Multiplex PCR Approach for Rapid African Swine Fever Virus Genotyping

Viruses Pub Date : 2024-09-13 DOI:10.3390/v16091460
Matthias Licheri, Manon Flore Licheri, Kemal Mehinagic, Emilia Radulovic, Nicolas Ruggli, Ronald Dijkman
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Abstract

African swine fever virus (ASFV) has been spreading through Europe, Asia, and the Caribbean after its introduction in Georgia in 2007 and, due to its particularly high mortality rate, poses a continuous threat to the pig industry. The golden standard to trace back the ASFV is whole genome sequencing, but it is a cost and time-intensive methodology. A more efficient way of tracing the virus is to amplify only specific genomic regions relevant for genotyping. This is mainly accomplished by amplifying single amplicons by PCR followed by Sanger sequencing. To reduce costs and processivity time, we evaluated a multiplex PCR based on the four primer sets routinely used for ASFV genotyping (B646L, E183L, B602L, and intergenic I73R-I329L), which was followed by Nanopore ligation-based amplicon sequencing. We show that with this protocol, we can genotype ASFV DNA originating from different biological matrices and correctly classify multiple genotypes and strains using a single PCR reaction. Further optimization of this method can be accomplished by adding or swapping the primer sets used for amplification based on the needs of a specific country or region, making it a versatile tool that can speed up the processing time and lower the costs of genotyping during ASFV outbreaks.
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用于快速非洲猪瘟病毒基因分型的多重 PCR 方法
非洲猪瘟病毒(ASFV)自 2007 年传入格鲁吉亚后,一直在欧洲、亚洲和加勒比海地区蔓延,由于其死亡率特别高,对养猪业构成了持续威胁。追溯 ASFV 的黄金标准是全基因组测序,但这种方法成本高、耗时长。追踪病毒的更有效方法是只扩增与基因分型相关的特定基因组区域。这主要是通过 PCR 扩增单个扩增子,然后进行 Sanger 测序。为了降低成本和缩短处理时间,我们评估了一种基于 ASFV 基因分型常用的四组引物(B646L、E183L、B602L 和基因间 I73R-I329L)的多重 PCR,然后进行基于 Nanopore 连接的扩增子测序。我们的研究结果表明,利用这一方法,我们可以对来自不同生物基质的 ASFV DNA 进行基因分型,并通过一次 PCR 反应对多个基因型和菌株进行正确分类。我们还可以根据特定国家或地区的需要,通过添加或交换扩增引物组来进一步优化这种方法,使其成为一种多功能工具,在 ASFV 爆发期间加快处理速度并降低基因分型的成本。
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