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半胱氨酸在人卵磷脂胆固醇酰基转移酶中的作用。

Roles of cysteines in human lecithin:cholesterol acyltransferase.

作者信息

Qu S J, Fan H Z, Blanco-Vaca F, Pownall H J

机构信息

Department of Medicine, Baylor College of Medicine, Houston, Texas 77030.

出版信息

Biochemistry. 1993 Mar 30;32(12):3089-94. doi: 10.1021/bi00063a021.

DOI:10.1021/bi00063a021
PMID:8457570
Abstract

Human lecithin:cholesterol acyltransferase (LCAT, E.C.2.3.1.43) is a serine-type esterase that contains six cysteines, two of which, Cys31 and Cys184, are free. The remaining cysteines form disulfide links. One of these is between Cys50 and Cys74 and the other is between Cys313 and Cys356. The cDNA of LCAT and mutants in which one or two of the six cysteines were replaced by glycine was expressed in COS-6 cells. Polymerase chain reactions and Northern blot analysis indicated that LCAT mRNA was produced by all transfectants. Western blots of all transfected cells probed with a polyclonal antibody revealed intracellular LCAT. Substitution of glycine for either Cys50, Cys74, Cys313, or Cys356 was associated with a nearly total absence of activity in the medium. No protein was secreted when glycine replaced either of the amino acid residues that link Cys313 and Cys356. The small amounts of the Cys50-->Gly and Cys74-->Gly mutants found in the medium had specific activities that were much lower than that of the wild-type LCAT. All other transfectants secreted immunologically measurable amounts of active enzyme. Mutants in which one or both free cysteines, Cys31 and Cys184, were replaced with glycine were less active than the wild type and only partially inhibited by a sulfhydryl blocking reagent. The substrate specificities of the Cys31-->Gly and Cys184-->Gly mutants differed from that of the wild type.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

人卵磷脂

胆固醇酰基转移酶(LCAT,E.C.2.3.1.43)是一种丝氨酸型酯酶,含有6个半胱氨酸,其中两个半胱氨酸,即Cys31和Cys184是游离的。其余的半胱氨酸形成二硫键。其中一个二硫键在Cys50和Cys74之间,另一个在Cys313和Cys356之间。LCAT的cDNA以及其中6个半胱氨酸中的一个或两个被甘氨酸取代的突变体在COS-6细胞中表达。聚合酶链反应和Northern印迹分析表明,所有转染细胞都产生了LCAT mRNA。用多克隆抗体检测所有转染细胞的Western印迹显示细胞内有LCAT。用甘氨酸取代Cys50、Cys74、Cys313或Cys356中的任何一个与培养基中几乎完全没有活性相关。当甘氨酸取代连接Cys313和Cys356的任何一个氨基酸残基时,没有蛋白质分泌。在培养基中发现的少量Cys50→Gly和Cys74→Gly突变体的比活性远低于野生型LCAT。所有其他转染细胞分泌免疫可检测量的活性酶。其中一个或两个游离半胱氨酸Cys31和Cys184被甘氨酸取代的突变体的活性低于野生型,并且仅被巯基封闭剂部分抑制。Cys31→Gly和Cys184→Gly突变体的底物特异性与野生型不同。(摘要截短至250字)

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