CONCENTRATION AND PURIFICATION OF BEEF EXTRACT MOCK ELUATES FROM WATER SAMPLES FOR THE DETECTION OF ENTEROVIRUSES, HEPATITIS-A VIRUS, AND NORWALK VIRUS BY REVERSE TRANSCRIPTION-PCR

In this study we developed a concentration and purification procedure to facilitate reverse transcription (RT)-PCR detection of enteric viruses in water sample concentrates obtained by conventional filter adsorption-elution methods. One liter of beef extract-glycine eluate with or without humic acid and seeded with poliovirus type 1, hepatitis A virus, and Norwalk virus was used as a model system, and the eluent was further processed for RT-PCR compatibility. The sample concentration and purification procedures which we used included polyethylene glycol precipitation, Pro-Cipitate precipitation, a second polyethylene glycol precipitation, spin column chromatography, and ultrafiltration. The sample volumes were reduced from 1 liter to 20 to 50 mu l, and the samples were purified enough so that viruses could be detected by the RT-PCR The ability to detect low levels of enteric viruses by molecular techniques was compared directly with the ability to detect enteric viruses by cell culture infectivity procedures. As little as 3 PFU of poliovirus type 1 in an initial 1 liter of mock eluate was detected by the RT PCR.