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GlnR-mediated regulation of nitrogen metabolism in the actinomycete Saccharopolyspora erythraea

机译:GlnR介导的放线菌性红多孢菌中氮代谢的调节

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Nitrogen source sensing, uptake, and assimilation are central for growth and development of microorganisms which requires the participation of a global control of nitrogen metabolism-associated genes at the transcriptional level. In soil-dwelling antibiotic-producing actinomycetes, this role is played by GlnR, an OmpR family regulator. In this work, we demonstrate that SACE_7101 is the ortholog of actinomycetes’ GlnR global regulators in the erythromycin producer Saccharopolyspora erythraea. Indeed, the chromosomal deletion of SACE_7101 severely affects the viability of S. erythraea when inoculated in minimal media supplemented with NaNO_3, NaNO_2, NH_4Cl, glutamine, or glutamate as sole nitrogen source. Combination of in silico prediction of cisacting elements, subsequent in vitro (through gel shift assays) and in vivo (real-time reverse transcription polymerase chain reaction) validations of the predicted target genes revealed a very large GlnR regulon aimed at adapting the nitrogen metabolism of S. erythraea. Indeed, enzymes/proteins involved in (i) uptake and assimilation of ammonium, (ii) transport and utilization of urea, (iii) nitriteitrate, (iv) glutamate/ glutamine, (v) arginine metabolism, (vi) nitric oxide biosynthesis, and (vii) signal transduction associated with the nitrogen source supplied have at least one paralog gene which expression is controlled by GlnR. Our work highlights a GlnR-binding site consensus sequence (t/gna/cAC-n6-GaAAc) which is similar although not identical to the consensus sequences proposed for other actinomycetes. Finally, we discuss the distinct and common features of the GlnRmediated transcriptional control of nitrogen metabolism between S. erythraea and the model organism Streptomyces coelicolor.
机译:氮源的感测,吸收和吸收对于微生物的生长和发育至关重要,而微生物的生长和发育则需要在转录水平上全面控制与氮代谢相关的基因。在居住在土壤中的抗生素生产放线菌中,该作用由OmpR家族调节物GlnR发挥。在这项工作中,我们证明SACE_7101是红霉素生产商Saccharopolyspora erythraea中放线菌的GlnR全球调节基因的直系同源物。实际上,当在补充有NaNO_3,NaNO_2,NH_4Cl,谷氨酰胺或谷氨酸作为唯一氮源的基本培养基中接种时,SACE_7101的染色体缺失会严重影响红斑链球菌的生存能力。结合计算机模拟预测作用分子,随后在体外(通过凝胶位移分析)和体内(实时逆转录聚合酶链反应)对预测靶基因的验证表明,GlnR调节子非常大,旨在适应氮代谢。红霉菌。实际上,涉及(i)铵的吸收和吸收,(ii)尿素的运输和利用,(iii)亚硝酸盐/硝酸盐,(iv)谷氨酸/谷氨酰胺,(v)精氨酸代谢,(vi)一氧化氮的酶/蛋白质与提供的氮源相关的生物合成和(vii)信号转导具有至少一个旁系同源基因,其表达受GlnR控制。我们的工作着重介绍了一个GlnR结合位点共有序列(t / gna / cAC-n6-GaAAc),尽管与其他放线菌的共有序列不同,但该序列相似。最后,我们讨论了GlnR介导的红细菌和模型有机体链霉菌链霉菌氮代谢的转录控制的独特和共同特征。

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