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幽门螺杆菌两个亚克隆之间的遗传差异与适应性比较。

Comparison of genetic divergence and fitness between two subclones of Helicobacter pylori.

作者信息

Björkholm B, Lundin A, Sillén A, Guillemin K, Salama N, Rubio C, Gordon J I, Falk P, Engstrand L

机构信息

Swedish Institute for Infectious Disease Control, 171 82 Solna, Karolinska Institute, 171 77 Stockholm, Sweden.

出版信息

Infect Immun. 2001 Dec;69(12):7832-8. doi: 10.1128/IAI.69.12.7832-7838.2001.

Abstract

Helicobacter pylori has a very plastic genome, reflecting its high rate of recombination and point mutation. This plasticity promotes divergence of the population by the development of subclones and presumably enhances adaptation to host niches. We have investigated the genotypic and phenotypic characteristics of two such subclones isolated from one patient as well as the genetic evolution of these isolates during experimental infection. Whole-genome genotyping of the isolates using DNA microarrays revealed that they were more similar to each other than to a panel of other genotyped strains recovered from different hosts. Nonetheless, they still showed significant differences. For example, one isolate (67:21) contained the entire Cag pathogenicity island (PAI), whereas the other (67:20) had excised the PAI. Phenotypic studies disclosed that both isolates expressed adhesins that recognized human histo-blood group Lewis(b) glycan receptors produced by gastric pit and surface mucus cells. In addition, both isolates were able to colonize, to equivalent density and with similar efficiency, germ-free transgenic mice genetically engineered to synthesize Lewis(b) glycans in their pit cells (12 to 14 mice/isolate). Remarkably, the Cag PAI-negative isolate was unable to colonize conventionally raised Lewis(b) transgenic mice harboring a normal gastric microflora, whereas the Cag PAI-positive isolate colonized 74% of the animals (39 to 40 mice/isolate). The genomic evolution of both isolates during the infection of conventionally raised and germ-free mice was monitored over the course of 3 months. The Cag PAI-positive isolate was also surveyed after a 10 month colonization of conventionally raised transgenic animals (n = 9 mice). Microarray analysis of the Cag PAI and sequence analysis of the cagA, recA, and 16S rRNA genes disclosed no changes in recovered isolates. Together, these results reveal that the H. pylori population infecting one individual can undergo significant divergence, creating stable subclones with substantial genotypic and phenotypic differences.

摘要

幽门螺杆菌具有高度可塑性的基因组,这反映了其高重组率和点突变率。这种可塑性通过亚克隆的形成促进了菌群的分化,并可能增强了对宿主生态位的适应性。我们研究了从一名患者分离出的两个此类亚克隆的基因型和表型特征,以及这些分离株在实验性感染期间的基因进化。使用DNA微阵列对分离株进行全基因组基因分型显示,它们彼此之间的相似性高于从不同宿主中回收的一组其他基因分型菌株。尽管如此,它们仍表现出显著差异。例如,一个分离株(67:21)包含完整的细胞毒素相关基因致病岛(Cag PAI),而另一个(67:20)则切除了该致病岛。表型研究表明,两个分离株均表达黏附素,这些黏附素可识别胃小凹和表面黏液细胞产生的人组织血型Lewis(b)聚糖受体。此外,两个分离株都能够在经过基因工程改造以在其小凹细胞中合成Lewis(b)聚糖的无菌转基因小鼠中定殖,定殖密度相当且效率相似(每个分离株12至14只小鼠)。值得注意的是,Cag PAI阴性分离株无法在具有正常胃微生物群的常规饲养的Lewis(b)转基因小鼠中定殖,而Cag PAI阳性分离株在74%的动物中定殖(每个分离株39至40只小鼠)。在3个月的时间里监测了两个分离株在常规饲养和无菌小鼠感染过程中的基因组进化。在对常规饲养的转基因动物进行10个月的定殖后(n = 9只小鼠),也对Cag PAI阳性分离株进行了调查。对Cag PAI的微阵列分析以及对cagA、recA和16S rRNA基因的序列分析表明,回收的分离株没有变化。总之,这些结果表明,感染一个个体的幽门螺杆菌菌群可发生显著分化,产生具有大量基因型和表型差异的稳定亚克隆。

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