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明亮突变型发光弧菌 ES114 揭示了控制生物发光和 lux 操纵子表达的条件和调控因子。

Bright mutants of Vibrio fischeri ES114 reveal conditions and regulators that control bioluminescence and expression of the lux operon.

机构信息

Department of Microbiology, University of Georgia, 1000 Cedar Street, Athens, GA 30602, USA.

出版信息

J Bacteriol. 2010 Oct;192(19):5103-14. doi: 10.1128/JB.00524-10. Epub 2010 Aug 6.

Abstract

Vibrio fischeri ES114, an isolate from the Euprymna scolopes light organ, produces little bioluminescence in culture but is ∼1,000-fold brighter when colonizing the host. Cell-density-dependent regulation alone cannot explain this phenomenon, because cells within colonies on solid medium are much dimmer than symbiotic cells despite their similar cell densities. To better understand this low luminescence in culture, we screened ∼20,000 mini-Tn5 mutants of ES114 for increased luminescence and identified 28 independent "luminescence-up" mutants with insertions in 14 loci. Mutations affecting the Pst phosphate uptake system led to the discovery that luminescence is upregulated under low-phosphate conditions by PhoB, and we also found that ainS, which encodes an autoinducer synthase, mediates repression of luminescence during growth on plates. Other novel luminescence-up mutants had insertions in acnB, topA, tfoY, phoQ, guaB, and two specific tRNA genes. Two loci, hns and lonA, were previously described as repressors of bioluminescence in transgenic Escherichia coli carrying the light-generating lux genes, and mutations in arcA and arcB were consistent with our report that Arc represses lux. Our results reveal a complex regulatory web governing luminescence and show how certain environmental conditions are integrated into regulation of the pheromone-dependent lux system.

摘要

发光弧菌 ES114 是从萤光章鱼发光器官中分离出来的一种菌株,在培养中产生的生物发光量很少,但在定植宿主时的发光强度却提高了约 1000 倍。仅靠细胞密度依赖性调控无法解释这一现象,因为尽管固体培养基上的菌落中的细胞密度与共生细胞相似,但它们的发光强度却要暗得多。为了更好地理解这种在培养中的低发光现象,我们对 ES114 的约 20000 个 mini-Tn5 突变体进行了筛选,以寻找发光增强的突变体,并在 14 个基因座中鉴定出了 28 个独立的“发光增强”突变体。影响 Pst 磷酸摄取系统的突变导致发现 PhoB 在低磷条件下上调发光,我们还发现 ainS 编码一种自动诱导物合成酶,在平板生长过程中介导对发光的抑制。其他新的发光增强突变体在 acnB、topA、tfoY、phoQ、guaB 和两个特定的 tRNA 基因中有插入。两个基因座 hns 和 lonA 先前被描述为携带发光基因的转 E. coli 中生物发光的抑制剂,而 arcA 和 arcB 的突变与我们的报告一致,即 Arc 抑制 lux。我们的结果揭示了一个复杂的调控网络,用于调控发光,展示了如何将某些环境条件整合到对依赖于信息素的 lux 系统的调控中。

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