E3S Web of Conferences (Jan 2024)
Quantitative PCR to determine the titer of infectious activity of the canine hepatitis virus
Abstract
This article presents data on the development and validation of a method for the indirect determination of the titer of infectivity of canine infectious hepatitis virus of genotype CAV-1 in raw materials for culture vaccines by real-time polymerase chain reaction using the Cq quantification cycle, including the following steps: eluting DNA of canine infectious hepatitis virus genotype CAV-1; performing amplification of a specific fragment orf 16 of canine infectious hepatitis virus genotype CAV-1 DNA using the original specific forward and reverse primers, as well as a molecular probe labeled with fluorescent dye FAM and luminescence quencher RTQ-1: CAV-1-T-F-primer with 5′-CGTAATGGGGAAACCTAGGGG-3′ design, CAV-1-T-R-primer with 5′-TCTGTGTTGTTTCTGTCTTGG-3′ design, and CAV-1-T-Pb-probe with 5′-FAM- CCAATCATCATCTCAACTCAACTAAATGCCGTG-RTQ1-3′ design; calculation of Cq quantification cycle from real-time PCR data; determination of the titer of infectivity of canine infectious hepatitis virus of genotype CAV-1 using a logarithmic function expressed as the equation lg TCAV-1 = -0.2979 × Ct + 9.2595 with an approximation reliability of 0.9941 and amplification efficiency of 99.38%. The analysis time is reduced to 3 h, and the analytical sensitivity is at least 1.0 lg TCD50/cm3.
