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Monitoring Methanotrophic Bacteria in Hybrid Anaerobic-Aerobic Reactors with PCR and a Catabolic Gene Probe

机译:利用PCR和分解代谢基因探针监测厌氧-好氧混合反应器中的甲烷营养细菌。

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摘要

We attempted to mimic in small upflow anaerobic sludge bed (UASB) bioreactors the metabolic association found in nature between methanogens and methanotrophs. UASB bioreactors were inoculated with pure cultures of methanotrophs, and the bioreactors were operated by using continuous low-level oxygenation in order to favor growth and/or survival of methanotrophs. Unlike the reactors in other similar studies, the hybrid anaerobic-aerobic bioreactors which we used were operated synchronously, not sequentially. Here, emphasis was placed on monitoring various methanotrophic populations by using classical methods and also a PCR amplification assay based on the mmoX gene fragment of the soluble methane monooxygenase (sMMO). The following results were obtained: (i) under the conditions used, Methylosinus sporium appeared to survive better than Methylosinus trichosporium; (ii) the PCR method which we used could detect as few as about 2,000 sMMO gene-containing methanotrophs per g (wet weight) of granular sludge; (iii) inoculation of the bioreactors with pure cultures of methanotrophs contributed greatly to increases in the sMMO-containing population (although the sMMO-containing population decreased gradually with time, at the end of an experiment it was always at least 2 logs larger than the initial population before inoculation); (iv) in general, there was a good correlation between populations with the sMMO gene and populations that exhibited sMMO activity; and (v) inoculation with sMMO-positive cultures helped increase significantly the proportion of sMMO-positive methanotrophs in reactors, even after several weeks of operation under various regimes. At some point, anaerobic-aerobic bioreactors like those described here might be used for biodegradation of various chlorinated pollutants.
机译:我们试图在小型上流厌氧污泥床(UASB)生物反应器中模拟自然发现的产甲烷菌和甲烷营养菌之间的代谢联系。 UASB生物反应器接种了纯甲基甲烷营养菌培养物,并通过连续的低水平氧合操作生物反应器,以促进甲烷营养菌的生长和/或存活。与其他类似研究中的反应器不同,我们使用的厌氧-好氧混合生物反应器是同步运行的,而不是顺序运行的。在这里,重点放在通过使用经典方法以及基于可溶性甲烷单加氧酶(sMMO)的mmoX基因片段的PCR扩增测定法监测各种甲烷营养种群。得到以下结果:(i)在所使用的条件下,甲基孢子孢子似乎比三孢子孢子菌存活更好; (ii)我们使用的PCR方法可检测到每克(湿重)颗粒污泥少至约2,000个含sMMO基因的甲烷营养生物; (iii)用纯甲基甲烷营养菌培养生物反应器极大地促进了含sMMO的种群的增加(尽管含sMMO的种群随时间逐渐减少,在实验结束时,它总是至少比sMMO大2个对数)。接种前的初始种群); (iv)一般而言,具有sMMO基因的人群与表现出sMMO活性的人群之间存在良好的相关性; (v)接种sMMO阳性培养物有助于显着增加反应器中sMMO阳性甲烷营养菌的比例,即使在各种条件下运行数周后也是如此。在某些时候,此处所述的厌氧-好氧生物反应器可用于各种含氯污染物的生物降解。

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