is fundamental to elucidating its role in normal nuclear function and in disease; however, few tools exist to examine the INM in living cells, and the INM-specific proteome remains poorly characterized. Here, we adapted split green fluorescent protein (split-GFP) to systematically localize known and predicted integral membrane proteins in Saccharomyces cerevisiae to the INM as opposed to the outer nuclear membrane. Our data suggest that components of the endoplasmic reticulum (ER) as well as other organelles are able to access the INM, particularly if they contain a small extraluminal domain. By pairing split-GFP with fluorescence correlation spectroscopy, we compared the composition of complexes at the INM and ER, finding that at least one is unique: Sbh2, but not Sbh1, has access to the INM. Collectively, our work provides a comprehensive analysis of transmembrane protein localization to the INM and paves the way for further research into INM composition and function.
机译:了解内核膜(INM)的蛋白质组成是阐明其在正常核功能和疾病中的作用的基础;然而,存在少量的工具来检查活细胞中的INM,并且特异性蛋白质组特征差。这里,我们改性分裂绿色荧光蛋白(分裂GFP)以系统地将已知的和预测的整体膜蛋白在酿酒酵母中以与外核膜相对的INM。我们的数据表明,内质网(ER)的组分以及其他细胞器能够进入INM,特别是如果它们含有小的喹臭域。通过用荧光相关光谱法配对分层GFP,我们将复合物的组成与INM和ER进行比较,发现至少一个是独特的:SBH2,但不是SBH1,可以进入INM。统称,我们的作品对INM的跨膜蛋白定位进行了综合分析,并为进一步研究INM成分和功能铺平了道路。

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