RECOMBINANT CALPAIN-II - IMPROVED EXPRESSION SYSTEMS AND PRODUCTION OF A 105A ACTIVE-SITE MUTANT FOR CRYSTALLOGRAPHY

被引:66
|
作者
ELCE, JS
HEGADORN, C
GAUTHIER, S
VINCE, JW
DAVIES, PL
机构
[1] Department of Biochemistry, Queen's University Kingston
来源
PROTEIN ENGINEERING | 1995年 / 8卷 / 08期
基金
英国医学研究理事会;
关键词
BICISTRONIC; CALPAIN; COMPATIBLE PLASMIDS; HIS-TAG; MUTAGENESIS;
D O I
10.1093/protein/8.8.843
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The bacterial production of recombinant rat calpain II has been improved greatly by the use of two compatible plasmids for the two subunits. The calpain small subunit C-terminal fragment (21 kDa) was expressed from a new A15-based vector created by cloning T7 control elements into pACYC177, This vector is compatible with the ColE1-based pET-24d(+) vector containing the calpain large subunit, and the yield of calpain activity was increased at least 16-fold by co-expression from these two vectors, A high level of activity was also obtained from a bicistronic construct containing both subunit cDNAs under the control of one T7 promoter. The addition of a C-terminal His-tag to the large subunit simplified purification without affecting subunit association or enzyme activity. The active-site cysteine 105 was mutated to alanine, causing complete loss of activity, The yield of purified C105A-calpain II (80 + 21 kDa) dimer following three column chromatography steps was 10 mg/l of cell culture, This provides a purified calpain, stable to autolysis and oxidation, which is likely to facilitate crystallization in both the presence and absence of calcium.
引用
收藏
页码:843 / 848
页数:6
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