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首页> 外文期刊>Protein Engineering >COMBINATORIAL MANIPULATION OF THREE KEY ACTIVE SITE RESIDUES IN GLYCINAMIDE RIBONUCLEOTIDE TRANSFORMYLASE
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COMBINATORIAL MANIPULATION OF THREE KEY ACTIVE SITE RESIDUES IN GLYCINAMIDE RIBONUCLEOTIDE TRANSFORMYLASE

机译:甘氨酰胺核糖核苷酸转化酶中三个关键活性位点残基的组合操作

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摘要

The enzyme glycinamide ribonucleotide transformylase (EC 2.1.2.2) has previously been shown to have three key polar active site residues important for catalysis: N106, H108 and D144, Mutations of any of these three residues lead to substantially decreased catalytic activity, although none of them are completely irreplaceable. In order to determine whether any alternative arrangement of amino acids at these three positions could lead to an active protein, all three of these residues were simultaneously subjected to saturation site-directed mutagenesis. The resulting combinatorial library of mutant genes was screened for those encoding active proteins using functional complementation, Glycinamide ribonucleotide transformylase was found to be capable of tolerating no more than one mutation amongst these key residues, since the only proteins found to be sufficiently active to allow growth of auxotrophic cells on selective media were the wild-type and enzymes containing a single mutation to one of these residues. It seems likely that no enzymes containing two or more mutations of these three residues possess significant catalytic activity, The combinatorial approach used could prove to be quite useful in protein engineering and protein evolution experiments. [References: 11]
机译:以前已证明甘氨酰胺核糖核苷酸转化酶(EC 2.1.2.2)具有三个对催化重要的关键极性活性位点残基:N106,H108和D144,这三个残基中的任何一个突变都会导致催化活性大大降低,尽管没有一个它们是完全不可替代的。为了确定在这三个位置上氨基酸的任何替代排列是否都可以导致活性蛋白,将所有这三个残基同时进行饱和定点诱变。使用功能互补对所得的突变基因组合文库进行筛选,筛选出编码活性蛋白的那些,发现甘氨酰胺核糖核苷酸转化酶能够耐受这些关键残基中的不超过一个突变,因为发现的唯一蛋白具有足够的活性以允许生长选择性培养基上的营养缺陷型细胞是野生型,并且这些残基之一含有单个突变的酶。似乎没有包含这三个残基的两个或多个突变的酶具有明显的催化活性。所使用的组合方法可能被证明在蛋白质工程和蛋白质进化实验中非常有用。 [参考:11]

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