Table 1 Results obtained in the comparative trial by the real-time PCR and the reference culture method a, b. Sample typec No. of samples % Valued κe N PA NA FN TP FP AC SE SP Minced meat 60 30 30 0 0 0 100 100 100 1.00 Poultry neck-skins 60 27 31 0 2 0 97 107 100 0.97 Pig carcass swabs 120 21 98 1 0 0 99 95 100 0.97 TOTAL 240 78 159 1 2 0 99 103 100 0.97 a PA: Positive Agreement, NA: Negative Agreement, TP: True Positive, FN: False Negative, FP: False Positive, AC: Relative Accuracy, SE: Relative Sensitivity,
SP: Relative Specificity, N = PA +NA + FN + TP + FP. b Results are given after confirmation. c Matrices as defined by NordVal [15]; matrix meat: minced meat BAY 63-2521 concentration (raw pork and veal) and poultry neck skins, matrix environmental samples: pig carcass swabs. Meat samples were artificially contaminated and swab samples potentially naturally contaminated. d See Materials and ARS-1620 clinical trial methods for accuracy, sensitivity and specificity equations. e Cohen’s kappa calculated according to NMKL procedure no. 20 [26]. The detection level of the two methods was 1–10 CFU/25 g sample
(corresponding to a relative detection level of 100%) in all cases except for the swabs inoculated with S. Enteritidis, selleck chemicals where it was 10–100 CFU/25 g for the NMKL method (relative detection level > 100%) (data not shown). To determine the relative accuracy, sensitivity and specificity, a total of 240 samples representing meat and environmental samples were analyzed by the PCR and NMKL methods (Table 1). A total of 80 out of 240 samples gave positive results by real-time PCR, compared Staurosporine with a total of 79 by the culture-based method. Two samples showed positive deviation (true positives by the PCR method) and one negative deviation (false negative by the PCR method) (Table 1). A very good agreement between the two methods was obtained using Cohen’s kappa (Table 1). Collaborative trial The purpose of the collaborative
trial was to determine the variability in the results obtained by the real-time PCR method detecting Salmonella in identical samples. The trial was conducted in accordance with the guidelines provided by NordVal [15]. The samples and the other contents of the ring trial kit sent out to the participants were found to be stable during the period of the trial (data not shown). The influence of the refrigerated transit was investigated prior to the collaborative trial, and no detrimental effects were found after three days (data not shown). Six laboratories participated in the collaborative trial, and valid results were obtained from five of the laboratories and used for the statistical analysis (Table 2). In agreement with the predefined criteria, results from one participant were excluded due to failure in the PCR analysis (lack of amplification in the positive control and several samples with no amplification of either the target or the IAC).