首页> 美国卫生研究院文献>Journal of Bacteriology >The capsule polysaccharide synthesis locus of streptococcus pneumoniae serotype 14: Identification of the glycosyl transferase gene cps14E.
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The capsule polysaccharide synthesis locus of streptococcus pneumoniae serotype 14: Identification of the glycosyl transferase gene cps14E.

机译:肺炎链球菌血清型14的胶囊多糖合成位点:糖基转移酶基因cps14E的鉴定。

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摘要

To identify a chromosomal region of Streptococcus pneumoniae serotype 14 involved in capsule polysaccharide synthesis, two strategies were used: (i) Tn916 mutagenesis, followed by the characterization of four unencapsulated mutants, and (ii) cross-hybridization with a capsule polysaccharide synthesis gene (cps) probe from S. agalactiae, which has a structurally similar capsule. The two approaches detected the same chromosomal region consisting of two adjacent EcoRI fragments. One of these EcoRI fragments was cloned and hybridized with a cosmid library. This resulted in clone cMKO2. A similar cosmid clone was obtained from an unencapsulated Tn916 mutant, Spnl4.H. Sequence analysis of the two cosmid clones revealed that in the Tn916 mutant, a gene, cps14E, which is homologous to other bacterial genes encoding glycosyl transferases, had been inactivated. An open reading frame immediately downstream of cps14E, designated cps14F, shows no significant homology with any known genes or proteins. A functional assay showed that cps14E encodes a glycosyl transferase and that a gene-specific knockout mutant lacks this enzyme activity, whereas inactivation of cps14F does not have this effect.
机译:为了鉴定参与胶囊多糖合成的肺炎链球菌血清型14的染色体区域,使用了两种策略:(i)Tn916诱变,然后表征四个未封装的突变体,以及(ii)与胶囊多糖合成基因交叉杂交(无乳链球菌的cps)探针,其结构相似。两种方法检测到由两个相邻的EcoRI片段组成的相同染色体区域。将这些EcoRI片段之一克隆并与粘粒文库杂交。这产生了克隆cMKO2。从未包囊的Tn916突变体Spn14.H获得相似的粘粒克隆。对两个粘粒克隆的序列分析表明,在Tn916突变体中,与编码糖基转移酶的其他细菌基因同源的cps14E基因已被灭活。紧邻cps14E下游的开放阅读框,称为cps14F,与任何已知的基因或蛋白质均无明显同源性。功能测定表明,cps14E编码糖基转移酶,而基因特异性敲除突变体缺乏这种酶活性,而cps14F的失活则没有这种作用。

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