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鱿鱼发光器官共生菌费氏弧菌游泳运动能力的遗传决定因素。

Genetic determinants of swimming motility in the squid light-organ symbiont Vibrio fischeri.

机构信息

Department of Medical Microbiology and Immunology, University of Wisconsin, Madison, Wisconsin.

出版信息

Microbiologyopen. 2013 Aug;2(4):576-94. doi: 10.1002/mbo3.96. Epub 2013 Jun 12.

Abstract

Bacterial flagellar motility is a complex cellular behavior required for the colonization of the light-emitting organ of the Hawaiian bobtail squid, Euprymna scolopes, by the beneficial bioluminescent symbiont Vibrio fischeri. We characterized the basis of this behavior by performing (i) a forward genetic screen to identify mutants defective in soft-agar motility, as well as (ii) a transcriptional analysis to determine the genes that are expressed downstream of the flagellar master regulator FlrA. Mutants with severe defects in soft-agar motility were identified due to insertions in genes with putative roles in flagellar motility and in genes that were unexpected, including those predicted to encode hypothetical proteins and cell division-related proteins. Analysis of mutants for their ability to enter into a productive symbiosis indicated that flagellar motility mutants are deficient, while chemotaxis mutants are able to colonize a subset of juvenile squid to light-producing levels. Thirty-three genes required for normal motility in soft agar were also downregulated in the absence of FlrA, suggesting they belong to the flagellar regulon of V. fischeri. Mutagenesis of putative paralogs of the flagellar motility genes motA, motB, and fliL revealed that motA1, motB1, and both fliL1 and fliL2, but not motA2 and motB2, likely contribute to soft-agar motility. Using these complementary approaches, we have characterized the genetic basis of flagellar motility in V. fischeri and furthered our understanding of the roles of flagellar motility and chemotaxis in colonization of the juvenile squid, including identifying 11 novel mutants unable to enter into a productive light-organ symbiosis.

摘要

细菌鞭毛运动是夏威夷短尾乌贼(Euprymna scolopes)发光器官被发光共生体费氏弧菌(Vibrio fischeri)定植所必需的复杂细胞行为。我们通过(i)正向遗传筛选来鉴定在软琼脂运动中缺陷的突变体,以及(ii)转录分析来确定在鞭毛主调控因子 FlrA 下游表达的基因,从而描述了这种行为的基础。由于在可能参与鞭毛运动的基因和意想不到的基因(包括预测编码假定蛋白和细胞分裂相关蛋白的基因)中插入,因此鉴定出在软琼脂运动中存在严重缺陷的突变体。对进入产生活性共生的突变体进行分析表明,鞭毛运动突变体存在缺陷,而趋化运动突变体能够定植部分幼乌贼达到发光水平。在没有 FlrA 的情况下,33 个在软琼脂中正常运动所需的基因也被下调,这表明它们属于费氏弧菌的鞭毛调控基因。对假定的鞭毛运动基因 motA、motB 和 fliL 的旁系同源基因进行诱变,发现 motA1、motB1 和 fliL1 和 fliL2(而非 motA2 和 motB2)可能有助于软琼脂运动。使用这些互补方法,我们描述了费氏弧菌鞭毛运动的遗传基础,并进一步了解了鞭毛运动和趋化性在幼乌贼定植中的作用,包括鉴定出 11 个无法进入产生活性器官共生的新突变体。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/d7ee/3948606/ee159b531633/mbo30002-0576-f1.jpg

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