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重组人法尼基蛋白转移酶的特性:克隆、表达、法尼基二磷酸结合以及与酵母异戊二烯基蛋白转移酶的功能同源性

Characterization of recombinant human farnesyl-protein transferase: cloning, expression, farnesyl diphosphate binding, and functional homology with yeast prenyl-protein transferases.

作者信息

Omer C A, Kral A M, Diehl R E, Prendergast G C, Powers S, Allen C M, Gibbs J B, Kohl N E

机构信息

Department of Cancer Research, Merck Research Laboratories, West Point, Pennsylvania 19486.

出版信息

Biochemistry. 1993 May 18;32(19):5167-76. doi: 10.1021/bi00070a028.

DOI:10.1021/bi00070a028
PMID:8494894
Abstract

We have isolated cDNAs encoding the alpha and beta subunits of human farnesyl-protein transferase (FPTase). The proteins encoded by these two cDNAs are 93-95% identical to the corresponding subunits of bovine and rat FPTase and show regions of homology with proteins encoded by Saccharomyces cerevisiae prenyl-protein transferase genes. Human FPTase expressed in Escherichia coli from a translationally coupled operon had kinetic properties similar to those of FPTase isolated from bovine brain. Examination of farnesyl diphosphate binding indicated that while neither individual subunit was capable of isoprenoid binding, a radiolabeled farnesyl diphosphate analog could be specifically photo-cross-linked to the beta subunit of FPTase holoenzyme. To further analyze subunit structure-function and to detect functional similarities with yeast prenyl-protein transferases (FPTase and two geranylgeranyl-protein transferases), amino acid changes homologous to those found in mutant yeast prenyl-protein transferase subunits were made in the subunits of human FPTase. Substitutions in either the alpha or beta subunits that decrease the activity of yeast prenyl-protein transferases were also observed to impair human FPTase. Kinetic analyses showed that these mutant human FPTases have Km and kcat values that are altered with respect to wild-type human FPTase.

摘要

我们已经分离出编码人法尼基蛋白转移酶(FPTase)α和β亚基的cDNA。这两个cDNA编码的蛋白质与牛和大鼠FPTase的相应亚基有93 - 95%的同一性,并且与酿酒酵母异戊二烯基蛋白转移酶基因编码的蛋白质显示出同源区域。从翻译偶联操纵子在大肠杆菌中表达的人FPTase具有与从牛脑中分离的FPTase相似的动力学性质。对法尼基二磷酸结合的研究表明,虽然单个亚基都不能结合类异戊二烯,但一种放射性标记的法尼基二磷酸类似物可以特异性地光交联到FPTase全酶的β亚基上。为了进一步分析亚基的结构功能,并检测与酵母异戊二烯基蛋白转移酶(FPTase和两种香叶基香叶基蛋白转移酶)的功能相似性,在人FPTase的亚基中进行了与突变酵母异戊二烯基蛋白转移酶亚基中发现的氨基酸变化同源的改变。在酵母异戊二烯基蛋白转移酶亚基中降低活性的α或β亚基中的取代也被观察到会损害人FPTase。动力学分析表明,这些突变的人FPTase的Km和kcat值相对于野生型人FPTase发生了改变。

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