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The regulatory genes involved in spiramycin and bitespiramycin biosynthesis

机译:参与Spiramycin和Bitespiramycin生物合成的调节基因

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Bitespiramycin (biotechnological spiramycin, Bsm) is a new 16-membered macrolide antibiotic produced by Streptomyces spiramyceticus WSJ-1 integrated exogenous genes. The gene cluster for Bsm biosynthesis consists of two parts: spiramycin biosynthetic gene cluster (92 kb) and two exogenous genes including 4 ''-O-isovaleryltransferase gene (ist) and a positive regulatory gene (acyB2) from S. thermotolerans. Four putative regulatory genes, bsm2, bsm23, bsm27 and bsm42, were identified by sequence analysis in the spiramycin gene cluster. The inactivation of bsm23 or bsm42 in S. spiramyceticus eliminated spiramycin production, while the deletion of bsm2 and bsm27 did not abolish spiramycin biosynthesis. The acyB2 gene, homologous with bsm42 gene, cannot recover the spiramycin production in Delta bsm42 mutant. The high expression of bsm42 significantly increased the spiramycin production, but overexpression of bsm23 inhibited its production in Delta bsm23 and wildtype strain. Bsm23 was shown to be involved in the regulation of the expression of bsm42 and acyB2 by electrophoretic mobility shift assays. The bsm42 gene was also positive regulator for ist expression inferred from the improved yield of 4 ''-isovalerylspiramycins in the S. lividans TK24 biotransformation test, but adding bsm23 decreased the production of 4 ''-isovalerylspiramycins. These results demonstrated Bsm42 was a pathway-specific activator for spiramycin or Bsm biosynthesis, but overexpression of Bsm23 alone was adverse to produce these antibiotics although Bsm23 was essential for positive regulation of spiramycin production.
机译:Bitespiramycin(生物技术螺霉素,BSM)是一种新的16元大环内酯抗生素,由Streptomyces血红蛋白WSJ-1集成外源基因产生。 BSM生物合成的基因簇由两部分组成:Spiramycin生物合成基因簇(92kb)和两个外源基因,包括4'-o-异戊烯酸直链流酶基因(IST)和来自S. Thermotolerans的阳性调节基因(ACYB2)。通过螺霉素基因簇中的序列分析鉴定了四个推定的调节基因,BSM2,BSM23,BSM47和BSM42。 BSM23或BSM42在S. Spiramyceticus的灭活消除了苯胺霉素生产,而BSM2和BSM27的缺失则没有消除螺霉素生物合成。 ACYB2基因与BSM42基因同源,不能在Delta BSM42突变体中回收螺霉素产生。 BSM42的高表达显着增加了螺霉素的产生,但BSM23的过表达抑制了ΔBSM23和野生型菌株的产量。 BSM23被证明通过电泳迁移率移位测定参与了BSM42和ACB2表达的调节。 BSM42基因也是IST表达的阳性调节剂,从S. Lividans TK24生物转化试验中的4'-Iisoperylspiramycins的提高产量推断出来,但添加BSM23降低了4''-Isovallylspiramycin的产生。这些结果证明了BSM42是螺霉素或BSM生物合成的途径特异性活化剂,但单独的BSM23的过度表达对于产生这些抗生素,尽管BSM23对于对鞘霉素产生的正规调节至关重要。

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