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通过增强绿色荧光蛋白(EGFP)荧光恢复监测哺乳动物细胞中错误酰化tRNA的抑制效率。

Monitoring mis-acylated tRNA suppression efficiency in mammalian cells via EGFP fluorescence recovery.

作者信息

Ilegems Erwin, Pick Horst M, Vogel Horst

机构信息

Institute of Biomolecular Sciences, Swiss Federal Institute of Technology, Lausanne CH-1015, Switzerland.

出版信息

Nucleic Acids Res. 2002 Dec 1;30(23):e128. doi: 10.1093/nar/gnf128.

Abstract

A reporter assay was developed to detect and quantify nonsense codon suppression by chemically aminoacylated tRNAs in mammalian cells. It is based on the cellular expression of the enhanced green fluorescent protein (EGFP) as a reporter for the site-specific amino acid incorporation in its sequence using an orthogonal suppressor tRNA derived from Escherichia coli. Suppression of an engineered amber codon at position 64 in the EGFP run-off transcript could be achieved by the incorporation of a leucine via an in vitro aminoacylated suppressor tRNA. Microinjection of defined amounts of mutagenized EGFP mRNA and suppressor tRNA into individual cells allowed us to accurately determine suppression efficiencies by measuring the EGFP fluorescence intensity in individual cells using laser-scanning confocal microscopy. Control experiments showed the absence of natural suppression or aminoacylation of the synthetic tRNA by endogenous aminoacyl-tRNA synthetases. This reporter assay opens the way for the optimization of essential experimental parameters for expanding the scope of the suppressor tRNA technology to different cell types.

摘要

开发了一种报告基因检测法,用于检测和定量哺乳动物细胞中化学氨酰化tRNA对无义密码子的抑制作用。它基于增强型绿色荧光蛋白(EGFP)的细胞表达,作为使用源自大肠杆菌的正交抑制性tRNA在其序列中进行位点特异性氨基酸掺入的报告基因。通过体外氨酰化抑制性tRNA掺入亮氨酸,可以实现对EGFP连续转录本中第64位工程化琥珀密码子的抑制。将确定量的诱变EGFP mRNA和抑制性tRNA显微注射到单个细胞中,使我们能够通过激光扫描共聚焦显微镜测量单个细胞中的EGFP荧光强度,准确确定抑制效率。对照实验表明不存在天然抑制或内源性氨酰-tRNA合成酶对合成tRNA的氨酰化作用。这种报告基因检测法为优化关键实验参数开辟了道路,从而将抑制性tRNA技术的应用范围扩展到不同细胞类型。

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