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鉴定羊种布鲁氏菌16M菌株在山羊宿主中生存所需的基因。

Identification of Brucella melitensis 16M genes required for bacterial survival in the caprine host.

作者信息

Zygmunt Michel S, Hagius Sue D, Walker Joel V, Elzer Philip H

机构信息

UR 1282, Unité de Recherche Infectiologie Animale et Santé Publique, Institut National de la Recherche Agronomique, 3738 Nouzilly, France.

出版信息

Microbes Infect. 2006 Nov-Dec;8(14-15):2849-54. doi: 10.1016/j.micinf.2006.09.002. Epub 2006 Oct 16.

Abstract

Brucella species are gram-negative bacteria which belong to alpha-Proteobacteria family. These organisms are zoonotic pathogens that induce abortion and sterility in domestic mammals and chronic infections in humans known as Malta fever. The virulence of Brucella is dependent upon its ability to enter and colonize the cells in which it multiplies. The genetic basis of this aspect is poorly understood. Signature-tagged mutagenesis (STM) was used to identify potential Brucella virulence factors. PCR amplification has been used in place of DNA hybridization to identify the STM-generated attenuated mutants. A library of 288 Brucella melitensis 16M tagged mini-Tn5 Km2 mutants, in 24 pools, was screened for its ability to colonize spleen, lymph nodes and liver of goats at three weeks post-i.v. infection. This comparative screening identified 7 mutants (approximately 5%) which were not recovered from the output pool in goats. Some genes were known virulence genes involved in biosynthesis of LPS (lpsA gene) or in intracellular survival (the virB operon). Other mutants included ones which had a disrupted gene homologous to flgF, a gene coding for the basal-body rod of the flagellar apparatus, and another with a disruption in a gene homologous to ppk which is involved in the biosynthesis of inorganic polyphosphate (PolyP) from ATP. Other genes identified encoded factors involved in DNA metabolism and oxidoreduction metabolism. Using STM and the caprine host for screening, potential virulence determinants in B. melitensis have been identified.

摘要

布鲁氏菌属是革兰氏阴性菌,属于α-变形菌科。这些微生物是人畜共患病原体,可导致家畜流产和不育,以及人类的慢性感染,即马耳他热。布鲁氏菌的毒力取决于其进入并在其中繁殖的细胞中定殖的能力。这方面的遗传基础尚不清楚。利用签名标签诱变(STM)来鉴定潜在的布鲁氏菌毒力因子。已使用PCR扩增代替DNA杂交来鉴定STM产生的减毒突变体。在静脉内感染三周后,对一个由288个布鲁氏菌16M标记的mini-Tn5 Km2突变体组成的文库(分为24个池)进行筛选,以检测其在山羊脾脏、淋巴结和肝脏中定殖的能力。这种比较筛选鉴定出7个突变体(约5%),这些突变体在山羊的输出池中未被回收。一些基因是已知的毒力基因,参与脂多糖的生物合成(lpsA基因)或细胞内存活(virB操纵子)。其他突变体包括一个基因被破坏的突变体,该基因与flgF同源,flgF是一种编码鞭毛装置基体杆的基因,另一个突变体的一个与ppk同源的基因被破坏,ppk参与从ATP生物合成无机多聚磷酸盐(PolyP)。鉴定出的其他基因编码参与DNA代谢和氧化还原代谢的因子。利用STM和山羊宿主进行筛选,已鉴定出布鲁氏菌中的潜在毒力决定因素。

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