鉴定和克隆肽合成酶基因的一般方法。

Peptide research Pub Date : 1994-09-01
K Turgay, M A Marahiel
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引用次数: 0

摘要

各种各样的生物活性肽是由大型多酶复合物采用硫模板机制非核糖体合成的。基于一些已知的和高度保守的编码多肽合成酶的基因结构,我们开发了一种通用聚合酶链反应(PCR)方法来扩增,克隆和鉴定部分推定的多肽合成酶基因。通过克隆产相毒素的假单胞菌pv的肽合成酶基因片段,我们发现。从地衣芽孢杆菌,它产生支肽抗生素杆菌肽,这种方法是适用的。它为许多非核糖体合成肽的生物合成基因提供了一个新的和潜在的通用途径。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A general approach for identifying and cloning peptide synthetase genes.

A wide variety of bioactive peptides are synthesized nonribosomally by large multienzyme complexes employing the thiotemplate mechanism. Based on the known and highly conserved structures of several genes encoding multifunctional peptide synthetases, we developed a universal polymerase chain reaction (PCR) approach for amplifying, cloning and identifying parts of putative peptide synthetase genes. We showed, by cloning fragments of peptide synthetase genes from the phaseolotoxin-producing strain Pseudomonas syringe pv. phaseolica and from Bacillus licheniformis, which produces the branched peptide antibiotic bacitracin, that this approach is applicable. It gives a new and potentially general access to the biosynthetic genes of many nonribosomally synthesized peptides.

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