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以单转录本分辨率对哺乳动物细胞中的实时基因表达进行成像。

Imaging real-time gene expression in Mammalian cells with single-transcript resolution.

作者信息

Wells Amber L, Condeelis John S, Singer Robert H, Zenklusen Daniel

机构信息

Department of Anatomy and Structural Biology, Albert Einstein College of Medicine, Bronx, NY 10461, USA.

出版信息

CSH Protoc. 2007 Nov 1;2007:pdb.prot4869. doi: 10.1101/pdb.prot4869.

Abstract

INTRODUCTIONThe MS2 system provides optimal sensitivity for single-molecule detection in cells. It requires two genetically encoded moieties: a reporter mRNA that contains MS2 binding site (MBS) stem loops and a fluorescent MS2 coat protein (MCP-xFP) that binds to the stem loops with high affinity, thus tagging the mRNA within the cell. This protocol describes transfection of COS-7 cells with reporter RNA (e.g., pRSV-Z-24 MBS-β-actin) and MCP-xFP (e.g., pPolII-MCP-GFP-NLS) plasmids using calcium phosphate precipitation. The reporter mRNA plasmid must be co-transfected with the MCP-xFP-NLS plasmid for simultaneous expression in a cell. The unbound MCP-xFP-NLS is sequestered in the nucleus, leaving only the MCP-xFP-NLS that is bound to the reporter mRNA in the cytoplasm. This provides a high signal-to-noise ratio (SNR) that permits detection of single mRNA molecules. The Delta T Imaging System is used for image acquisition of fluorescent particles in the cells.

摘要

引言

MS2系统为细胞内单分子检测提供了最佳灵敏度。它需要两个基因编码部分:一个包含MS2结合位点(MBS)茎环的报告mRNA和一个与茎环高亲和力结合的荧光MS2外壳蛋白(MCP-xFP),从而在细胞内标记mRNA。本方案描述了使用磷酸钙沉淀法将报告RNA(如pRSV-Z-24 MBS-β-肌动蛋白)和MCP-xFP(如pPolII-MCP-GFP-NLS)质粒转染到COS-7细胞中。报告mRNA质粒必须与MCP-xFP-NLS质粒共转染,以便在细胞中同时表达。未结合的MCP-xFP-NLS被隔离在细胞核中,仅留下与细胞质中报告mRNA结合的MCP-xFP-NLS。这提供了高信噪比(SNR),从而能够检测单个mRNA分子。Delta T成像系统用于采集细胞中荧光颗粒的图像。

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