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首页> 外文期刊>Journal of general plant pathology >Essential regulator gene toxR for toxoflavin biosynthesis of Burkholderia glumae
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Essential regulator gene toxR for toxoflavin biosynthesis of Burkholderia glumae

机译:毛泽东氏菌毒素生物合成的必需调节剂基因TOXR

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Burkholderia glumae (synonym: Pseudomonas glumae) is the causal agent of rice grain rot and seedling rot. This bacterium produces toxoflavin as a virulence factor for disease elicitation. Toxoflavin biosynthesis is completed by the transfer of methyl groups with catalytic action of a methyltransferase that is encoded by the toxA gene. In this study, we identified a 900-bp nucleotide sequence as a candidate gene to regulate the toxA gene. It was located upstream of the toxA gene. This novel regulatory element was named the toxR gene. When the toxR gene of B. glumae was disrupted by homologous recombination, one mutant (MY411) lost the ability to produce toxoflavin and to elicit the disease in rice seedlings. In addition, the expression of toxA mRNA was not detected by the reverse transcription-polymerase chain reaction, suggesting that the toxR gene is responsible for transcription of the toxA gene. The amino acid sequence deduced from the toxR gene was highly homologous to the LysR family transcriptional activators in some prokaryotes. Its amino-terminal had a helix-turn-helix DNA-binding motif to bind to a T-N_(11)-A sequence motif of the toxA promoter. These results indicated that the toxR gene encoded the activator protein to promote transcription of the toxA gene and conceivably of downstream toxoflavin biosynthesis genes.
机译:Burkholderia glumae(同义词:pseudomonas glumae)是水稻腐烂和幼苗腐烂的因果因子。该细菌产生毒素作为疾病引发的毒力因素。通过将甲基转移与由TOXA基因编码的甲基转移酶的催化作用转移完成的致辛酰胺生物合成。在该研究中,我们将900-BP核苷酸序列鉴定为候选基因以调节TOXA基因。它位于Toxa基因的上游。这种新型调节因素被命名为TOXR基因。当B.Glumae的ToxR基因被同源重组破坏时,一个突变体(My411)失去了生产毒素的能力并引发水稻幼苗中的疾病。另外,逆转录聚合酶链反应未检测到TOXA mRNA的表达,表明TOXR基因负责转录TOXA基因。从TOXR基因推导的氨基酸序列与一些原核生物中的Lysr家族转录活化剂高度同源。其氨基末端具有螺旋转螺旋DNA结合基序,结合TOXA启动子的T-N_(11)-A序列基序。这些结果表明,TOXR基因编码了活化剂蛋白以促进TOXA基因的转录,并可以想到下游毒物生物合成基因。

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