首页> 美国卫生研究院文献>Journal of Bacteriology >Role for Phosphoglucomutase in Vibrio fischeri-Euprymna scolopes Symbiosis
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Role for Phosphoglucomutase in Vibrio fischeri-Euprymna scolopes Symbiosis

机译:磷酸葡萄糖突变酶在费氏弧菌-Euprymna弧菌共生中的作用

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摘要

Vibrio fischeri, a luminescent marine bacterium, specifically colonizes the light organ of its symbiotic partner, the Hawaiian squid Euprymna scolopes. In a screen for V. fischeri colonization mutants, we identified a strain that exhibited on average a 10-fold decrease in colonization levels relative to that achieved by wild-type V. fischeri. Further characterization revealed that this defect did not result from reduced luminescence or motility, two processes required for normal colonization. We determined that the transposon in this mutant disrupted a gene with high sequence identity to the pgm (phosphoglucomutase) gene of Escherichia coli, which encodes an enzyme that functions in both galactose metabolism and the synthesis of UDP-glucose. The V. fischeri mutant grew poorly with galactose as a sole carbon source and was defective for phosphoglucomutase activity, suggesting functional identity between E. coli Pgm and the product of the V. fischeri gene, which was therefore designated pgm. In addition, lipopolysaccharide profiles of the mutant were distinct from that of the parent strain and the mutant exhibited increased sensitivity to various cationic agents and detergents. Chromosomal complementation with the wild-type pgm allele restored the colonization ability to the mutant and also complemented the other noted defects. Unlike the pgm mutant, a galactose-utilization mutant (galK) of V. fischeri colonized juvenile squid to wild-type levels, indicating that the symbiotic defect of the pgm mutant is not due to an inability to catabolize galactose. Thus, pgm represents a new gene required for promoting colonization of E. scolopes by V. fischeri.
机译:费氏弧菌(Vibrio fischeri)是一种发光的海洋细菌,专门定居于其共生伴侣夏威夷鱿鱼虾up(Euprymna scolopes)的光器官。在筛选费氏弧菌定殖突变体的过程中,我们鉴定出了相对于野生型费氏弧菌定殖水平平均降低10倍的菌株。进一步的特征表明,该缺陷不是由于正常定植所需的两个过程,即发光或运动减少所致。我们确定该突变体中的转座子破坏了与大肠杆菌pgm(磷酸葡萄糖变位酶)基因具有高度序列同一性的基因,该基因编码一种在半乳糖代谢和UDP-葡萄糖合成中均起作用的酶。以半乳糖为唯一碳源的费氏弧菌突变体生长较差,并且磷酸葡萄糖突变酶活性存在缺陷,表明大肠杆菌Pgm和费氏弧菌基因产物之间具有功能同一性,因此将其命名为pgm。另外,该突变体的脂多糖谱与亲本菌株的脂多糖谱不同,并且该突变体对各种阳离子试剂和去污剂表现出增加的敏感性。与野生型pgm等位基因的染色体互补恢复了突变体的定植能力,并且还补充了其他明显的缺陷。与pgm突变体不同,费氏弧菌的半乳糖利用突变体(galK)将少年鱿鱼定殖到野生型水平,这表明pgm突变体的共生缺陷不是由于无法分解代谢半乳糖。因此,pgm代表了促进 E定植的新基因。 V)。费舍里

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