APPLICATION OF NESTED REVERSE TRANSCRIPTION PCR FOR DETECTION OF BOVINE VIRAL DIARRHEA VIRUS IN SEMEN
AMIN, A., ABD-ELMONEM, M., ALI, N. (2003). APPLICATION OF NESTED REVERSE TRANSCRIPTION PCR FOR DETECTION OF BOVINE VIRAL DIARRHEA VIRUS IN SEMEN. EKB Journal Management System, 51(4), 497-507. doi: 10.21608/vmjg.2003.375462
A AMIN; MERVAT I ABD-ELMONEM; NAWAL M ALI. "APPLICATION OF NESTED REVERSE TRANSCRIPTION PCR FOR DETECTION OF BOVINE VIRAL DIARRHEA VIRUS IN SEMEN". EKB Journal Management System, 51, 4, 2003, 497-507. doi: 10.21608/vmjg.2003.375462
AMIN, A., ABD-ELMONEM, M., ALI, N. (2003). 'APPLICATION OF NESTED REVERSE TRANSCRIPTION PCR FOR DETECTION OF BOVINE VIRAL DIARRHEA VIRUS IN SEMEN', EKB Journal Management System, 51(4), pp. 497-507. doi: 10.21608/vmjg.2003.375462
AMIN, A., ABD-ELMONEM, M., ALI, N. APPLICATION OF NESTED REVERSE TRANSCRIPTION PCR FOR DETECTION OF BOVINE VIRAL DIARRHEA VIRUS IN SEMEN. EKB Journal Management System, 2003; 51(4): 497-507. doi: 10.21608/vmjg.2003.375462

APPLICATION OF NESTED REVERSE TRANSCRIPTION PCR FOR DETECTION OF BOVINE VIRAL DIARRHEA VIRUS IN SEMEN

Veterinary Medical Journal (Giza)
Volume 51, Issue 4, October 2003, Pages 497-507    PDF (2.97 M)
Document Type: Original Article
DOI: 10.21608/vmjg.2003.375462
Authors
A AMIN* 1; MERVAT I ABD-ELMONEM2; NAWAL M ALI2
1Biotechnology Research Unit, Animal Reproduction Research Institute, Giza, Egypt.
2Virology Department, Animal Health Research Institute, Giza, Egypt
Abstract
A nested reverse transcription-polymerase chain reaction (RT-PCR) was employed for detection of bovine viral diarrhea virus (BVDV) in 59 semen samples collected from farms of known history of BVDV infection. The results indicated that 6 (10.2%) and 8 (13.6%) net and extended semen samples, respectively, were culture positive and 53 (89.8%) and 51 (86.4%) were culture-negative. On the other hand, 10 (16.9%) and 10 (16.9%) net and extended semen samples, respectively, were nested RT-PCR-positive and 49 (83.1%) and 49 (83.1%) were nested RT- PCR-negative. Ten semen samples were collected from BVDV-free animals to be used as negative control samples and they tested negative by culture, nested RT-PCR and double PCR. The re- vised sensitivity and specificity of nested RT-PCR in net and extended semen samples were 100.00 %. On the other hand, the sensitivity of culture technique in net and extended semen samples were 60.00% and 80 %, respectively, while the specificity were 100% in both net and extended semen, The results indicated that nested RT-PCR is reliable, rapid, highly sensitive, and specific for accurate detection of BVDV in semen samples. According to the best of our knowledge, our work is the first to report a nested RT-PCR assay that has proved to be efficient in detecting the presence of BVDV in semen. Finally, we recommend the use of nested RT-PCR assay as a supplemental diagnostic tool for detection and identification of BVDV in semen.
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