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A genetic screen identifies genes and sites involved in pilin antigenic variation in Neisseria gonorrhoeae

机译:遗传筛选可鉴定淋病奈瑟菌中菌毛蛋白抗原变异的基因和位点

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It has previously been shown that the frequency of pilin antigenic variation in Neisseria gonorrhoeae (the gonococcus, Gc) is regulated by iron availability. To identify factors involved in pilin variation in an iron-dependent or an iron-independent manner, we conducted a genetic screen of transposon-mutated gonococci using a pilus-dependent colony morphology phenotype to detect antigenic variation deficient mutants. Forty-six total mutants representing insertions in 30 different genes were shown to have reduced colony morphology changes resulting from impaired pilin variation. Five mutants exhibited an iron-dependent decrease in pilin variation, while the remaining 41 displayed an iron-independent decrease in pilin variation. Based on the levels of antigenic variation impairment, we defined the genes as being essential for, important for, or involved in antigenic variation. DNA repair and DNA transformation frequencies of each mutant were measured to determine whether other recombination-based processes were also affected in the mutants. Each mutant was placed into one of six classes based on their pilin variation, DNA repair and DNA transformation phenotypes. Among the many genes identified, recR is shown to be an additional member of the gonococcal RecF-like recombination pathway. In addition, recG and ruvA represent the first evidence that the processing of Holliday junctions is required for pilin antigenic variation. Moreover, two independent insertions in a non-coding region upstream of the pilE gene suggest that cis-acting sequences important for pilin variation are found in that region. Finally, insertions that effect expression of the thrB and thrC genes suggest that molecules in the threonine biosynthetic pathway are important for pilin variation. Many of the other genes identified in this genetic screen do not have an obvious role in pilin variation, DNA repair, or DNA transformation.
机译:以前已经证明,淋病奈瑟氏球菌(淋球菌,Gc)中菌毛蛋白抗原变异的频率受铁的可用性调节。为了鉴定以铁依赖性或铁非依赖性方式参与菌毛蛋白变异的因素,我们使用菌毛依赖性菌落形态表型对转座子突变的淋球菌进行了遗传筛选,以检测缺乏抗原变异的突变体。代表在30种不同基因中插入的46个突变体显示出菌毛蛋白变异受损导致菌落形态变化减少。 5个突变体的铁蛋白变异性降低了铁依赖性,而其余的41个突变体的铁蛋白变异性降低了铁。基于抗原变异损害的水平,我们将基因定义为对抗原变异至关重要,对抗原变异重要或与抗原变异有关。测量每个突变体的DNA修复和DNA转化频率,以确定其他基于重组的过程在突变体中是否也受到影响。根据其菌毛素变异,DNA修复和DNA转化表型,将其分为六类之一。在鉴定出的许多基因中,recR被证明是淋球菌RecF样重组途径的另一个成员。此外,recG和ruvA代表了第一个证据,表明菌毛蛋白抗原变异需要加工Holliday连接。此外,在pilE基因上游非编码区的两个独立插入表明在该区域发现了对菌毛蛋白变异重要的顺式作用序列。最后,影响thrB和thrC基因表达的插入表明,苏氨酸生物合成途径中的分子对于菌毛蛋白变异很重要。在此基因筛选中鉴定出的许多其他基因在菌毛素变异,DNA修复或DNA转化中没有明显作用。

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