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一个高度保守的苜蓿中华根瘤菌操纵子在微需氧条件下通过FixLJ系统被诱导,并且通过NnrR被一氧化氮(NO)诱导。

A highly conserved Sinorhizobium meliloti operon is induced microaerobically via the FixLJ system and by nitric oxide (NO) via NnrR.

作者信息

de Bruijn Frans J, Rossbach Silvia, Bruand Claude, Parrish Jodi R

机构信息

Laboratoire des Interactions Plantes Micro-organismes (LIPM), UMR CNRS 2594/INRA 441, BP 52627, 31326 Castanet-Tolosan Cedex, France.

出版信息

Environ Microbiol. 2006 Aug;8(8):1371-81. doi: 10.1111/j.1462-2920.2006.01030.x.

Abstract

A previously generated collection of 11 Tn5-luxAB insertion mutants of Sinorhizobium meliloti harbouring lux reporter gene fusions induced under microaerobic (1% O2) conditions was further characterized and mapped on the sequenced S. meliloti genome. One highly induced gene fusion from this collection (loe-7) was found to be located in the intergenic region between sma1292, encoding a putative protease/collagenase, and a gene of unknown function (sma1294). The loe-7 fusion had been shown previously to be partially controlled by the oxygen sensor/regulator FixLJ system, but significant ( approximately 40%) Lux activity remained in a fixLJ mutant background. Therefore, a secondary Tn1721 mutagenesis of the loe-7 strain was carried out. Nine Tn1721 ('dark') insertions completely abolishing the Lux activity of the loe-7 fusion under microaerobic conditions were isolated. Surprisingly, five dark insertions mapped in denitrification genes [napA, napC, nirK--two insertions--and sma1245 encoding a NnrR-like transcriptional regulator controlling denitrification in response to nitric oxide (NO)]; Tn1721 insertions in the respiration genes fixG and fixP resulted in a reduced expression of the loe-7-lux fusion, and insertions in the regulatory genes fixJ and fixK1 resulted in low, but still detectable Lux activity. On the contrary, insertions in the norD or norQ genes resulted in constitutive Lux activity. In these mutant strains, NO would be expected to accumulate under microaerobic conditions. NO was found to be able to strongly induce the loe-7-luxAB fusion under microaerobic and aerobic conditions, but only in the presence of the functional nnrR-like gene (sma1245). These results suggest that NO, via the NnrR regulator, can serve as a signal molecule to induce the loe-7-luxAB fusion in concert with the FixLJ system.

摘要

之前构建了一批11个苜蓿中华根瘤菌(Sinorhizobium meliloti)的Tn5-luxAB插入突变体,这些突变体带有在微氧(1% O₂)条件下诱导的lux报告基因融合体,对其进行了进一步表征,并定位到已测序的苜蓿中华根瘤菌基因组上。发现该集合中的一个高度诱导的基因融合体(loe-7)位于sma1292(编码一种假定的蛋白酶/胶原酶)和一个功能未知的基因(sma1294)之间的基因间隔区。loe-7融合体先前已被证明部分受氧传感器/调节系统FixLJ控制,但在fixLJ突变体背景中仍保留显著(约40%)的Lux活性。因此,对loe-7菌株进行了二次Tn1721诱变。分离出9个在微氧条件下完全消除loe-7融合体Lux活性的Tn1721(“暗”)插入突变体。令人惊讶的是,5个暗插入突变体位于反硝化基因中[napA、napC、nirK(两个插入突变体)以及编码响应一氧化氮(NO)控制反硝化作用的类NnrR转录调节因子的sma1245];呼吸基因fixG和fixP中的Tn1721插入导致loe-7-lux融合体表达降低,调节基因fixJ和fixK1中的插入导致低水平但仍可检测到的Lux活性。相反,norD或norQ基因中的插入导致组成型Lux活性。在这些突变菌株中,预计在微氧条件下NO会积累。发现NO能够在微氧和好氧条件下强烈诱导loe-7-luxAB融合体,但仅在存在功能性类nnrR基因(sma1245)的情况下。这些结果表明,NO通过NnrR调节因子,可以作为一种信号分子,与FixLJ系统协同诱导loe-7-luxAB融合体。

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