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使用非极性氯霉素抗性盒通过插入诱变鉴定大肠杆菌O4中的O抗原聚合酶(rfc)基因。

Identification of the O antigen polymerase (rfc) gene in Escherichia coli O4 by insertional mutagenesis using a nonpolar chloramphenicol resistance cassette.

作者信息

Lukomski S, Hull R A, Hull S I

机构信息

Department of Microbiology and Immunology, Baylor College of Medicine, Houston, Texas 77030, USA.

出版信息

J Bacteriol. 1996 Jan;178(1):240-7. doi: 10.1128/jb.178.1.240-247.1996.

Abstract

Computer analysis of the O4 polysaccharide gene cluster of Escherichia coli revealed the presence of two open reading frames (ORFs) encoding strongly hydrophobic polypeptides. O antigen polymerase, which is encoded by the rfc gene, is a potential membrane protein and therefore should be hydrophobic. To identify the rfc gene, these two ORFs were subjected to insertional mutagenesis. A chloramphenicol resistance cassette was designed which, when properly inserted, does not cause a polar effect in downstream genes. Each of two ORFs, cloned into a plasmid vector, was inactivated with this cassette. Two types of mutants bearing chromosomal insertions of the cassettes in each ORF were constructed by homologous recombination. These mutants were characterized by PCR, Southern blotting, and transverse-alternating-field electrophoresis. Only one class of mutants exhibited the expected O polymerase-deficient phenotype; they produced O4-specific, semirough lipopolysaccharide. Therefore, this ORF was identified as the rfc gene. The chromosomal rfc mutation was complemented in trans by the rfc gene expressed from a plasmid vector.

摘要

对大肠杆菌O4多糖基因簇进行计算机分析发现,存在两个编码强疏水性多肽的开放阅读框(ORF)。由rfc基因编码的O抗原聚合酶是一种潜在的膜蛋白,因此应该具有疏水性。为了鉴定rfc基因,对这两个ORF进行了插入诱变。设计了一个氯霉素抗性盒,当它正确插入时,不会对下游基因产生极性效应。将两个ORF分别克隆到质粒载体中,并用该盒使其失活。通过同源重组构建了两种在每个ORF中带有盒式染色体插入的突变体。通过PCR、Southern印迹和横向交变电场电泳对这些突变体进行了表征。只有一类突变体表现出预期的O聚合酶缺陷表型;它们产生O4特异性的半粗糙脂多糖。因此,这个ORF被鉴定为rfc基因。染色体rfc突变通过从质粒载体表达的rfc基因进行反式互补。

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