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利用 ara 系统和 asd 基因通过遗传重组构建条件致死性沙门氏菌突变体。

Construction of a conditional lethal Salmonella mutant via genetic recombination using the ara system and asd gene.

机构信息

Swine Science & Technology Center, Gyeongnam National University of Science and Technology, 150 Chilam-dong, Jinju, Gyeongnam, 660-758, South Korea.

出版信息

J Microbiol Methods. 2011 Nov;87(2):202-7. doi: 10.1016/j.mimet.2011.08.004. Epub 2011 Aug 17.

Abstract

In order to construct a conditional lethal Salmonella mutant, an arabinose-regulated recombinant genetic system was used. The Salmonella aspartate semialdehyde dehydrogenase (asd) gene was localized under the control of araC P(araBAD) in a plasmid to create the araC P(araBAD)::asd cassette. The cassette was cloned into a plasmid carrying a p15A replication origin to create the recombinant plasmid pMMP55. The growth of Salmonella MMP10 harboring pMMP55 was dependent on the presence of arabinose. In the presence of arabinose, the Asd deficiency due to chromosomal deletion of asd in the Salmonella host was complemented by the asd gene transcribed and translated under the P(araBAD) promoter and araBAD Shine-Dalgarno (SD) sequence in pMMP55. Growth inhibition of the strain was demonstrated by arabinose depletion in M9 minimal medium, indicating that the strain were unable to grow in an arabinose-limited environment. In addition, the analysis of a 50% lethal dose (LD50) using mice revealed that the strain MMP10 exhibited attenuation by approximately 100-fold relative to that of the unmodified strain. In conclusion, these data suggest that the araC P(araBAD)::asd system developed in this study can be used to construct conditional lethal Salmonella mutants for application as safe, live-attenuated Salmonella vaccines.

摘要

为了构建条件致死性沙门氏菌突变体,我们使用了阿拉伯糖调控的重组遗传系统。将沙门氏菌天冬氨酸半醛脱氢酶(asd)基因置于 araC P(araBAD)的控制下,在质粒中创建 araC P(araBAD)::asd 盒。该盒被克隆到携带 p15A 复制原点的质粒中,以创建重组质粒 pMMP55。携带 pMMP55 的沙门氏菌 MMP10 的生长依赖于阿拉伯糖的存在。在阿拉伯糖存在的情况下,由于沙门氏菌宿主中 asd 基因的缺失导致 Asd 缺乏,由 pMMP55 中 P(araBAD)启动子和 araBAD Shine-Dalgarno (SD)序列转录和翻译的 asd 基因进行了补充。在 M9 最小培养基中通过阿拉伯糖耗尽证明了菌株的生长抑制,表明该菌株无法在阿拉伯糖有限的环境中生长。此外,使用小鼠分析 50%致死剂量 (LD50) 表明,与未修饰的菌株相比,菌株 MMP10 的衰减约为 100 倍。总之,这些数据表明,本研究中开发的 araC P(araBAD)::asd 系统可用于构建条件致死性沙门氏菌突变体,作为安全的、活减毒沙门氏菌疫苗。

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