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编码与细胞黏附相关蛋白HMW1的重组基因在肺炎支原体中的表达以及将HMW4鉴定为一种产物。

Expression in Mycoplasma pneumoniae of the recombinant gene encoding the cytadherence-associated protein HMW1 and identification of HMW4 as a product.

作者信息

Hahn T W, Krebes K A, Krause D C

机构信息

Department of Microbiology, University of Georgia, Athens 30602, USA.

出版信息

Mol Microbiol. 1996 Mar;19(5):1085-93. doi: 10.1046/j.1365-2958.1996.455985.x.

Abstract

Mycoplasma pneumoniae is a major cause of tracheobronchitis and pneumonia in older children and young adults. The lack of adequate tools for genetic analysis has hindered the elucidation of function and regulation of mycoplasma virulence determinants. We describe here the use of a transposon vector to deliver the cloned gene for the cytadherence-associated protein HMW1 in M. pneumoniae. A 4.95 kbp BamHI fragment encoding all but the C-terminal end of HMW1 was cloned into a modified Tn4001 and transformed into wild-type M. pneumoniae and into a non-cytadhering mutant lacking HMW1-HMW5. Southern blot hybridizations confirmed insertion of the transposon and the presence of both the resident and recombinant hmw1 alleles. Analysis by Western immunoblotting revealed a truncated HMW1 (HMW1') in the transformants, the level of HMW1' being dependent upon the orientation of the hmw1 gene in the transposon and the site of insertion. Similar expression patterns were noted in wild-type and mutant backgrounds. However, expression of wild-type levels of HMW1' in the mutant did not restore adherence. Finally, HMW4 and HMW1 were shown to be products of the same gene, HMW4 being a heat-modified derivative of HMW1.

摘要

肺炎支原体是大龄儿童和青年气管支气管炎及肺炎的主要病因。缺乏足够的基因分析工具阻碍了对支原体毒力决定因素的功能和调控的阐明。我们在此描述了使用转座子载体将肺炎支原体中与细胞黏附相关的蛋白HMW1的克隆基因导入的方法。将编码HMW1除C末端外所有序列的4.95 kbp BamHI片段克隆到修饰的Tn4001中,并转化到野生型肺炎支原体以及缺乏HMW1 - HMW5的非黏附突变体中。Southern印迹杂交证实转座子的插入以及常驻和重组hmw1等位基因的存在。Western免疫印迹分析显示转化体中存在截短的HMW1(HMW1'),HMW1'的水平取决于hmw1基因在转座子中的方向和插入位点。在野生型和突变体背景中观察到类似的表达模式。然而,在突变体中野生型水平的HMW1'表达并未恢复黏附能力。最后,证明HMW4和HMW1是同一基因的产物,HMW4是HMW1的热修饰衍生物。

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