Unexpected cases in field diagnosis of African swine fever virus in Vietnam: The needs consideration when performing molecular diagnostic tests.

Anh Duc Truong Duc Viet Ly Thi Hao Vu Van Tuan Hoang Thi Chinh Nguyen Thi Nhu Chu Huyen Thi Nguyen The Vinh Nguyen Ngoc Thi Pham Ha Thi Thanh Tran Hoang Vu Dang

Open Vet J

Department of Biochemistry and Immunology, National Institute of Veterinary Research (NIVR), Hanoi, Vietnam.

Published: August 2020

The study investigates discrepancies in detecting African swine fever virus (ASFV) using conventional and real-time PCR methods, highlighting a potential issue with primer and probe mismatches.
Results indicated that a single mismatch in the probe binding region could lead to false-negative results in real-time PCR, emphasizing the importance of precise primer design.
The research calls for careful consideration of molecular diagnostic methods and updated ASFV sequence databases for effective epidemiological surveillance.

Background: The first confirmed case of African swine fever (ASF) in Vietnam was reported officially in February 2019. To date, ASF virus (ASFV) have been detected in 63/63 provinces in Vietnam. Currently, real-time polymerase chain reaction (PCR) is considered to be a powerful tool for viral detection in field samples, including ASFV. However, some recent reports have suggested that mismatches in primer and probe binding regions may directly affect real-time PCR qualification, leading a false-negative result.

Aim: This study aims to further examine a conflicting result obtained from two OIE recommended methods, conventional PCR and real-time PCR, for ASFV detection.

Methods: Two ASF suspected pigs from different provinces in the north of Vietnam were selected for this study based on clinical signs and postmortem lesions. The different results obtained by OIE-recommended conventional PCR and real-time PCR were further analyzed by the Sanger sequencing method and virus isolation in combination with hemadsorption (HAD) test using porcine alveolar macrophages cells.

Results: The results showed that when the primer sequence matched perfectly with the sequences of field isolates, a mutation in probe binding region was found, indicating that a single mismatch in the probe binding site may cause a false-negative result by real-time PCR in detecting ASFV in clinical samples in Vietnam. An agreement between conventional PCR, using PPA1/PPA2 primers and two golden standard methods, virus isolation in combination with HAD assay, and sequencing method was observed in this study.

Conclusion: A single mismatch in the probe binding site caused a failse-negative result by realtime PCR method in field diagnosis of ASFV. The needs consideration when selecting the appropriate molecular diagnostic methods is based on the current databases of ASFV sequences, particularly for epidemiological surveillance of ASF.

Download full-text PDF	Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC7419073	PMC
http://dx.doi.org/10.4314/ovj.v10i2.8	DOI Listing

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