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首页> 外文期刊>Applied and Environmental Microbiology >Metabolism of Benzoate, Cyclohex-1-ene Carboxylate, and Cyclohexane Carboxylate by “Syntrophus aciditrophicus” Strain SB in Syntrophic Association with H2-Using Microorganisms
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Metabolism of Benzoate, Cyclohex-1-ene Carboxylate, and Cyclohexane Carboxylate by “Syntrophus aciditrophicus” Strain SB in Syntrophic Association with H2-Using Microorganisms

机译:“ Syntrophus aciditrophicus”菌株SB在与H2-利用微生物的养分结合中代谢苯甲酸酯,环己-1-烯羧酸盐和环己烷羧酸盐

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摘要

The metabolism of benzoate, cyclohex-1-ene carboxylate, and cyclohexane carboxylate by “Syntrophus aciditrophicus” in cocultures with hydrogen-using microorganisms was studied. Cyclohexane carboxylate, cyclohex-1-ene carboxylate, pimelate, and glutarate (or their coenzyme A [CoA] derivatives) transiently accumulated during growth with benzoate. Identification was based on comparison of retention times and mass spectra of trimethylsilyl derivatives to the retention times and mass spectra of authentic chemical standards. 13C nuclear magnetic resonance spectroscopy confirmed that cyclohexane carboxylate and cyclohex-1-ene carboxylate were produced from [ring-13C6]benzoate. None of the metabolites mentioned above was detected in non-substrate-amended or heat-killed controls. Cyclohexane carboxylic acid accumulated to a concentration of 260 μM, accounting for about 18% of the initial benzoate added. This compound was not detected in culture extracts ofRhodopseudomonas palustris grown phototrophically orThauera aromatica grown under nitrate-reducing conditions. Cocultures of “S. aciditrophicus” andMethanospirillum hungatei readily metabolized cyclohexane carboxylate and cyclohex-1-ene carboxylate at a rate slightly faster than the rate of benzoate metabolism. In addition to cyclohexane carboxylate, pimelate, and glutarate, 2-hydroxycyclohexane carboxylate was detected in trace amounts in cocultures grown with cyclohex-1-ene carboxylate. Cyclohex-1-ene carboxylate, pimelate, and glutarate were detected in cocultures grown with cyclohexane carboxylate at levels similar to those found in benzoate-grown cocultures. Cell extracts of “S. aciditrophicus” grown in a coculture withDesulfovibrio sp. strain G11 with benzoate or in a pure culture with crotonate contained the following enzyme activities: an ATP-dependent benzoyl-CoA ligase, cyclohex-1-ene carboxyl-CoA hydratase, and 2-hydroxycyclohexane carboxyl-CoA dehydrogenase, as well as pimelyl-CoA dehydrogenase, glutaryl-CoA dehydrogenase, and the enzymes required for conversion of crotonyl-CoA to acetate. 2-Ketocyclohexane carboxyl-CoA hydrolase activity was detected in cell extracts of “S. aciditrophicus”-Desulfovibrio sp. strain G11 benzoate-grown cocultures but not in crotonate-grown pure cultures of “S. aciditrophicus”. These results are consistent with the hypothesis that ring reduction during syntrophic benzoate metabolism involves a four- or six-electron reduction step and that once cyclohex-1-ene carboxyl-CoA is made, it is metabolized in a manner similar to that in R. palustris.
机译:研究了“ ”与含氢微生物共培养时苯甲酸,环己-1-烯羧酸盐和环己烷羧酸盐的代谢。环己烷羧酸酯,环己-1-烯羧酸酯,庚二酸酯和戊二酸酯(或其辅酶A [CoA]衍生物)在苯甲酸酯生长过程中瞬时积累。鉴定是基于三甲基甲硅烷基衍生物的保留时间和质谱与真实化学标准品的保留时间和质谱进行比较。 13 C核磁共振波谱证实,环己烷羧酸盐和环己-1-烯羧酸盐是由[ ring - 13 C 6产生的]苯甲酸酯。在未修饰底物或加热杀死的对照中均未检测到上述代谢物。环己烷甲酸累积到260μM的浓度,约占最初添加的苯甲酸酯的18%。在硝酸还原条件下生长的 Rhodopseudomonas palustris 的培养提取物或 Thauera aromaa 的培养提取物中未检测到该化合物。 “ S”的共培养。嗜酸性营养菌”和“饥饿感甲基螺菌”的代谢速率比苯甲酸酯代谢速率快一些。除环己烷羧酸酯,庚二酸酯和戊二酸酯外,在与环己-1-烯羧酸酯一起培养的共培养物中还检测到了痕量的2-羟基环己烷羧酸酯。在与环己烷羧酸盐共培养的共培养物中,检测到环己-1-烯羧酸盐,庚二酸酯和谷氨酸盐的水平与在苯甲酸盐种植的共培养物中发现的水平相似。 “ S”的细胞提取物。与 Desulfovibrio sp共培养的嗜酸性营养菌”。带有苯甲酸酯或在巴豆酸酯的纯培养物中的G11菌株含有以下酶活性:ATP依赖的苯甲酰CoA连接酶,环己-1-烯羧基CoA水合酶和2-羟基环己烷羧基CoA脱氢酶,以及pimelyl- CoA脱氢酶,戊二酰-CoA脱氢酶,以及将巴豆酰-CoA转化为乙酸盐所需的酶。在“ em” S的细胞提取物中检测到2-酮环己烷羧基-CoA水解酶活性。嗜酸性营养菌”-脱硫弧菌 sp.。菌株G11苯甲酸盐种植的共培养物,而不是巴豆酸盐生长的纯培养物“ S”。嗜酸菌”。这些结果与以下假设相吻合:在同养型苯甲酸代谢过程中,环的还原涉及四或六电子的还原步骤,并且一旦制成环己-1-烯羧基-CoA,其代谢方式类似于 > R。 palustris

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