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Thiocyanate Degradation by a Highly Enriched Culture of the Neutrophilic Halophile Thiohalobacter sp. Strain FOKN1 from Activated Sludge and Genomic Insights into Thiocyanate Metabolism

机译:中性嗜盐嗜盐菌嗜盐菌种的高度富集培养可降解硫氰酸盐。来自活性污泥的FOKN1菌株和硫氰酸盐代谢的基因组学见解

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摘要

Thiocyanate (SCN ) is harmful to a wide range of organisms, and its removal is essential for environmental protection. A neutrophilic halophile capable of thiocyanate degradation, . strain FOKN1, was highly enriched (relative abundance; 98.4%) from activated sludge collected from a bioreactor receiving thiocyanate-rich wastewater. The enrichment culture degraded 3.38 mM thiocyanate within 140 h, with maximum activity at pH 8.8, 37°C, and 0.18 M sodium chloride. Thiocyanate degradation was inhibited by 30 mg L phenol, but not by thiosulfate. Microbial thiocyanate degradation is catalyzed by thiocyanate dehydrogenase, while limited information is currently available on the molecular mechanisms underlying thiocyanate degradation by the thiocyanate dehydrogenase of neutrophilic halophiles. Therefore, (meta)genomic and proteomic analyses of enrichment cultures were performed to elucidate the whole genome sequence and proteome of . strain FOKN1. The 3.23-Mb circular . strain FOKN1 genome was elucidated using a PacBio RSII sequencer, and the expression of 914 proteins was identified by tandem mass spectrometry. The . strain FOKN1 genome had a gene encoding thiocyanate dehydrogenase, which was abundant in the proteome, suggesting that thiocyanate is degraded by thiocyanate dehydrogenase to sulfur and cyanate. The sulfur formed may be oxidized to sulfate by the sequential oxidation reactions of dissimilatory sulfite reductase, adenosine-5′-phosphosulfate reductase, and dissimilatory ATP sulfurylase. Although the . strain FOKN1 genome carried a gene encoding cyanate lyase, its protein expression was not detectable. The present study advances the understanding of the molecular mechanisms underlying thiocyanate degradation by the thiocyanate dehydrogenase of neutrophilic halophiles.
机译:硫氰酸盐(SCN)对多种生物有害,因此去除对环境保护至关重要。能够降解硫氰酸盐的嗜中性嗜盐菌。 FOKN1菌株从生物反应器中收集的活性污泥中高度富集(相对丰度; 98.4%),该反应器接收到富含硫氰酸盐的废水。浓缩培养物在140小时内降解了3.38 mM的硫氰酸盐,在pH 8.8、37°C​​和0.18 M的氯化钠下具有最大的活性。 30 mg L苯酚可抑制硫氰酸盐的降解,但硫代硫酸盐则不能。微生物硫氰酸盐的降解是由硫氰酸盐脱氢酶催化的,而有关中性嗜盐菌的硫氰酸盐脱氢酶降解硫氰酸盐的分子机理的信息尚不多。因此,进行了富集培养的(元)基因组和蛋白质组学分析,以阐明的全基因组序列和蛋白质组。菌株FOKN1。 3.23 Mb圆形。使用PacBio RSII测序仪阐明了FOKN1菌株的基因组,并通过串联质谱鉴定了914个蛋白的表达。的。 FOKN1菌株的基因组中有一个编码硫氰酸盐脱氢酶的基因,该蛋白质在蛋白质组中含量很高,表明硫氰酸盐被硫氰酸盐脱氢酶降解为硫和氰酸盐。所形成的硫可以通过异化亚硫酸还原酶,腺苷5'-磷酸磷酸还原酶和异化ATP硫酸化酶的顺序氧化反应氧化为硫酸盐。虽然 。 FOKN1菌株的基因组携带一个编码氰酸酯裂解酶的基因,其蛋白表达无法检测到。本研究提高了对嗜中性嗜盐菌的硫氰酸盐脱氢酶降解硫氰酸盐的分子机制的理解。

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