Complete genome analysis of a novel recombinant isolate of pepper veinal mottle virus from mainland China

The viral symptoms of the pepper sample display mottle, yellowing and malformation on leaf, this pepper plant was sampled in a survey of pepper diseases in Hunan province, China in 2014. Total RNA infected pepper sample was extracted by an RNeasy mini kit (QIAGEN, Germany). Full-length cDNA was synthesized by using an oligo(dT)18 primer and TransScript® All-in-One First-Strand cDNA Synthesis SuperMix for PCR Kit (TransGen Biotech, Beijing,China) according to manufacturer’s introduction. The complete genome sequence of the isolate PVMV-HN was amplified from eight overlapping fragments using specific primers (Additional file 1: Table S1), and the 5’- and 3’-terminal ends of the genome was reconfirmed by 5’-RACE and 3’-RACE, respectively, as described previously [9]. PCR products were cloned into pEASY-T5 Vector (TransGen, Beijing, China) and sequenced by Sangon Biotechnology Co., Ltd. (Shanghai, China) using an ABI3730 automated DNA sequencer (Applied Biosystems, USA). Sequences were assembled using DNAMAN version 8 (Lynnon, Quebec, Canada). Sequences analysis and comparison of PVMV-HN to the reference sequences were performed using DNAStar 7.01 package (DNASTAR, Madison, USA). The complete RNA genome or polyprotein sequences and CP sequences of other PVMV isolates and other Potyviruses were downloaded from the National Center for Biotechnology Information (NCBI) database (http://​www.​ncbi.​nlm.​nih.​gov/​). The information of all used sequences was listed in Additional file 1: Table S2. Multiple nucleotide sequence alignments were performed with CLUST W, possible recombination events were evaluated by Recombination Detection Program (RDP3) [13] and a phylogenetic tree was reconstructed by the maximum-likelihood method using MEGA5 [14].

The complete genome of the PVMV-HN isolate comprises 9793 nucleotides (nt), with 194 nt at the 5’ non-translated region (NTR) and 373 nt at the 3’ NTR. Similar as other potyviruses, a large typical open reading frame (ORF) was identified as a polyprotein containing 3074 amino acids (aa) with an AUG start codon and UGA stop codon. PVM-HN shares 99 % nucleotide sequence identity with PVMV isolate of Ghana (DQ645484), and 98 % with PVMV isolate of Taiwan (FJ617225) with genome level, however, only 94 % nucleotide sequence identity with PVMV isolates (GQ918276 and GQ918274) from Mali with polyprotein gene level.

A search for possible recombination event was carried out using RDP3, there were three modules (Maxchi, Chimaera and SiScan) of RDP3 supported possible two recombination events between PVMV-HN with PVMV isolates from Ghana and Taiwan with high confidence (p < 2.25 × 10⁻⁵, Fig. 1). The sites of beginning and ending breakpoint were occurring at 3764 nt and 4146 nt, 4726 nt and 5275 nt, respectively. The potential major and minor parents were the PVMV-p (Ghana isolate) and PVMV-ns1 (Taiwan isolate). The existing two recombination events in PVMV-HN probably hinted it was a novel recombinant.

Phylogenetic analysis of PVMV-HN isolate from China to other potyviruses based on nucleotide sequences of complete genome or polyprotein gene level (Fig. 2a) and CP gene level (Fig. 2b) was built and two unique consensus trees topology were obtained. The two major clades were distinct existence well supported by bootstrap values associated to the branches of the tree (Fig. 2a). The first clade comprises of PVY, Pepper mottle virus, Potato virus V, and the second one includes PVMV and ChiVMV, shows close relationship of PVMV with ChiVMV, as mentioned by Moury et al. [1]. PVMV group was divided into two subgroups, the Africa subgroup and the East Asia subgroup. It is possible that the diversification of PVMV group was relevant with geography. Phylogenetic analysis of more PVMV isolates from different geographic origins based on nucleotide sequence of CP gene was also built and divided 12 PVMV isolates into two distinct major groups (Fig. 2b), reconfirmed that the diversification of PVMV group was relevant with geography, and PVMV-HN from China clustered in the East Asia subgroup. Additionally, phylogenetic analysis suggested that PVMV-HN likely originate from Taiwan and India as its closest evolution relationship (Fig. 2). Thus the recombination events (Fig. 1) were likely critical for PVMV-HN adaption and epidemic [15]. More sequences of PVMV isolates in China would help to understand phylogenetic relationship of PVMV in mainland China with that in other geography.

This study provided the first complete genome sequence about PVMV from mainland China and revealed it is probably a novel recombinant.

The complete genome sequence of the isolate of PVMV-HN is permanently available in the GenBank database under the accession number KR002568.