耻垢分枝杆菌中cydAB编码的细胞色素bd氧化酶的特性分析。
Characterization of the cydAB-encoded cytochrome bd oxidase from Mycobacterium smegmatis.
作者信息
Kana B D, Weinstein E A, Avarbock D, Dawes S S, Rubin H, Mizrahi V
机构信息
MRC/SAIMR/WITS Molecular Mycobacteriology Research Unit, South African Institute for Medical Research, Johannesburg, South Africa.
出版信息
J Bacteriol. 2001 Dec;183(24):7076-86. doi: 10.1128/JB.183.24.7076-7086.2001.
The cydAB genes from Mycobacterium smegmatis have been cloned and characterized. The cydA and cydB genes encode the two subunits of a cytochrome bd oxidase belonging to the widely distributed family of quinol oxidases found in prokaryotes. The cydD and cydC genes located immediately downstream of cydB encode a putative ATP-binding cassette-type transporter. At room temperature, reduced minus oxidized difference spectra of membranes purified from wild-type M. smegmatis displayed spectral features that are characteristic of the gamma-proteobacterial type cytochrome bd oxidase. Inactivation of cydA or cydB by insertion of a kanamycin resistance marker resulted in loss of d-heme absorbance at 631 nm. The d-heme could be restored by transformation of the M. smegmatis cyd mutants with a replicating plasmid carrying the highly homologous cydABDC gene cluster from Mycobacterium tuberculosis. Inactivation of cydA had no effect on the ability of M. smegmatis to exit from stationary phase at 37 or 42 degrees C. The growth rate of the cydA mutant was tested under oxystatic conditions. Although no discernible growth defect was observed under moderately aerobic conditions (9.2 to 37.5 x 10(2) Pa of pO(2) or 5 to 21% air saturation), the mutant displayed a significant growth disadvantage when cocultured with the wild type under extreme microaerophilia (0.8 to 1.7 x 10(2) Pa of pO(2) or 0.5 to 1% air saturation). These observations were in accordance with the two- to threefold increase in cydAB gene expression observed upon reduction of the pO(2) of the growth medium from 21 to 0.5% air saturation and with the concomitant increase in d-heme absorbance in spectra of membranes isolated from wild-type M. smegmatis cultured at 1% air saturation. Finally, the cydA mutant displayed a competitive growth disadvantage in the presence of the terminal oxidase inhibitor, cyanide, when cocultured with wild type at 21% air saturation in an oxystat. In conjunction with these findings, our results suggest that cytochrome bd is an important terminal oxidase in M. smegmatis.
耻垢分枝杆菌的cydAB基因已被克隆并进行了特性分析。cydA和cydB基因编码细胞色素bd氧化酶的两个亚基,该氧化酶属于原核生物中广泛分布的喹啉氧化酶家族。紧邻cydB下游的cydD和cydC基因编码一种假定的ATP结合盒式转运蛋白。在室温下,从野生型耻垢分枝杆菌纯化的膜的还原减去氧化差光谱显示出γ-变形菌属型细胞色素bd氧化酶的特征光谱特征。通过插入卡那霉素抗性标记使cydA或cydB失活导致631 nm处d-血红素吸光度丧失。通过用携带来自结核分枝杆菌的高度同源的cydABDC基因簇的复制质粒转化耻垢分枝杆菌cyd突变体,可以恢复d-血红素。cydA失活对耻垢分枝杆菌在37或42℃下从稳定期退出的能力没有影响。在恒氧条件下测试了cydA突变体的生长速率。虽然在中度需氧条件下(pO₂为9.2至37.5×10² Pa或空气饱和度为5至21%)未观察到明显的生长缺陷,但当在极端微需氧条件下(pO₂为0.8至1.7×10² Pa或空气饱和度为0.5至1%)与野生型共培养时,该突变体表现出显著的生长劣势。这些观察结果与在生长培养基中pO₂从21%降低到0.5%空气饱和度时观察到的cydAB基因表达增加两到三倍以及在1%空气饱和度下培养的野生型耻垢分枝杆菌分离的膜光谱中d-血红素吸光度的相应增加一致。最后,当在恒氧仪中于21%空气饱和度下与野生型共培养时,cydA突变体在存在末端氧化酶抑制剂氰化物的情况下表现出竞争性生长劣势。结合这些发现,我们的结果表明细胞色素bd是耻垢分枝杆菌中的一种重要末端氧化酶。
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