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首页> 外文期刊>Archives of Microbiology >Use of gene probes to assess the impact and effectiveness of aerobic in situ bioremediation of TCE
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Use of gene probes to assess the impact and effectiveness of aerobic in situ bioremediation of TCE

机译:使用基因探针评估TCE有氧原位生物修复的影响和效果

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Gene probe hybridization was used to determine distribution and expression of co-metabolic genes at a contaminated site as it underwent in situ methanotrophic bioremediation of trichloroethylene (TCE). The bioremediation strategies tested included a series of air, air:methane, and air:methane:nutrient pulses of the test plot using horizontal injection wells. During the test period, the levels of TCE reduced drastically in almost all test samples. Sediment core samples (n = 367) taken from 0 m (surface)–43 m depth were probed for gene coding for methanotrophic soluble methane monooxygenase (sMMO) and heterotrophic toluene dioxygenase (TOD), which are known to co-metabolize TCE. The same sediment samples were also probed for genes coding for methanol dehydrogenase (MDH) (catalyzing the oxidation of methanol to formaldehyde) to assess specifically changes in methylotrophic bacterial populations in the site. Gene hybridization results showed that the frequency of detection of sMMO genes were stimulated approximately 250% following 1% methane:air (v/v) injection. Subsequent injection of 4% methane:air (v/v) resulted in an 85% decline probably due to nutrient limitations, since addition of nutrients (gaseous nitrogen and phosphorus) thereafter caused an increase in the frequency of detection of sMMO genes. Detection of TOD genes declined during the process, and eventually they were non-detectable by the final treatment, suggesting that methanotrophs displaced the TOD gene containing heterotrophs. Active transcription of sMMO and TOD was evidenced by hybridization to mRNA. These analyses combined with results showing the concomitant decline in TCE concentrations, increases in chloride concentration and increases in methanotroph viable counts, provide multiple lines of evidence that TCE remediation was caused specifically by methanotrophs. Our results suggest that sMMO genes are responsible for most, if not all, of the observed biodegradation of TCE. This study demonstrates that the use of nucleic acid analytical methods provided a gene specific assessment of the effects of in situ treatment technologies.
机译:基因探针杂交被用来确定代谢基因在受污染部位的分布和表达,因为它正在进行三氯乙烯(TCE)的甲烷营养生物修复。测试的生物修复策略包括使用水平注入井对测试区的一系列空气,空气:甲烷和空气:甲烷:养分脉冲进行测试。在测试期间,几乎所有测试样品中的三氯乙烯含量都急剧下降。从沉积物核心样品(n = 367)中抽取深度0 m(表面)-43 m,以寻找编码甲基营养生物可溶性甲烷单加氧酶(sMMO)和异养性甲苯双加氧酶(TOD)的基因,这些基因已知会共同代谢TCE。还对相同的沉积物样品进行了编码甲醇脱氢酶(MDH)(催化甲醇氧化为甲醛)的基因的探测,以评估该位点甲基营养菌群体的特异性变化。基因杂交结果表明,在注入1%甲烷:空气(v / v)后,刺激sMMO基因的检测频率大约提高了250%。随后注入4%的甲烷:空气(v / v)可能导致85%的下降,这可能是由于营养限制所致,因为随后添加营养(气态氮和磷)会导致sMMO基因检测的频率增加。在此过程中,TOD基因的检测下降,最终在最终处理中无法检测到,这表明甲烷营养生物取代了含有异养生物的TOD基因。 sMMO和TOD的主动转录通过与mRNA杂交得以证明。这些分析与结果相结合,显示出TCE浓度随之下降,氯化物浓度增加和甲烷氧化菌活菌计数增加,提供了多条证据表明TCE修复专门由甲烷氧化菌引起。我们的结果表明,sMMO基因是导致大多数(即使不是全部)TCE生物降解的原因。这项研究表明,核酸分析方法的使用为原位治疗技术的效果提供了基因特异性评估。

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