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酵母人工染色体中人类载脂蛋白B基因的诱变揭示了载脂蛋白(a)的附着位点。

Mutagenesis of the human apolipoprotein B gene in a yeast artificial chromosome reveals the site of attachment for apolipoprotein(a).

作者信息

McCormick S P, Ng J K, Taylor S, Flynn L M, Hammer R E, Young S G

机构信息

Gladstone Institute of Cardiovascular Disease, San Francisco, CA 94141-9100, USA.

出版信息

Proc Natl Acad Sci U S A. 1995 Oct 24;92(22):10147-51. doi: 10.1073/pnas.92.22.10147.

Abstract

Lipoprotein(a) [Lp(a)] is a lipoprotein formed by the disulfide linkage of apolipoprotein (apo) B100 of a low density lipoprotein particle to apolipoprotein(a). Prior studies have suggested that one of the C-terminal Cys residues of apo-B100 is involved in the disulfide linkage of apo-B100 to apo(a). To identify the apo-B100 Cys residue involved in the formation of Lp(a), we constructed a yeast artificial chromosome (YAC) spanning the human apo-B gene and used gene-targeting techniques to change Cys-4326 to Gly. The mutated YAC DNA was used to generate transgenic mice expressing the mutant human apo-B100 (Cys4326Gly). Unlike the wild-type human apo-B100, the mutant human apo-B100 completely lacked the ability to bind to apo(a) and form Lp(a). This study demonstrates that apo-B100 Cys-4326 is required for the assembly of Lp(a) and shows that gene targeting in YACs, followed by the generation of transgenic mice, is a useful approach for analyzing the structure of large proteins coded for by large genes.

摘要

脂蛋白(a)[Lp(a)]是一种由低密度脂蛋白颗粒的载脂蛋白(apo)B100与载脂蛋白(a)通过二硫键连接形成的脂蛋白。先前的研究表明,apo-B100的一个C末端半胱氨酸残基参与了apo-B100与apo(a)的二硫键连接。为了鉴定参与Lp(a)形成的apo-B100半胱氨酸残基,我们构建了一个跨越人类apo-B基因的酵母人工染色体(YAC),并使用基因靶向技术将半胱氨酸-4326突变为甘氨酸。突变的YAC DNA被用于生成表达突变型人类apo-B100(Cys4326Gly)的转基因小鼠。与野生型人类apo-B100不同,突变型人类apo-B100完全丧失了与apo(a)结合并形成Lp(a)的能力。这项研究表明,apo-B100半胱氨酸-4326是Lp(a)组装所必需的,并表明在YAC中进行基因靶向,随后生成转基因小鼠,是分析由大基因编码的大蛋白结构的一种有用方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8538/40753/0dea436a6621/pnas01500-0246-a.jpg

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