Real-Time PCR Quantification of Vibrio parahaemolyticus in Oysters Using an Alternative Matrix

Author:

KAUFMAN G. E.1,BLACKSTONE G. M.2,VICKERY M. C. L.2,BEJ A. K.1,BOWERS J.3,BOWEN MICHAEL D.4,MEYER RICHARD F.4,DePAOLA A.2

Affiliation:

1. 1Department of Biology, University of Alabama at Birmingham, Birmingham, Alabama 35294-1170

2. 2U.S. Food and Drug Administration, Gulf Coast Seafood Laboratory, P.O. Box 158, Dauphin Island, Alabama 36528-0158

3. 3U.S. Food and Drug Administration, Office of Math and Statistics, 5100 Paint Branch Parkway, College Park, Maryland 20740

4. 4Centers for Disease Control and Prevention, 1600 Clifton Road, Atlanta, Georgia 30333, USA

Abstract

This study examined the relationship between levels of total Vibrio parahaemolyticus found in oyster tissues and mantle fluid with the goal of using mantle fluid as a template matrix in a new quantitative real-time PCR assay targeting the thermolabile hemolysin (tlh) gene for the enumeration of total V. parahaemolyticus in oysters. Oysters were collected near Mobile Bay, Ala., in June, July, and September and tested immediately after collection and storage at 26°C for 24 h. Initial experiments using DNA colony hybridization targeting tlh demonstrated that natural V. parahaemolyticus levels in the mantle fluid of individual oysters were strongly correlated (r = 0.85, P < 0.05) with the levels found in their tissues. When known quantities of cultured V. parahaemolyticus cells were added to real-time PCR reactions that contained mantle fluid and oyster tissue matrices separately pooled from multiple oysters, a strong linear correlation was observed between the real-time PCR cycle threshold and the log concentration of cells inoculated into each PCR reaction (mantle fluid: r = 0.98, P < 0.05; and oyster: r = 0.99, P < 0.05). However, the mantle fluid exhibited less inhibition of the PCR amplification than the homogenized oyster tissue. Analysis of natural V. parahaemolyticus populations in mantle fluids using both colony hybridization and real-time PCR demonstrated a significant (P < 0.05) but reduced correlation (r =−0.48) between the two methods. Reductions in the efficiency of the real-time PCR that resulted from low population densities of V. parahaemolyticus and PCR inhibitors present in the mantle fluid of some oysters (with significant oyster-to-oyster variation) contributed to the reduction in correlation between the methods that was observed when testing natural V. parahaemolyticus populations. The V. parahaemolyticus–specific real-time PCR assay used for this study could estimate elevated V. parahaemolyticus levels in oyster mantle fluid within 1 h from sampling time.

Publisher

International Association for Food Protection

Subject

Microbiology,Food Science

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