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创伤弧菌中荚膜合成所必需的一种表异构酶基因。

An epimerase gene essential for capsule synthesis in Vibrio vulnificus.

作者信息

Zuppardo A B, Siebeling R J

机构信息

Department of Biological Sciences, Louisiana State University, Baton Rouge, Louisiana 70803, USA.

出版信息

Infect Immun. 1998 Jun;66(6):2601-6. doi: 10.1128/IAI.66.6.2601-2606.1998.

Abstract

The extracellular capsule polysaccharide (CPS) of Vibrio vulnificus is a primary virulence factor which allows survival of the bacteria in the human host. To study the genes involved in expression of the capsule, we generated mutants that lost the ability to produce CPS following the insertion of a minitransposon into the genome of an encapsulated, clinical strain of V. vulnificus. A genomic region, from one nonencapsulated mutant, containing the transposon and flanking V. vulnificus DNA was cloned, and a probe complementary to the chromosomal DNA immediately adjacent to the transposon was used to locate this fragment in the genome of the encapsulated parent strain. The fragment, which contained a putative capsule gene, was cloned and, when supplied in trans, complemented the mutation in the nonencapsulated mutant to restore capsule production. In addition, virulence studies, using the 50% lethal dose assay, showed that the restoration of capsule production also restored the virulence of the organism. Sequence analysis of the gene disrupted by the transposon revealed that it matched a nucleotide-sugar epimerase of Vibrio cholerae O139, with 75 and 85% identities at the nucleotide and amino acid levels, respectively. In addition, computer analysis recognized epimerases of various organisms as highly similar to the putative epimerase of V. vulnificus. Finally, a combination of PCR amplification and Southern blotting showed that this epimerase is common to at least 10 strains of V. vulnificus that each express a serologically distinct CPS. Our results indicate that the epimerase gene is essential for capsule expression in V. vulnificus.

摘要

创伤弧菌的细胞外荚膜多糖(CPS)是一种主要的毒力因子,它使细菌能够在人类宿主中存活。为了研究参与荚膜表达的基因,我们构建了一些突变体,这些突变体是通过将一个微型转座子插入到一株有荚膜的创伤弧菌临床菌株的基因组中后,失去了产生CPS的能力。从一个无荚膜突变体中克隆了一个包含转座子和侧翼创伤弧菌DNA的基因组区域,并使用一个与紧邻转座子的染色体DNA互补的探针,在有荚膜的亲本菌株基因组中定位该片段。包含一个假定的荚膜基因的片段被克隆出来,当以反式提供时,它互补了无荚膜突变体中的突变,从而恢复了荚膜的产生。此外,使用50%致死剂量测定法进行的毒力研究表明,荚膜产生的恢复也恢复了该生物体的毒力。对被转座子破坏的基因进行序列分析发现,它与霍乱弧菌O139的一种核苷酸 - 糖差向异构酶匹配,在核苷酸和氨基酸水平上分别具有75%和85%的同一性。此外,计算机分析识别出各种生物体的差向异构酶与创伤弧菌假定的差向异构酶高度相似。最后,PCR扩增和Southern印迹分析相结合表明,这种差向异构酶在至少10株创伤弧菌中是常见的,这些菌株各自表达一种血清学上不同的CPS。我们的结果表明,差向异构酶基因对于创伤弧菌的荚膜表达至关重要。

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本文引用的文献

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Novel Vibrio cholerae O139 genes involved in lipopolysaccharide biosynthesis.
J Bacteriol. 1997 Apr;179(8):2740-7. doi: 10.1128/jb.179.8.2740-2747.1997.
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Annu Rev Microbiol. 1996;50:285-315. doi: 10.1146/annurev.micro.50.1.285.
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