4.8 Article

DNA Extraction-Free Quantification of Dehalococcoides spp. in Groundwater Using a Hand-Held Device

Journal

ENVIRONMENTAL SCIENCE & TECHNOLOGY
Volume 48, Issue 23, Pages 13855-13863

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/es503472h

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Funding

  1. 21st Century Michigan Economic Development Corporation [GR-476 PO 085P3000517]
  2. Strategic Environmental Research and Development Program [ER-2309]

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Nucleic acid amplification of biomarkers is increasingly used to measure microbial activity and predict remedial performance in sites with trichloroethene (TCE) contamination. Field-based genetic quantification of microorganisms associated with bioremediation may help increase accuracy that is diminished through transport and processing of groundwater samples. Sterivex cartridges and a previously undescribed mechanism for eluting biomass was used to concentrate cells. DNA extraction-free loop mediated isothermal amplification (LAMP) was monitored in real-time with a point of use device (termed Gene-Z). A detection limit of 10(5) cells L-1 was obtained, corresponding to sensitivity between 10 to 100 genomic copies per reaction for assays targeting the Dehalococcoides spp. specific 16S rRNA gene and vcrA gene, respectively. The quantity of Dehalococcoides spp. genomic copies measured from two TCE contaminated groundwater samples with conventional means of quantification including filtration, DNA extraction, purification, and qPCR was comparable to the field ready technique. Overall, this method of measuring Dehalococcoides spp. and vcrA genes in groundwater via direct amplification without intentional DNA extraction and purification is demonstrated, which may provide a more accurate mechanism of predicting remediation rates.

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