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产气荚膜梭菌中编码依赖丙酮酰的组氨酸脱羧酶的基因的克隆、测序、表达及定点诱变

Cloning, sequencing, expression, and site-directed mutagenesis of the gene from Clostridium perfringens encoding pyruvoyl-dependent histidine decarboxylase.

作者信息

van Poelje P D, Snell E E

机构信息

Department of Chemistry, University of Texas, Austin 78712.

出版信息

Biochemistry. 1990 Jan 9;29(1):132-9. doi: 10.1021/bi00453a016.

DOI:10.1021/bi00453a016
PMID:2108713
Abstract

The DNA encoding pyruvoyl-dependent histidine decarboxylase (HisDCase) of Clostridium perfringens was cloned, sequenced, and overexpressed in Escherichia coli. The gene encodes a single polypeptide of 320 amino acids, Mr 35,526, demonstrating that clostridial HisDCase, which has an (alpha beta)6 structure, is synthesized as a precursor (proHisDCase, pi 6). No pi subunits of proHisDCase were observed in crude or purified preparations of the cloned HisDCase; they appear to undergo rapid cleavage in vivo to the alpha (Mr 24,887) and beta (Mr 10,526) subunits characteristic of this HisDCase. This cleavage occurs between Ser-96 and Ser-97; Ser-97 gives rise to the catalytically essential pyruvoyl group blocking the N-termini of the alpha subunits of the active enzyme. When Ser-97 was converted to an alanyl residue by site-specific mutagenesis, the expressed, inactive protein (pi' 6) contained a single peptide species (pi', Mr 35,510) that was not cleaved either in vivo or in vitro. These results support previous conclusions that activation of the wild-type clostridial proenzyme occurs via nonhydrolytic serinolysis. Although clostridial HisDCase has only a 47% sequence similarity to HisDCase from Lactobacillus 30a, all of the residues known to be important for substrate binding and catalytic action of the Lactobacillus HisDCase are conserved in the C. perfringens enzyme. While the encoded N-terminal Met of clostridial HisDCase is removed by E. coli, the cloned enzyme retains a 10-residue presequence (NKNLEANRNR) not present in the mature enzyme isolated from C. perfringens.

摘要

产气荚膜梭菌中编码依赖丙酮酰基的组氨酸脱羧酶(HisDCase)的DNA被克隆、测序,并在大肠杆菌中过中过表达。该基因编码一个由320个氨基酸组成的单一多肽,分子量为35,526,表明具有(αβ)6结构的梭菌HisDCase是以前体形式(proHisDCase,pI 6)合成的。在克隆的HisDCase的粗提物或纯化制剂中未观察到proHisDCase的pI亚基;它们似乎在体内迅速裂解为该HisDCase特有的α亚基(分子量24,887)和β亚基(分子量10,526)。这种裂解发生在Ser-96和Ser-97之间;Ser-97产生了活性酶α亚基N端封闭的催化必需丙酮酰基。当通过定点诱变将Ser-97转化为丙氨酰残基时,表达的无活性蛋白(pI' 6)包含一个单一肽段(pI',分子量35,510),其在体内或体外均未裂解。这些结果支持了先前的结论,即野生型梭菌原酶的激活是通过非水解性丝氨酸解作用发生的。尽管梭菌HisDCase与来自乳酸杆菌30a的HisDCase只有47%的序列相似性,但已知对乳酸杆菌HisDCase的底物结合和催化作用重要的所有残基在产气荚膜梭菌酶中都是保守的。虽然梭菌HisDCase编码的N端甲硫氨酸被大肠杆菌去除,但克隆的酶保留了一个10个残基的前导序列(NKNLEANRNR),该序列不存在于从产气荚膜梭菌分离的成熟酶中。

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