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用于检测单细胞中mRNA、细胞外蛋白质和细胞外蛋白质复合物的邻近测序。

Proximity sequencing for the detection of mRNA, extracellular proteins and extracellular protein complexes in single cells.

作者信息

Vistain Luke, Keisham Bijentimala, Xia Junjie, Phan Hoang Van, Tay Savaş

机构信息

Pritzker School of Molecular Engineering, The University of Chicago, Chicago, IL, USA.

Institute for Genomics and Systems Biology, The University of Chicago, Chicago, IL, USA.

出版信息

Nat Protoc. 2024 Dec;19(12):3568-3589. doi: 10.1038/s41596-024-01030-x. Epub 2024 Aug 15.

Abstract

Complex cellular functions occur via the coordinated formation and dissociation of protein complexes. Functions such as the response to a signaling ligand can incorporate dozens of proteins and hundreds of complexes. Until recently, it has been difficult to measure multiple protein complexes at the single-cell level. Here, we present a step-by-step procedure for proximity sequencing, which enables the simultaneous measurement of proteins, mRNA and hundreds of protein complexes located on the outer membrane of cells. We guide the user through probe creation, sample preparation, staining, sequencing and computational quantification of protein complexes. This protocol empowers researchers to study, for example, the interplay between transcriptional states and cellular functions by coupling measurements of transcription to measurements of linked effector molecules, yet could be generalizable to other paired events. The protocol requires roughly 16 h spread over several days to complete by users with expertise in basic molecular biology and single-cell sequencing.

摘要

复杂的细胞功能通过蛋白质复合物的协同形成和解离来实现。诸如对信号配体的反应等功能可能涉及数十种蛋白质和数百种复合物。直到最近,在单细胞水平上测量多种蛋白质复合物一直很困难。在这里,我们展示了一种用于邻近测序的分步程序,该程序能够同时测量位于细胞外膜上的蛋白质、mRNA和数百种蛋白质复合物。我们指导用户完成蛋白质复合物的探针创建、样品制备、染色、测序和计算定量。该方案使研究人员能够通过将转录测量与相关效应分子的测量相结合,例如研究转录状态与细胞功能之间的相互作用,但也可推广到其他配对事件。对于具有基础分子生物学和单细胞测序专业知识的用户来说,该方案大约需要在几天内分散16小时才能完成。

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