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基于mRNA展示技术筛选具有所需功能的蛋白质:蛋白酶-底物案例研究

mRNA-display-based selections for proteins with desired functions: a protease-substrate case study.

作者信息

Valencia C Alexander, Cotten Steven W, Dong Biao, Liu Rihe

机构信息

School of Pharmacy and Carolina Center for Genomic Sciences, The University of North Carolina at Chapel Hill, Chapel Hill, North Carolina 27599, USA.

出版信息

Biotechnol Prog. 2008 May-Jun;24(3):561-9. doi: 10.1021/bp070473a. Epub 2008 May 10.

Abstract

mRNA-display is an amplification-based, iterative rounds of in vitro protein selection technique that circumvents a number of difficulties associated with yeast two-hybrid and phage display. Because of the covalent linkage between the genotype and the phenotype, mRNA-display provides a powerful means for reading and amplifying a peptide or protein sequence after it has been selected from a library with a diversity in the range of 10(12)-10(13). In this paper, we briefly review the recent progress in using mRNA-display to identify affinity reagents, binding partners, and enzyme substrates from synthetic peptide or natural proteome libraries. To facilitate the use of mRNA-display in research laboratories without previous experience, we provide a detailed analysis of the critical steps of an mRNA-display-based selection in a case study for the identification of the natural substrates of caspases, including the generation of an mRNA-displayed proteome library, removal of abundant sequences, and selection of proteins with desired functions. The advantages and technical limitations of mRNA-display as a general peptide or protein selection tool are also addressed.

摘要

信使核糖核酸展示技术是一种基于扩增的、多轮体外蛋白质筛选技术,它克服了与酵母双杂交和噬菌体展示相关的许多困难。由于基因型和表型之间的共价连接,信使核糖核酸展示技术为从多样性范围在10(12)-10(13)的文库中筛选出肽或蛋白质序列后读取和扩增该序列提供了一种强大的手段。在本文中,我们简要回顾了利用信使核糖核酸展示技术从合成肽或天然蛋白质组文库中鉴定亲和试剂、结合伴侣和酶底物的最新进展。为便于没有前期经验的研究实验室使用信使核糖核酸展示技术,我们在一个鉴定半胱天冬酶天然底物的案例研究中,对基于信使核糖核酸展示技术的筛选关键步骤进行了详细分析,包括构建信使核糖核酸展示的蛋白质组文库、去除丰度高的序列以及筛选具有所需功能的蛋白质。还讨论了信使核糖核酸展示技术作为一种通用的肽或蛋白质筛选工具的优点和技术局限性。

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