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含水层源假单胞菌在好氧和反硝化条件下还原 Cr(VI) 的生理和转录研究。

Physiological and transcriptional studies of Cr(VI) reduction under aerobic and denitrifying conditions by an aquifer-derived pseudomonad.

机构信息

Earth Sciences Division, Lawrence Berkeley National Laboratory, Berkeley, California 94720, USA.

出版信息

Environ Sci Technol. 2010 Oct 1;44(19):7491-7. doi: 10.1021/es101152r.

Abstract

Cr(VI) is a widespread groundwater contaminant that is a potent toxin, mutagen, and carcinogen. In situ reductive immobilization is a favored approach for Cr(VI) bioremediation, and Cr(VI) reduction has been reported in a variety of aerobic, facultative, and anaerobic bacteria, including a number of pseudomonads. However, studies comparing Cr(VI) reduction under aerobic and denitrifying conditions in the same organism are not available. We have conducted studies with strain RCH2, a bacterium similar to Pseudomonas stutzeri that we isolated from a Cr-contaminated aquifer. Cell suspension studies with lactate demonstrated that Cr(VI) reduction could occur under either denitrifying or aerobic conditions (at comparable specific rates) and that reduction was at least 20-fold more rapid when the terminal electron acceptor (i.e., nitrate or O(2)) was present. Our results suggest that Cr(VI) reduction by strain RCH2 under either aerobic or denitrifying conditions is primarily cometabolic in the sense that the physiological electron acceptor (oxygen or nitrate) appears to be required. Under both aerobic and denitrifying conditions, the gene(s) associated with chromate reduction are not inducible by Cr. Continuous culture (chemostat) studies showed strong correlations (r(2) values >0.93) between nitrate reduction rate and the transcript copy number of either nirS (cytochrome cd(1) nitrite reductase) or narG (nitrate reductase α subunit). As our studies indicate that anaerobic Cr(VI) reduction by this pseudomonad requires active denitrification and that denitrification and chromate reduction rates are highly correlated (r(2) > 0.99), monitoring expression of such denitrification genes in biostimulated aquifers could provide valuable proxy information for in situ chromate reduction by similar bacteria even if the specific genes involved in chromate reduction have not been identified. We also report incomplete removal of reduced Cr from solution and on artifacts in the widely used diphenylcarbazide assay for Cr(VI), most notably, its complete inactivation in the presence of millimolar nitrite.

摘要

六价铬是一种广泛存在于地下水中的污染物,具有很强的毒性、致突变性和致癌性。原位还原固定化是一种用于六价铬生物修复的首选方法,已经有报道称,多种需氧、兼性和厌氧细菌都能还原六价铬,包括一些假单胞菌。然而,在同一生物体中比较好氧和反硝化条件下的六价铬还原的研究尚未见报道。我们用 RCH2 菌株进行了研究,RCH2 菌株类似于我们从铬污染含水层中分离到的恶臭假单胞菌。用乳酸盐进行细胞悬浮研究表明,六价铬还原可以在反硝化或好氧条件下进行(特定比速率相当),并且当末端电子受体(即硝酸盐或 O₂)存在时,还原速率至少快 20 倍。我们的研究结果表明,RCH2 菌株在好氧或反硝化条件下还原六价铬主要是共代谢的,因为生理电子受体(氧气或硝酸盐)似乎是必需的。在好氧和反硝化条件下,与铬酸盐还原相关的基因都不能被铬诱导。连续培养(恒化器)研究表明,硝酸盐还原速率与nirS(细胞色素 cd₁ 亚硝酸盐还原酶)或 narG(硝酸盐还原酶 α 亚基)的转录拷贝数之间存在很强的相关性(r² 值>0.93)。由于我们的研究表明,这种假单胞菌的厌氧六价铬还原需要活性反硝化,并且反硝化和铬酸盐还原速率高度相关(r²>0.99),因此即使尚未确定参与铬酸盐还原的特定基因,监测此类生物刺激含水层中这些反硝化基因的表达也可以为类似细菌的原位铬酸盐还原提供有价值的替代信息。我们还报告了从溶液中不完全去除还原的 Cr,并指出了广泛使用的二苯卡巴肼法测定六价铬存在的缺陷,特别是在存在亚硝酸盐毫摩尔浓度时,其完全失活。

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