Abstract:Objective To develop a RT-PCR method for determination of Encephalomyocarditis virus ( EMCV) in Mongolian gerbils and Laboratory mice. Methods The primers were designed and synthesised according to the published EMCV specific sequences of VP1 gene. RT - PCR method is established,carries on the specificity,sensitivity,stability test. The method is used to detected 62 Mongolian gerbils and 12 mice. Results The developed RT-PCR method is good in specificity,ensitivity,stability; and its minimum detection limit using the recombinant plasmid containing EMCV gene as atemplate was 4. 1pg /μL,and the lowest detection virus titer is 10 - 7 ml- 1. The 62 Mongolian gerbils after RT - PCRdetection were negative; The 12 mice after RT -PCR detection,there were one EMCV positive,compared with the EMCV in Genebank,The homologies in nucleotide sequence of one positive mice is 85% ; there were 5 mice can be detected EMCV in the body of the 6 mice by artificial infection EMCV. Conclusion The developed RT-PCR method is good in specificity,ensitivity,stability,can be used in detecting the EMCV in laboratory animal,such as Mongolian gerbils andmice.
