University of Tabriz Journal of Zoonotic Diseases 2476-535X 9 4 2025 09 01 Simultaneous detection of Dengue virus serotypes by nested-multiplex PCR 998 1007 19864 10.22034/jzd.2025.19864 EN David Shayan Institute of Molecular Biological System Transfer, Tehran, Iran/Department of Biology, Kish International Campus, University of Tehran, Tehran, Iran Reza Heidari Medical Biotechnology Research Center, AJA University of Medical Sciences, Tehran, Iran Parviz Shayan Research Center of Ticks and Tick-borne Diseases, Department of Parasitology, Faculty of Veterinary Medicine, University of Tehran, Tehran, Iran/ Institute of Molecular Biological System Transfer, Tehran, Iran Journal Article 2025 03 14 <em>Dengue</em> virus is a single positive RNA virus causing <em>Dengue</em> fever (break-bone fever), belonging to the <em>Flavivirus</em> in the family of <em>Flaviviridae</em>. Four antigenically distinct serotypes have been reported from this virus developing infection with asymptomatic or clinical signs of high fever, headache, body aches, nausea and rash in human.  This virus is mainly transmitted by mosquitoes <em>Aedes aegypti</em> or <em>Aedes albopictus</em> and in the last decade it has gained importance in the public health in Iran. It was reported that non-human primates, bovids, horses, pigs, birds, and rodents can be infected with this virus. Therefore, early detection of the virus in mosquitoes and humans can be important in controlling the disease. In the present study, we introduce a primer pair detecting <em>Dengue</em> virus (all four serotypes) and a nested-Multiplex PCR detecting each serotype simultaneously. For this aim we used recombinant plasmid constructs (D1-, D2-, D3- and D4- pEX-A128 plasmid) having ca. 660 nucleotides from 5` end of the corresponding serotype and larvae of <em>Aedes</em> mosquito. Our results confirmed that the 5` end of the virus is suitable for simultaneously detection of <em>Dengue</em> virus serotypes by RT-PCR and discrimination of serotypes from each other by multiplex PCR. In conclusion, we propose that to lower the cost, the <em>Dengue</em> virus should be preferably detected first by serotype common RT-PCR. In the case of positive result, the serotype determination can be performed by nested-multiplex PCR. Since for the management of public health, monitoring of the circulating <em>Dengue</em> virus is of great importance, the presented method is a suitable assay for this aim.  DDengue virus RT PCR Multiplex PCR Serotypes RNA virus https://jzd.tabrizu.ac.ir/article_19864_03622284bbb7f8499c78c3dd46de7069.pdf