首页> 美国卫生研究院文献>Journal of Bacteriology >CcaR Is an Autoregulatory Protein That Binds to the ccaR and cefD-cmcI Promoters of the Cephamycin C-Clavulanic Acid Cluster in Streptomyces clavuligerus
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CcaR Is an Autoregulatory Protein That Binds to the ccaR and cefD-cmcI Promoters of the Cephamycin C-Clavulanic Acid Cluster in Streptomyces clavuligerus

机译:CcaR是与链霉菌克拉维链霉菌中头霉素C-克拉维酸簇的ccaR和cefD-cmcI启动子结合的自调节蛋白

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摘要

The putative regulatory CcaR protein, which is encoded in the β-lactam supercluster of Streptomyces clavuligerus, has been partially purified by ammonium sulfate precipitation and heparin affinity chromatography. In addition, it was expressed in Escherichia coli, purified as a His-tagged recombinant protein (rCcaR), and used to raise anti-rCcaR antibodies. The partially purified CcaR protein from S. clavuligerus was able to bind DNA fragments containing the promoter regions of the ccaR gene itself and the bidirectional cefD-cmcI promoter region. In contrast, CcaR did not bind to DNA fragments with the promoter regions of other genes of the cephamycin-clavulanic acid supercluster including lat, blp, claR, car-cyp, and the unlinked argR gene. The DNA shifts obtained with CcaR were prevented by anti-rCcaR immunoglobulin G (IgG) antibodies but not by anti-rabbit IgG antibodies. ccaR and the bidirectional cefD-cmcI promoter region were fused to the xylE reporter gene and expressed in Streptomyces lividans and S. clavuligerus. These constructs produced low catechol dioxygenase activity in the absence of CcaR; activity was increased 1.7- to 4.6-fold in cultures expressing CcaR. Amplification of the ccaR promoter region lacking its coding sequence in a high-copy-number plasmid in S. clavuligerus ATCC 27064 resulted in a reduced production of cephamycin C and clavulanic acid, by 12 to 20% and 40 to 60%, respectively, due to titration of the CcaR regulator. These findings confirm that CcaR is a positively acting autoregulatory protein able to bind to its own promoter as well as to the cefD-cmcI bidirectional promoter region.
机译:假定的调节性CcaR蛋白,在棒状链霉菌的β-内酰胺超簇中编码,已通过硫酸铵沉淀和肝素亲和色谱法部分纯化。此外,它在大肠杆菌中表达,纯化为带有His标记的重组蛋白(rCcaR),并用于产生抗rCcaR抗体。来自棒状链霉菌的部分纯化的CcaR蛋白能够结合含有ccaR基因本身的启动子区域和双向cefD-cmcI启动子区域的DNA片段。相反,CcaR不与具有头孢霉素-克拉维酸超簇的其他基因的启动子区域结合的DNA片段,包括lat,blp,claR,car-cyp和未连接的argR基因。用抗rCcaR免疫球蛋白G(IgG)抗体可防止CcaR获得的DNA转移,但可通过抗兔IgG抗体防止。 ccaR和双向cefD-cmcI启动子区域融合到xylE报告基因,并在链霉菌青紫链霉菌和克拉维链霉菌中表达。在没有CcaR的情况下,这些构建体产生了较低的儿茶酚双加氧酶活性。在表达CcaR的培养物中,活性增加了1.7倍至4.6倍。在 S中的高拷贝数质粒中,缺少其编码序列的ccaR启动子区域的扩增。由于滴定了CcaR调节剂,棒状杆菌ATCC 27064导致头孢霉素C和棒酸的产量分别降低了12%至20%和40%至60%。这些发现证实CcaR是一种正向作用的自调节蛋白,能够与其自身的启动子以及 cefD-cmcI 双向启动子区域结合。

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