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Detection and Quantification of Methyl tert-Butyl Ether-Degrading Strain PM1 by Real-Time TaqMan PCR

机译:实时TaqMan PCR检测和定量降解甲基叔丁基醚的菌株PM1

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The fuel oxygenate methyl tert-butyl ether (MTBE), a widely distributed groundwater contaminant, shows potential for treatment by in situ bioremediation. The bacterial strain PM1 rapidly mineralizes and grows on MTBE in laboratory cultures and can degrade the contaminant when inoculated into groundwater or soil microcosms. We applied the TaqMan quantitative PCR method to detect and quantify strain PM1 in laboratory and field samples. Specific primers and probes were designed for the 16S ribosomal DNA region, and specificity of the primers was confirmed with DNA from 15 related bacterial strains. A linear relationship was measured between the threshold fluorescence (C T) value and the quantity of PM1 DNA or PM1 cell density. The detection limit for PM1 TaqMan assay was 2 PM1 cells/ml in pure culture or 180 PM1 cells/ml in a mixture of PM1 withEscherichia coli cells. We could measure PM1 densities in solution culture, groundwater, and sediment samples spiked with PM1 as well as in groundwater collected from an MTBE bioaugmentation field study. In a microcosm biodegradation study, increases in the population density of PM1 corresponded to the rate of removal of MTBE.
机译:含氧化合物甲基叔丁基醚(MTBE)是一种分布广泛的地下水污染物,具有通过原位生物修复进行处理的潜力。细菌菌株PM1在实验室培养物中迅速矿化并在MTBE上生长,当接种到地下水或土壤微观环境中时,可以降解污染物。我们应用TaqMan定量PCR方法检测和定量实验室和现场样品中的PM1菌株。针对16S核糖体DNA区域设计了特异性引物和探针,并用来自15个相关细菌菌株的DNA证实了引物的特异性。测量阈值荧光(C T)值与PM1 DNA数量或PM1细胞密度之间的线性关系。 PM1 TaqMan测定的检出限为纯培养物中2 PM1细胞/ ml或PM1与大肠杆菌细胞混合物中的180 PM1细胞/ ml。我们可以测量溶液培养物,地下水,掺有PM1的沉积物样品以及MTBE生物强化田间研究收集的地下水中的PM1密度。在微观生物降解研究中,PM1种群密度的增加与MTBE的去除速率相对应。

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