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基于聚合酶链反应的新型抗菌肽brevinin-2R在大肠杆菌中的基因合成、分子克隆、高水平表达、纯化及特性分析

PCR-based gene synthesis, molecular cloning, high level expression, purification, and characterization of novel antimicrobial peptide, brevinin-2R, in Escherichia coli.

作者信息

Mehrnejad Faramarz, Naderi-Manesh Hossein, Ranjbar Bijan, Maroufi Bahman, Asoodeh Ahmad, Doustdar Farahnoosh

机构信息

Department of Biophysics, Faculty of Science, Tarbiat Modarres University, Tehran, Iran.

出版信息

Appl Biochem Biotechnol. 2008 May;149(2):109-18. doi: 10.1007/s12010-007-8024-z. Epub 2007 Sep 5.

Abstract

Brevinin-2R, a member of a new family of antimicrobial peptides isolated from the skin of Rana ridibunda, displays antimicrobial activity against bacteria and fungi. In this study, we have used an assembly PCR method for the fast and extremely accurate synthesis of the brevinin-2R gene. A total of six primers were assembled in a single step PCR, and the assembly was then amplified by PCR to produce the final gene. The synthetic gene was cloned into the pET32a (+) vector to allow the expression of brevinin-2R as a Trx fusion protein in Escherichia coli. The results indicated that the expression level of the fusion protein could reach up to 25% of the total cell proteins. The expression products could be easily purified by Ni-NTA chromatography and released from the fusion protein by factor Xa protease. The peptide displayed antimicrobial activity similar to that of the purified brevinin that was reported earlier. This method allows the fast synthesis of a gene that optimized the overexpression in the E. coli system and production of sufficiently large amounts of peptide for functional and structural characterizations.

摘要

Brevinin-2R是从食用蛙皮肤中分离出的一个新的抗菌肽家族的成员,对细菌和真菌具有抗菌活性。在本研究中,我们使用了一种组装PCR方法来快速且极其准确地合成brevinin-2R基因。总共六个引物在一步PCR中组装,然后通过PCR扩增该组装体以产生最终基因。将合成基因克隆到pET32a(+)载体中,以便在大肠杆菌中表达作为Trx融合蛋白的brevinin-2R。结果表明,融合蛋白的表达水平可达总细胞蛋白的25%。表达产物可通过Ni-NTA色谱轻松纯化,并通过Xa因子蛋白酶从融合蛋白中释放出来。该肽显示出与先前报道的纯化brevinin相似的抗菌活性。这种方法允许快速合成一个优化了在大肠杆菌系统中过表达的基因,并生产出足够大量的肽用于功能和结构表征。

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