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从人胚肾细胞中利用转位酶Oxa1L纯化线粒体核糖体

Purification of Mitochondrial Ribosomes with the Translocase Oxa1L from HEK Cells.

作者信息

Yang Hanting, Desai Nirupa

机构信息

MRC Laboratory of Molecular Biology, Cambridge CB2 0QH, UK.

出版信息

Bio Protoc. 2021 Aug 5;11(15):e4110. doi: 10.21769/BioProtoc.4110.

Abstract

Mitochondrial ribosomes (mitoribosomes) perform protein synthesis inside mitochondria, the organelles responsible for energy conversion and adenosine triphosphate (ATP) production in eukaryotic cells. To investigate their functions and structures, large-scale purification of intact mitoribosomes from mitochondria-rich animal tissues or HEK cells have been developed. However, the fast purification of mitoribosomes anchored to the mitochondrial inner membrane in complex with the Oxa1L translocase remains particularly challenging. Herein, we present a protocol recently developed and modified in our lab that provides details for the efficient isolation of intact mitoribosomes with its translocase Oxa1L. We combined the cell culture of PDE12 or wild-type HEK293 cell lines with the isolation of mitochondria and the purification steps used for the biochemical and structural studies of mitoribosomes and Oxa1L. Graphic abstract: The protocol described herein includes two main sections: 1) isolation of mitochondria from HEK cells; and 2) purification of mitoribosome-Oxa1L from mitochondria. RB: Resuspension Buffer (see Recipes) (Created with BioRender.com).

摘要

线粒体核糖体(mitoribosomes)在真核细胞中负责能量转换和三磷酸腺苷(ATP)生成的细胞器——线粒体内进行蛋白质合成。为了研究其功能和结构,人们已经开发出从富含线粒体的动物组织或人胚肾(HEK)细胞中大规模纯化完整线粒体核糖体的方法。然而,与Oxa1L转位酶结合的、锚定在线粒体内膜上的线粒体核糖体的快速纯化仍然极具挑战性。在此,我们介绍一种最近在我们实验室开发并改进的方法,该方法详细说明了有效分离完整线粒体核糖体及其转位酶Oxa1L的步骤。我们将PDE12或野生型HEK293细胞系的细胞培养与线粒体分离以及用于线粒体核糖体和Oxa1L生化及结构研究的纯化步骤相结合。图形摘要:本文所述方法包括两个主要部分:1)从HEK细胞中分离线粒体;2)从线粒体中纯化线粒体核糖体 - Oxa1L。RB:重悬缓冲液(见配方)(由BioRender.com创建)

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