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一种用于枯草芽孢杆菌中系统基因失活的载体。

A vector for systematic gene inactivation in Bacillus subtilis.

作者信息

Vagner Valerie, Dervyn Etienne, Ehrlich S Dusko

机构信息

Genetique Microbienne, lnstitut National de la Recherche Ag ronom ique,Domaine de Vilvefl, 78352 Jouy-en-Josas cedex,France.

出版信息

Microbiology (Reading). 1998 Nov;144 ( Pt 11):3097-3104. doi: 10.1099/00221287-144-11-3097.

Abstract

To study the functions of the uncharacterized open reading frames identified in the Bacillus subtilis genome, several vectors were constructed to perform insertional mutagenesis in the chromosome. All the pMUTIN plasmids carry a lacZ reporter gene and an inducible Pspac promoter, which is tightly regulated and can be induced about 1000-fold. The integration of a pMUTIN vector into the target gene has three consequences: (1) the target gene is inactivated; (2) lacZ becomes transcriptionally fused to the gene, allowing its expression pattern to be monitored; (3) the Pspac promoter controls the transcription of downstream genes in an IPTG-dependent fashion. This last feature is important because B. subtilis genes are often organized in operons. The potential polar effects generated by the integration of the vectors can be alleviated by addition of IPTG. Also, conditional mutants of essential genes can be obtained by integrating pMUTIN vectors upstream of the target gene. The vectors are currently being used for systematic inactivation of genes without known function within the B. subtilis European consortium. pMUTIN characteristics and the inactivation of eight genes in the resA-serA region of the chromosome are presented.

摘要

为了研究在枯草芽孢杆菌基因组中鉴定出的未表征开放阅读框的功能,构建了几种载体以在染色体中进行插入诱变。所有pMUTIN质粒都携带一个lacZ报告基因和一个可诱导的Pspac启动子,该启动子受到严格调控,可被诱导约1000倍。pMUTIN载体整合到靶基因中会产生三个结果:(1)靶基因失活;(2)lacZ与该基因转录融合,从而可以监测其表达模式;(3)Pspac启动子以IPTG依赖的方式控制下游基因的转录。最后一个特征很重要,因为枯草芽孢杆菌基因通常以操纵子形式组织。通过添加IPTG可以减轻载体整合产生的潜在极性效应。此外,通过将pMUTIN载体整合到靶基因上游,可以获得必需基因的条件突变体。目前,这些载体正在枯草芽孢杆菌欧洲联盟内用于对无已知功能的基因进行系统失活。本文介绍了pMUTIN的特性以及染色体resA-serA区域中八个基因的失活情况。

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