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C 端特异性蛋白质降解:Tsp 蛋白酶的活性与底物特异性

C-terminal specific protein degradation: activity and substrate specificity of the Tsp protease.

作者信息

Keiler K C, Silber K R, Downard K M, Papayannopoulos I A, Biemann K, Sauer R T

机构信息

Department of Biology, Massachusetts Institute of Technology, Cambridge 02139, USA.

出版信息

Protein Sci. 1995 Aug;4(8):1507-15. doi: 10.1002/pro.5560040808.

Abstract

The activity of Tsp, a periplasmic endoprotease of Escherichia coli, has been characterized by assaying the cleavage of protein and peptide substrates, determining the cleavage sites in several substrates, and investigating the kinetics of the cleavage reaction. Tsp efficiently cleaves substrates that have apolar residues and a free alpha-carboxylate at the C-terminus. Tsp cleaves its substrates at a discrete number of sites but with rather broad primary sequence specificity. In addition to preferences for residues at the C-terminus and cleavage sites, Tsp displays a preference for substrates that are not stably folded: unstable variants of Arc repressor are better substrates than a hyperstable mutant, and a peptide with little stable structure is cleaved more efficiently than a protein substrate. These data are consistent with a model in which Tsp cleavage of a protein substrate involves binding to the C-terminal tail of the substrate, transient denaturation of the substrate, and then recognition and hydrolysis of specific peptide bonds.

摘要

通过检测蛋白质和肽底物的切割情况、确定几种底物中的切割位点以及研究切割反应的动力学,对大肠杆菌周质内蛋白酶Tsp的活性进行了表征。Tsp能有效切割在C端具有非极性残基和游离α - 羧基的底物。Tsp在离散数量的位点切割其底物,但具有相当广泛的一级序列特异性。除了对C端残基和切割位点有偏好外,Tsp还表现出对不稳定折叠底物的偏好:Arc阻遏物的不稳定变体比超稳定突变体是更好的底物,并且结构稳定性低的肽比蛋白质底物更有效地被切割。这些数据与一个模型一致,在该模型中,Tsp对蛋白质底物的切割涉及与底物C端尾部的结合、底物的瞬时变性,然后识别并水解特定的肽键。

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