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Proofreading in Trans by an Aminoacyl-tRNA Synthetases Model for Single Site Editing by Isoleucyl-tRNA Synthetase

机译:反式的氨酰基-tRNA合成酶模型对异亮氨酸-tRNA合成酶进行单点校对

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摘要

Editing of errors in amino acid selection by an aminoacyl-tRNA synthetase prevents attachment of incorrect amino acids to tRNA, thereby greatly enhancing accuracy of translation of the genetic code. Editing of the non-protein amino acid homocysteine, a frequent type of an error-correcting process, involves reaction of the side chain sulfhydryl group of homocysteine with its activated carboxyl group forming a cyclic thioester, homocysteine thiolactone. Here, it is shown that isoleucyl-tRNA synthetase (lleRS), which occasionally misactivates homocysteine in vitro and in vivo, catalyzes reactions of activated isoleucine with organic thiols (analogues of the side chain of homocysteine). That these enzymatic reactions occur between Ile-tRNAIle or Ile-AMP (bound in the synthetic sub-site) and a thiol (an analogue of the side chain of homocysteine, bound in the editing sub-site), indicates that the two sub-sites are physically close on the surface of IleRS, forming a single synthetic/editing active site of the enzyme. Although IleRS?Val-AMP undergoes thiolysis as efficiently as do IleRS?Ile-AMP and IleRS?Ile-tRNAIle, IleRS?Val-tRNAIle does not react with thiols. These and other data suggest that the mischarged valine residue in IleRS?Val-tRNAIle is, most likely, positioned off the enzyme.
机译:通过氨基酸酰基-tRNA合成酶编辑氨基酸选择错误可防止将不正确的氨基酸附着到tRNA,从而大大提高了遗传密码翻译的准确性。非蛋白质氨基酸高半胱氨酸的编辑是一种常见的错误校正方法,涉及高半胱氨酸的侧链巯基与其活化的羧基反应,形成环状硫酯,高半胱氨酸硫代内酯。在这里,表明异亮氨酰-tRNA合成酶(lleRS)在体外和体内偶尔失活高半胱氨酸,它催化了活化的异亮氨酸与有机硫醇的反应(高半胱氨酸侧链的类似物)。这些酶促反应发生在Ile-tRNA Ile 或Ile-AMP(结合在合成子位点)和硫醇(高半胱氨酸侧链的类似物,结合在编辑子位点)之间),表示这两个子位点在IleRS的表面上物理上接近,形成了该酶的单个合成/编辑活性位点。尽管IleRS?Val-AMP与IleRS?Ile-AMP和IleRS?Ile-tRNA Ile 一样有效地进行硫解,但IleRS?Val-tRNA Ile 不会与硫醇反应。这些和其他数据表明,IleRS?Val-tRNA Ile 中错误带电荷的缬氨酸残基很可能位于酶的附近。

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