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Possible Involvement of a Tetrathionate Reductase Homolog in Dissimilatory Arsenate Reduction by Anaeromyxobacter sp. Strain PSR-1

机译:四分离化酸还原酶同源物在厌氧杆菌SP减少的含糊不化化砷酸盐的可能涉及。 应变PSR-1

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Anaeromyxobacter sp. strain PSR-1, a dissimilatory arsenate [As(V)]-reducing bacterium, can utilize As(V) as a terminal electron acceptor for anaerobic respiration. A previous draft genome analysis revealed that strain PSR-1 lacks typical respiratory As(V) reductase genes ( arrAB ), which suggested the involvement of another protein in As(V) respiration. Dissimilatory As(V) reductase activity of strain PSR-1 was induced under As(V)-respiring conditions and was localized predominantly in the periplasmic fraction. The activity was visualized by partially denaturing gel electrophoresis, and liquid chromatography-tandem mass spectrometry analysis identified proteins involved in the active band. Among these proteins, a protein annotated as molybdopterin-dependent oxidoreductase (PSR1_00330) exhibited the highest sequence coverage, 76%. Phylogenetic analysis revealed that this protein was a homolog of tetrathionate reductase catalytic subunit TtrA. However, the crude extract of strain PSR-1 did not show significant tetrathionate reductase enzyme activity. Comparative proteomic analysis revealed that the protein PSR1_00330 and a homolog of tetrathionate reductase electron transfer subunit TtrB (PSR1_00329) were expressed abundantly and specifically under As(V)-respiring conditions, respectively. The genes encoding PSR1_00330 and PSR1_00329 formed an operon-like structure along with a gene encoding a c -type cytochrome ( cyt c ), and their transcription was upregulated under As(V)-respiring conditions. These results suggest that the protein PSR1_00330, which lacks tetrathionate reductase activity, functions as a dissimilatory As(V) reductase in strain PSR-1. Considering the wide distribution of TtrA homologs among bacteria and archaea, they may play a hitherto unknown role along with conventional respiratory As(V) reductase (Arr) in the biogeochemical cycling of arsenic in nature.IMPORTANCE Dissimilatory As(V)-reducing prokaryotes play significant roles in arsenic release and contamination in groundwater and threaten the health of people worldwide. Generally, such prokaryotes reduce As(V) by means of a respiratory As(V) reductase designated Arr. However, some dissimilatory As(V)-reducing prokaryotes such as Anaeromyxobacter sp. strain PSR-1 lack genes encoding Arr, suggesting the involvement of other protein in As(V) reduction. In this study, using multiple proteomic and transcriptional analyses, it was found that the dissimilatory As(V) reductase of strain PSR-1 was a protein closely related to the tetrathionate reductase catalytic subunit (TtrA). Tetrathionate reductase is known to play a role in anaerobic respiration of Salmonella on tetrathionate, but strain PSR-1 showed neither growth on tetrathionate nor significant tetrathionate reductase enzyme activity. These results suggest the possibility that TtrA homologs encoded in a wide variety of archaeal and bacterial genomes might function as dissimilatory As(V) reductases.
机译:Anaeromyxobacter sp。菌株PSR-1,一种分化砷酸盐[AS(v)] - 还原细菌可以用作(v)作为厌氧呼吸的末端电子受体。先前的基因组分析表明,菌株PSR-1缺乏典型的呼吸系统(v)还原酶基因(arrab),这表明另一种蛋白质涉及(v)呼吸。诱导菌株PSR-1的含量异化作为(v)还原酶活性在AS(v) - 份额条件下诱导,主要在周质级分中定位。通过部分变性凝胶电泳来观察活性,液相色谱 - 串联质谱分析鉴定有效带中的蛋白质。在这些蛋白质中,作为钼醇依赖性氧化还原酶(PSR1_00330)注释的蛋白质表现出最高的序列覆盖率,76%。系统发育分析显示,该蛋白质是四乙酸盐还原酶催化亚单位TTRA的同源物。然而,菌株PSR-1的粗提物未显示出显着的四分离化还原酶酶活性。对比蛋白质组学分析显示,蛋白质PSR1_00330和四分离化还原酶电子转移亚单位TTRB(PSR1_00329)的同源物分别表达,特别是在(v) - 重量的条件下。编码PSR1_00330和PSR1_00329的基因与编码C型细胞色素(CYT C)的基因一起形成摩尔式结构,并且它们的转录在AS(v) - 缺乏条件下。这些结果表明,缺乏四分离化还原酶活性的蛋白质PSR1_00330,用作菌株PSR-1中的差异(V)还原酶。考虑到细菌和古代TTRA同源物的广泛分布,它们可能在砷的生物地球化学循环中与常规呼吸系统(v)还原酶(ARR)一起发挥迄今未知的作用。称为(v)缩影原核生物的分化在地下水中的砷释放和污染方面的显着作用,威胁全世界人民的健康。通常,这种原核生物通过呼吸作为(v)还原酶指定ARR减少为(v)。但是,一些含糊diacuatory的原核生物如厌氧杆菌SP。菌株PSR-1缺乏编码ARR的基因,表明其他蛋白质的累积为(v)减少。在该研究中,使用多种蛋白质组学和转录分析,发现菌株PSR-1的含量(V)还原酶是与四分离化还原酶催化亚基(TTRA)密切相关的蛋白质。已知四分离化酸还原酶在四分离化物上的沙门氏菌的厌氧呼吸中发挥作用,但菌株PSR-1既不均未对四阴离子进行生长,也不是大致的四乙酸还原酶酶活性。这些结果表明,在各种古藻和细菌基因组中编码的TTRA同源物可能起到(V)还原酶的含量异化。

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