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Novel plasmids for gene expression analysis and for genetic manipulation in the gastric pathogen Helicobacter pylori.

机译:用于在胃病原体幽门螺杆菌中进行基因表达分析和基因操作的新型质粒。

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To facilitate gene expression analysis in the human gastric pathogen Helicobacter pylori, we constructed the plasmids pHPLAC-KAN and pHPLAC-CAT containing a promoterless Escherichia coli lacZ gene located upstream from the antibiotic resistance genes aphA-3 or cat, respectively. The suitability of the plasmids for H. pylori mutagenesis and gene expression analysis was evaluated by plasmid integration into the genome of H. pylori strain 1061 by single homologous recombination, using the rpl9 gene encoding ribosomal protein L9 as target. By monitoring beta-galactosidase production from the resulting rpl9::lacZ fusion, it was demonstrated that H. pylori rpl9 displays the classical growth phase-dependent regulation of components of the protein synthesis machinery, as beta-galactosidase production dropped fivefold in the stationary growth phase. The plasmids described in this study extend our methodological repertoire for genetic modification and molecular analysis of H. pylori, and may also be of use for other bacteria, as the resistance cassettes and the lacZ gene are active in the related Campylobacter species.
机译:为了促进人胃病原体幽门螺杆菌中的基因表达分析,我们构建了质粒pHPLAC-KAN和pHPLAC-CAT,它们分别包含位于抗生素抗性基因aphA-3或cat上游的无启动子大肠杆菌lacZ基因。使用编码核糖体蛋白L9的rpl9基因作为靶标,通过单次同源重组将质粒整合入幽门螺杆菌菌株1061的基因组中,评估质粒对幽门螺杆菌诱变和基因表达分析的适用性。通过监测所得rpl9 :: lacZ融合体产生的β-半乳糖苷酶产量,证明幽门螺杆菌rpl9表现出蛋白质合成机制各组分的经典生长阶段依赖性调节,因为β-半乳糖苷酶产量在固定生长中下降了五倍相。这项研究中描述的质粒扩展了我们的方法库,可用于幽门螺杆菌的基因修饰和分子分析,并且还可用于其他细菌,因为耐药盒和lacZ基因在相关弯曲杆菌属中具有活性。

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