Petricoin E F, Danaher R J, Stein D C
Department of Microbiology, University of Maryland, College Park 20742.
J Bacteriol. 1991 Dec;173(24):7896-902. doi: 10.1128/jb.173.24.7896-7902.1991.
The genetic locus (lsi-1) responsible for the transformation of the lipooligosaccharide (LOS)-defective Neisseria gonorrhoeae mutant FA5100 to LOS expression was studied by deletion mutagenesis and sequence analysis. An open reading frame that was preceded by a leader sequence containing regions with the potential to form hairpin loops was identified. A perfect sigma 70 promoter consensus sequence was found upstream from this open reading frame. Promoter function was screened for functionality by using lac fusion cassettes and in vitro transcription-translation analysis. A frameshift mutation in the lsi-1 gene was constructed by site-directed mutagenesis and introduced into the chromosome of FA19, the LOS-expressing isogenic parent strain of FA5100. The mutant was characterized by Southern blotting, sodium dodecyl sulfate-polyacrylamide gel electrophoresis, and Western blotting (immunoblotting) and found to be phenotypically identical to FA5100.
通过缺失诱变和序列分析,研究了负责将脂寡糖(LOS)缺陷型淋病奈瑟菌突变体FA5100转化为LOS表达的基因座(lsi-1)。鉴定出一个开放阅读框,其前面的前导序列包含有可能形成发夹环的区域。在该开放阅读框上游发现了一个完美的σ70启动子共有序列。通过使用lac融合盒和体外转录-翻译分析筛选启动子功能的功能性。通过定点诱变构建lsi-1基因中的移码突变,并将其引入FA19的染色体中,FA19是FA5100的表达LOS的同基因亲本菌株。通过Southern印迹、十二烷基硫酸钠-聚丙烯酰胺凝胶电泳和Western印迹(免疫印迹)对该突变体进行表征,发现其表型与FA5100相同。
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