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使用杆状病毒表达系统生产的具有生物活性的单体和异源二聚体重组人钙蛋白酶I。

Biologically active monomeric and heterodimeric recombinant human calpain I produced using the baculovirus expression system.

作者信息

Meyer S L, Bozyczko-Coyne D, Mallya S K, Spais C M, Bihovsky R, Kaywooya J K, Lang D M, Scott R W, Siman R

机构信息

Cephalon, Inc., West Chester, PA 19380, U.S.A.

出版信息

Biochem J. 1996 Mar 1;314 ( Pt 2)(Pt 2):511-9. doi: 10.1042/bj3140511.

Abstract

Calpain I is a heterodimeric protein that is part of a family of calcium-activated intracellular cysteine proteases presumed to play a role in mediating signals transduced by calcium. Expression of bioactive recombinant human calpain I has been achieved using the baculovirus expression system, by either co-infection with two viruses, each expressing one of the subunits, or infection with a single virus containing both subunits. The approximately 80 kDa catalytic subunit exhibited calcium-dependent proteolytic activity when expressed alone or with the approximately 30 kDa regulatory subunit. Baculoviral recombinant calpain I appeared fully active in that the catalytic subunit in unpurified cell extracts exhibited calcium-dependent autocatalytic cleavage at the correct locus. The amount of approximately 80 kDa subunit accumulated at steady state was greatly increased by co-expression of the approximately 30 kDa subunit, suggesting a possible role for enzyme stabilization by the latter subunit. The recombinant human calpain I was purified to near homogeneity and compared with purified native human erythrocyte calpain I. The recombinant and native enzymes had equivalent inhibition constants for structurally diverse calpain inhibitors, identical calcium activation profiles, and similar specific activities, demonstrating the suitability of using the recombinant protein for studies of the native enzyme.

摘要

钙蛋白酶I是一种异二聚体蛋白,属于钙激活的细胞内半胱氨酸蛋白酶家族,推测其在介导由钙转导的信号中发挥作用。使用杆状病毒表达系统已实现生物活性重组人钙蛋白酶I的表达,方法是通过两种病毒共感染,每种病毒表达一个亚基,或者用含有两个亚基的单一病毒感染。单独表达或与约30 kDa调节亚基一起表达时,约80 kDa的催化亚基表现出钙依赖性蛋白水解活性。杆状病毒重组钙蛋白酶I似乎完全有活性,因为未纯化的细胞提取物中的催化亚基在正确位点表现出钙依赖性自催化切割。通过共表达约30 kDa亚基,稳态时积累的约80 kDa亚基的量大大增加,这表明后者亚基可能在酶稳定中发挥作用。重组人钙蛋白酶I被纯化至接近均一,并与纯化的天然人红细胞钙蛋白酶I进行比较。重组酶和天然酶对结构多样的钙蛋白酶抑制剂具有相同的抑制常数,相同的钙激活曲线,以及相似的比活性,这表明使用重组蛋白研究天然酶是合适的。

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