Suppr超能文献

用于监测蛋白质组装的支撑细胞膜片。

Supported Cell Membrane Sheets to Monitor Protein Assembly.

作者信息

Erlendsson Simon, Thorsen Thor Seneca, Madsen Kenneth Lindegaard

机构信息

Molecular Neuropharmacology and Genetics Laboratory, Department of Neuroscience, Faculty of Health and Medical Sciences, The Panum Institute-Maersk Tower 7.5, University of Copenhagen, 2200 Copenhagen N, Denmark.

出版信息

Bio Protoc. 2019 Sep 20;9(18):e3368. doi: 10.21769/BioProtoc.3368.

Abstract

Studying protein-protein and protein-lipid interactions in their native environment is highly desirable, yet, the heterogeneity and complexity of cellular systems limits the repertoire of experimental methods available. In cells, interactions are often taking place in confined microenvironments where factors such as avidity, hindered diffusion, reduced dimensionality, crowding . strongly influence the binding kinetics and therefore it can be problematic to equate binding affinities obtained by bulk in-solution methods (, Fluorescence Polarization, Isothermal titration calorimetry, Microscale thermophoresis) with those occurring in real cellular environments. The Supported Cell Membrane Sheet method presented here, addresses these issues by allowing access to the inner leaflet of the apical plasma membrane. The method is a highly versatile, near-native platform for both qualitative and quantitative studies of protein-protein and protein-lipid interactions occurring directly in or on the plasma membrane.

摘要

在蛋白质的天然环境中研究蛋白质-蛋白质和蛋白质-脂质相互作用是非常必要的,然而,细胞系统的异质性和复杂性限制了可用实验方法的种类。在细胞中,相互作用通常发生在受限的微环境中,诸如亲和力、扩散受阻、维度降低、拥挤等因素会强烈影响结合动力学,因此,将通过大量溶液内方法(如荧光偏振、等温滴定量热法、微量热泳)获得的结合亲和力与真实细胞环境中发生的结合亲和力等同起来可能会有问题。本文介绍的支持细胞膜片法通过允许接触顶端质膜的内小叶来解决这些问题。该方法是一个高度通用的、接近天然状态的平台,可用于直接在质膜中或质膜上发生的蛋白质-蛋白质和蛋白质-脂质相互作用的定性和定量研究。

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