Rapid method for separation of bacterial DNA from humic substances in sediments for polymerase chain reaction.

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Appl Environ Microbiol. 1992 July; 58(7): 2292-2295

Rapid method for separation of bacterial DNA from humic substances in sediments for polymerase chain reaction.

Y L Tsai and B H Olson

County Sanitation Districts of Orange County, Fountain Valley, California 92728.

ABSTRACT

The polymerase chain reaction (PCR) was used to amplify an Escherichiacoli 16S ribosomal gene fragment from sediments with high contentsof humic substances. Total DNA was extracted from 1 g of E.coli seeded or unseeded samples by a rapid freeze-and-thaw method.Several approaches (use of Bio-Gel P-6 and P-30 and SephadexG-50 and G-200 columns, as well as use of the Stoffel fragment)were used to reduce interference with the PCR. The best resultswere obtained when crude DNA extracts containing humic substanceswere purified by using Sephadex G-200 spun columns saturatedwith Tris-EDTA buffer (pH 8.0). Eluted fractions were collectedfor PCR analyses. The amplified DNA fragment was obtained fromseeded sediments containing fewer than 70 E. coli cells perg. Because only 1/100 of the eluted fractions containing DNAextracts from 70 cells per g was used for the PCR, the sensitivityof detection was determined to be less than 1 E. coli cell.Thus, DNA direct extraction coupled with this technique to removeinterference by humic substances and followed by the PCR canbe a powerful tool to detect low numbers of bacterial cellsin environmental samples containing humic substances.

Appl Environ Microbiol. 1992 July; 58(7): 2292-2295

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