TABLE 3.
Quantitative detection of M. agalactiae in raw sheep milka
| Approximate M. agalactiae cells/25 ml | Approximate M. agalactiae genome equivalents/reactionb | Signal ratioc | CT value ± SEMd | Relative accuracye |
|---|---|---|---|---|
| 2.5 × 107 | 1 × 105 | 9/9 | 24.20 ± 0.02 | 87.17 |
| 2.5 × 106 | 1 × 104 | 9/9 | 27.12 ± 0.06 | 115.14 |
| 2.5 × 105 | 1 × 103 | 9/9 | 30.50 ± 0.05 | 110.98 |
| 2.5 × 104 | 1 × 102 | 9/9 | 34.09 ± 0.06 | 91.81 |
| 2.5 × 103 | 10 | 9/9 | 37.33 ± 0.23 | 97.43 |
| 2.5 × 102 | 1 | 9/9 | 38.63 ± 0.32 | NA |
| 25 | 0.1 | 0/9 | NAf | NA |
| 3 | 0.01 | 0/9 | NA | NA |
| 0f | 0 | 0/9 | NA | NA |
Raw milk was collected directly from a sheep farm. Data show results from three independent experiments with three PCR replicates used in each. The overall efficiency was 0.996, and the linearity (R2) was 0.9989. NA, not applicable.
Estimated numbers of M. agalactiae genome equivalents in each PCR run, assuming 100% DNA extraction efficiency, are shown. Each reaction mixture contained 2 μl of a DNA preparation taken from the 1:10 dilution of the initial 50 μl extracted from 25 ml of raw sheep milk.
Number of positive results out of nine reactions.
Mean CT value ± standard error of the mean (SEM) at which fluorescence intensity was equal to a fixed threshold. The experimental results were statistically significant (P < 0.05) taking into account unavoidable errors associated with serial dilutions.
Degree of correspondence between results obtained with the standard plating technique (M. agalactiae CFU/25 ml) and those obtained with the p40 Q-PCR method (M. agalactiae genome equivalents/25 ml).
Noncontaminated milk.