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Metabolic Pathways Leading to Mercury Methylation in Desulfovibrio desulfuricans LS

机译:导致Desulfovibrio desulfuricans LS中甲基化的代谢途径

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The synthesis of methylmercury by Desulfovibrio desulfuricans LS was investigated on the basis of 14C incorporation from precursors and the measurement of relevant enzyme activities in cell extracts. The previously observed incorporation of C-3 from serine into methylmercury was confirmed by measurement of relatively high activities of serine hydroxymethyltransferase and other enzymes of this pathway. High rates of label incorporation into methylmercury from H14COO- and H14CO3- prompted the assay of enzymes of the acetyl coenzyme A (CoA) synthase pathway. These enzymes were found to be present but at activity levels much lower than those reported for acetogens. Propyl iodide inhibited methylmercury and acetyl-CoA syntheses to similar extents, and methylmercury synthesis was found to compete with acetyl-CoA synthesis for methyl groups. On the basis of these findings, we propose that in methylmercury synthesis by D. desulfuricans LS the methyl group is transferred from CH3-tetrahydrofolate via methylcobalamin. The methyl group may originate from C-3 of serine or from formate via the acetyl-CoA synthase pathway. These pathways are not unique to D. desulfuricans LS, and thus the ability of this bacterium to methylate mercury is most likely associated with the substrate specificity of its enzymes.
机译:基于前体的14 C掺入和细胞提取物中相关酶活性的测定,研究了Desulfovibrio desulfuricans LS合成甲基汞的方法。通过测量丝氨酸羟甲基转移酶和该途径其他酶的相对较高的活性,证实了先前观察到的C-3从丝氨酸掺入甲基汞中。从H14COO-和H14CO3-到甲基汞的标记物掺入率很高,促使人们测定了乙酰辅酶A(CoA)合酶途径的酶。发现存在这些酶,但活性水平大大低于报道的产乙酸酶。碘代丙对甲基汞和乙酰辅酶A的合成抑制程度相似,并且发现甲基汞的合成与乙酰辅酶A的甲基竞争。根据这些发现,我们提出在脱硫尿霉菌LS合成甲基汞的过程中,甲基是从CH3-四氢叶酸经甲基钴胺素转移的。甲基可以经由乙酰辅酶A合酶途径源自丝氨酸的C-3或甲酸盐。这些途径不是脱硫葡萄球菌LS独有的,因此,这种细菌将汞甲基化的能力很可能与其酶的底物特异性有关。

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