The Additional 15 nt of 5′ UTR in a Novel Recombinant Isolate of Chilli Veinal Mottle Virus in Solanum nigrum L. Is Crucial for Infection

An isolate of chilli veinal mottle virus (ChiVMV; genus Potyvirus) of Solanum nigrum L. from southwest China (ChiVMV-YunN/Yuxi) was identified and sequenced (GenBank: OP404087). Comparison with other ChiVMV isolates and recombination analyses suggested a recombinant origin. The most significant recombination event among all 21 complete ChiVMV isolates was an ending breakpoint at 1408–1488 for ChiVMV-YunN/Yuxi with ChiVMV-TaiW and ChiVMV-YunN/Ca operating as the respective major and minor parents. Interestingly, the 5′ UTR of ChiVMV-YunN/Yuxi is 15 nucleotides (‘AAAAATAAAACAACC’) longer than other reported isolates. A full-length clone of ChiVMV-YunN/Yuxi was constructed and was shown to be infectious in Nicotiana benthamiana. The additional 15 nt of 5′ UTR in ChiVMV-YunN/Yuxi was stable when transmitted through three generations. Experiments with modified clones showed that the additional 15 nt are essential for infection by this isolate.


Introduction
Chilli veinal mottle virus (ChiVMV) is a member of the genus Potyvirus from the family Potyviridae and was first reported in West Malaysia in 1979 [1]. It has now become prevalent among several economically important crops in Asia including chilli, tomato and tobacco [2], causing symptoms of mosaic, distortion and vein banding on the leaves [1]. The ChiVMV genome has 9.7 kb of single-stranded RNA, excluding a poly (A) tail, which encodes a polyprotein that is cleaved into 10 mature functional proteins by virus-encoded proteases [3,4].
Genetic recombination is common in potyvirus populations [5]. Known ChiVMV isolates cluster with high probability into two clades [6] and recombination between isolates appears to be a significant factor affecting their diversity [6][7][8]. Coat protein (CP) gene sequences are used to estimate genetic diversity and to identify recombination events [6]. Recombination analysis revealed that the CP gene of isolate KX236451 is likely a recombinant between Pakistani isolate KT876050 (as the major parent) and the Indian isolate JN692501 (as the minor parent) [8]. Previous work in our laboratory predicted that two Chinese and one Pakistan isolate are recombinants and that recombination contributes to the variation in the CP sequences [7]. The CP to 3 UTR region appears to be a hotspot for recombination among ChiVMV isolates [7,8]. Curiously, recombination has not been reported to be a major factor in the regions of the ChiVMV genome with the greatest overall diversity (P1, P3 and 6K2 coding regions).
Protein translation is the pivotal process in viral life cycles. Most cellular mRNAs rely on canonical mechanisms to initiate protein synthesis [9]. These mRNAs are modified at the 5 end with a methyl guanylate cap and 3 end with a poly(A) tail (a stretch of adenine nucleotides with a variable length) [10,11]. Potyviruses mainly rely on cis-acting elements in their 5 UTR to initiate the translation of their polyprotein [12]. The 5 UTRs of potyviruses can function as internal ribosomal entry sites (IRESes) without the need to scan from the 5 end of their multi-AUG UTRs [13]. The 5' UTR is responsible for conferring capindependent translation, even onto reporter mRNAs. The stable stem-loop (SL) structures of the 5 UTR of tobacco etch virus (TEV) serve as cap-independent regulatory elements (CIREs) to identify the elements responsible for its regulatory function and promote capindependent translation [14]. Therefore, the 5 UTRs of TEV and pea seedborne mosaic virus (PSbMV) RNAs are found to significantly increase gene expression [15]. Mutational analysis of the 5' UTR of potato virus Y (PVY) is conducted to find the last 55 nucleotides necessary for the enhancement, and the 5' UTR may play a very important role in the translational enhancement in plant cells [16].
In this study, we report a new recombinant ChiVMV-YunN/Yuxi (GenBank: OP404087) from Solanum nigrum L., which has a recombinant event in its P1 region. In addition, the 5 UTR of ChiVMV-YunN/Yuxi is 15 nucleotides longer than the other reported isolates and we show that these additional nucleotides are important for viral infection.

Sample Collection, De Novo Assembly and RACE
During a local virus survey in 2021, 40 samples of S. nigrum plants with virus-like symptoms were collected from Huang Caoba village in Hongta district ( Figure 1). To assess the viral species present in the viral samples, 10 samples of leaves were mixed into a pool (4 pools were obtained) and the total RNA was extracted from mixed fresh leaves using a TRIzol reagent (Invitrogen). The mRNA was purified from total RNA using poly-T oligo-attached magnetic beads. RNA integrity was checked using an Agilent 2100 Bioanalyzer (Agilent Technologies). The TruSeq RNA Sample Preparation Kit (Illumina) was used to construct cDNA libraries according to the manufacturer's instructions. The high-throughput transcriptome sequencing was performed on an Illumina NovaSeq 6000 platform with PE150 bp and a CLC Genomics Workbench 20 (QIAGEN) was used for sequencing and data analysis. The contigs were generated de novo and compared with amino acid sequences in GenBank using BLASTx.
To obtain the full-length sequence of ChiVMV, the 3 -end first strand cDNA was synthesized with M4T primers using ReverTra Ace™ qPCR RT Kit (Toyobo) according to the manufacturer's instructions (Table S1 and Figure 2A,B), and the PCR products were then amplified with M4 and 3'-RACE-F using KOD-plus-Neo (Toyobo) [17,18]. For 5 RACE, the first strand cDNA was synthesized with a gene-specific reverse primer 5'-RACE-ChiVMV-YunN-R and the adapter primer ZHM1 was ligated to cDNA/RNA duplexes using T4 RNA ligase (Takara) ( Figure S1A). The PCR product of 5 RACE was amplified with ZHM2 and 5'-RACE-R, and then cloned and sequenced [19]. To ensure the integrity and authenticity of full-length sequences, two overlapping sequence fragments were amplified with the primer pairs ChiVMV-2L-1 and ChiVMV-2L-2 ( Figure S1B).

Viral Recombination Analysis
The recombination detection program RDP5 was used to predict recombination events among all 21 full-length sequences (20 in NCBI and 1 in this study) ( Table S2). The program simultaneously uses a range of different recombination detection methods to detect recombination events within aligned sequences. These methods include the BOOTSCAN-NING method, the GENECONV method, the maximum chi-square method (MAXCHI), the CHIMAERA method, the sister-scanning method (SISCAN), the 3SEQ method, and the VisRD method [20]. Recombinant events that were identified by at least three methods and p values of less than 1 × 10 −6 were considered credible. and minor (ChiVMV-YunN/Ca) parents and the recombinant region was highlighted in pink. Multiple nucleotide sequences were aligned using MUSCLE and then analyzed using RDP5 with default parameters.

Viral Recombination Analysis
The recombination detection program RDP5 was used to predict recombination events among all 21 full-length sequences (20 in NCBI and 1 in this study) ( Table S2). The program simultaneously uses a range of different recombination detection methods to detect recombination events within aligned sequences. These methods include the BOOTSCANNING method, the GENECONV method, the maximum chi-square method (MAXCHI), the CHIMAERA method, the sister-scanning method (SISCAN), the 3SEQ method, and the VisRD method [20]. Recombinant events that were identified by at least three methods and p values of less than 1 × 10 −6 were considered credible.

Phylogenetic and Sequence Analysis
Complete genome sequences of ChiVMV were obtained from GenBank and this study (Table S2). Pairwise nucleotide sequence comparisons were performed using the SDT (Species Demarcation Tool) v1.2 program. The evolutionary history was inferred using the maximum likelihood method [21]. The best-fit nucleotide substitution model was determined to be neighbor-joining by MEGA X [22]. Evolutionary analyses were conducted in MEGA X with 1000 bootstrap replicates.  Supplementary Table S2. : Sequence determined in this study. (B) Amino acid (aa) and nucleotide (nt) sequence the identities of the 10 mature proteins and nucleotide identities of the untranslated regions (UTR) of ChiVMV-YunN/Yuxi with those of other isolates. Increasing levels of saturation of green denote high and low levels of amino acid similarity. (C) Recombination (RDP) and genetic map of ChiVMV-YunN/Yuxi showing major (ChiVMV-TaiW) and minor (ChiVMV-YunN/Ca) parents and the recombinant region was highlighted in pink. Multiple nucleotide sequences were aligned using MUSCLE and then analyzed using RDP5 with default parameters.

Phylogenetic and Sequence Analysis
Complete genome sequences of ChiVMV were obtained from GenBank and this study (Table S2). Pairwise nucleotide sequence comparisons were performed using the SDT (Species Demarcation Tool) v1.2 program. The evolutionary history was inferred using the maximum likelihood method [21]. The best-fit nucleotide substitution model was determined to be neighbor-joining by MEGA X [22]. Evolutionary analyses were conducted in MEGA X with 1000 bootstrap replicates.

Plasmid Construction and Agroinfiltration
RT-PCR was performed using KOD-plus-Neo (Toyobo) and in accordance with the manufacturer's protocol. PCR products were purified with the Gel Extraction Kit (Omega, Norcross, GA, USA). To generate infectious clones, the ClonExpress II One Step Cloning Kit (Vazyme) was used for homologous recombination. The full-length ChiVMV was amplified with a primer pair and recombined with the linearized binary vector pCB301-MD [1]. To confirm infectivity, the infectious clones were transformed into Agrobacterium tumefaciens Viruses 2023, 15, 1428 5 of 12 and inoculated as described before [1]. The mGFP tagging and mutagenesis of clones were also constructed via homologous recombination and the primer combinations were listed in Table S1 ( Figure S1D).

Virion's Purification
Leaves were homogenized in an extraction buffer (0.05 M K 2 HPO 4 ; 0.01 M Na 2 -EDTA; 1% (w/v) Na 2 SO 3 ; 5% (v/v) ethanol adjusted to pH 7.6) using 3 mL per gram of leaves. The homogenate was filtered through preboiled cheesecloth, centrifuged at 8000× g for 30 min, and the pellet discarded. Triton X-100 was added to the supernatant to a final concentration of 1% (v/v). This was stirred gently for 1 h and then centrifuged for 3 h at 90,000× g on a sucrose cushion of 20% (w/v) sucrose in an extraction buffer, filling approx. 25% of each tube. The supernatant was discarded, and the pellet was suspended in the buffer (the same as the extraction buffer but without ethanol) via overnight soaking.

Sap Inoculation and Western Blot
We cut symptomatic young leaves from the infected plants and ground them in a 1 mL phosphate buffer. We dipped segments of our forefingers into the sap and rubbed them gently over the leaves. Immediately after inoculation, we rinsed the leaves with double-distilled water. Then, we transferred the plants to the glasshouse.
Reverse transcription (RT) was performed using the ReverTra AceTM qPCR RT Master Mix (Toyobo) and a polymerase chain reaction (PCR) was performed by KOD-plus-Neo (Toyobo). RT was performed at 42 • C for 60 min with M4T followed by 72 • C for 10 min. The cycling conditions for the subsequent PCR were: 98 • C 5 min, then 32 cycles of 98 • C for 30 s, 55 • C for 30 s, 68 • C for 1 kb/min; and 68 • C for 10 min. The additional 15 nt was detected with primer pairs UTR f/r (with 15 nt) or UTR d15 f/UTR r (without 15 nt) ( Table S1).

Sequence, Phylogenetic and Recombinant Analysis of ChiVMV-YunN/Yuxi from Solanum nigrum L. in Yuxi City
Recently, ChiVMV has often been detected in solanaceous crops in Yunnan province, China. Virus-like symptoms (interveinal leaf crinkle, vein distorting and systemic mosaic) were also observed in Solanum nigrum L. This is a weed found in and around chilli fields and which is also grown as a Cd hyperaccumulator plant for remediating Cd-polluted soil [23] throughout Yuxi city, Yunnan province ( Figure 1A). The typical symptoms of 40 samples were collected from two sites in Huang Caoba village in Hongta district. To assess the viral species present in viral samples, 10 samples of leaves were mixed into a pool (4 pools were obtained) and sent for next-generation RNA-sequencing (NGS). In order to confirm the suspected presence of ChiVMV, we used primer pair Det-ChiVMV f and Det-ChiVMV r to amplify a partial fragment of the CP by RT-PCR (Table S1). Fragments with a predicted size of approximately 581 bp were obtained in 28 of the 40 samples. To confirm the infectivity of the virus, Nicotiana benthamiana plants were mechanically inoculated with sap from S. nigrum leaves ( Figure 1B). Western blot analysis confirmed the presence of ChiVMV in the systemic (non-inoculated) leaves of inoculated plants ( Figure 1C). Virions were purified and visualized via negative stain transmission electron microscopy (TEM) ( Figure 1D). Then, viral RNA was confirmed by RT-PCR and a 1153 bp sequence was obtained which had a 93.8% nt identity to ChiVMV-GD (Gen-Bank: KU987835.1). To ensure the integrity and authenticity of the full-length sequence of ChiVMV, two overlapping sequence fragments were amplified with the primer pairs ChiVMV-2L-1 and ChiVMV-2L-2 (Table S1). The RT-PCR products were expected to be sizes 6859 bp and 6674 bp, thus overlapping by 3792 bp (Figure S1A-C). The complete sequence was 9741 nt long (GenBank: OP404087), and we tentatively designated this virus as chilli veinal mottle virus isolate Yunnan Yuxi (ChiVMV-YunN/Yuxi).
The complete genomic RNA sequence of ChiVMV-YunN/Yuxi has a 5 UTR (nts 1-186) and 3 UTR (nts 9457-9741), with a single large open reading frame (ORF) encoding a polyprotein of 3089 aa residues. To investigate the phylogenetic relationships between ChiVMV-YunN/Yuxi and other ChiVMV (es), the full genome sequences of 20 ChiVMV isolates were retrieved from GenBank, and a NJ phylogenetic tree was inferred by Mega X. The isolates clustered into two groups, with ChiVMV-YunN/Yuxi in Group I (Figure 2A). ChiVMV-YunN/Yuxi had an 84.0-89.7% nucleotide identity to other Group I sequences and an 82.2-86.1% identity to isolates of Group II ( Figure 2B). Among the different genome regions, the greatest differences between isolates were found in P1 ( Figure 2B). The 5 part (5 UTR to P1) of ChiVMV-YunN/Yuxi had the highest nucleotide identity (95.7%) to the corresponding region of ChiVMV-YunN/Ca (Group II), but the 3 part (HC-Pro to 3 UTR) was most closely related (92.5% nucleotide identity) to ChiVMV-TaiW in Group I ( Figure S2). A phylogenetic analysis also showed that the 5 part of ChiVMV-YunN/Yuxi clustered into Group II, but that the 3 part clustered in Group I ( Figure S2). This suggested that ChiVMV-YunN/Yuxi might be a recombinant between Group I and Group II isolates.

ChiVMV-YunN/Yuxi Has a Longer 5 UTR Than Other Isolates That Is Stable in Subculture
Interestingly, the 5 UTR of ChiVMV-YunN/Yuxi is 15 nucleotides ('AAAAATAAAA-CAACC') longer than other reported isolates ( Figure S3). To confirm the presence of additional 15 nt in 5 UTR, virus infected-plants were collected, and RT-PCR confirmed the presence of 5 UTR, with an additional 15 nt in the systemic (non-inoculated) leaves of inoculated plants ( Figure 1E). Concurrently, an infectious clone of ChiVMV-YunN/Yuxi was constructed for further investigation. The full-length cDNA infectious clone (pChiVMV) was transformed into A. tumefaciens, which was then delivered to N. benthamiana plantlets by infiltration. Severe mosaic was detected in systemic leaves at 5 days post-infiltration ( Figure 3A). The flexuous filamentous virions were observed in new non-inoculated leaves by TEM ( Figure 3B) and Western blot confirmed that the virus had spread systemically in the inoculated plants ( Figure 3C). These results demonstrate the infectivity of the fulllength ChiVMV-YunN/Yuxi. The virus was then transmitted by sap inoculation for three generations, and all plants developed severe mosaic symptoms in their systemic leaves 4 days after inoculation ( Figure 3D). RT-PCR also confirmed that the additional 15 nt in the 5 UTR were stable during this subculture ( Figure 3E). inoculated plants ( Figure 1E). Concurrently, an infectious clone of ChiVMV-YunN/Yuxi was constructed for further investigation. The full-length cDNA infectious clone (pChiVMV) was transformed into A. tumefaciens, which was then delivered to N. benthamiana plantlets by infiltration. Severe mosaic was detected in systemic leaves at 5 days postinfiltration ( Figure 3A). The flexuous filamentous virions were observed in new non-inoculated leaves by TEM ( Figure 3B) and Western blot confirmed that the virus had spread systemically in the inoculated plants ( Figure 3C). These results demonstrate the infectivity of the full-length ChiVMV-YunN/Yuxi. The virus was then transmitted by sap inoculation for three generations, and all plants developed severe mosaic symptoms in their systemic leaves 4 days after inoculation ( Figure 3D). RT-PCR also confirmed that the additional 15 nt in the 5′ UTR were stable during this subculture ( Figure 3E).

The Additional 15 nt in the 5′ UTR Are Crucial in Viral Infection
To trace and observe infection by ChiVMV-YunN/Yuxi more conveniently, an mGFPtagged cDNA infectious clone was then constructed. The sequence encoding a NIa protease cleavage site (EGGEVTHQ/SG) was introduced between the eGFP and CP coding sequences ( Figure S1D). In order to study the biological functions of 15 nt in ChiVMV-YunN/Yuxi 5′ UTR, the vector of pChiVMVd15-GFP was constructed. This was identical to

The Additional 15 nt in the 5 UTR Are Crucial in Viral Infection
To trace and observe infection by ChiVMV-YunN/Yuxi more conveniently, an mGFPtagged cDNA infectious clone was then constructed. The sequence encoding a NIa protease cleavage site (EGGEVTHQ/SG) was introduced between the eGFP and CP coding sequences ( Figure S1D). In order to study the biological functions of 15 nt in ChiVMV-YunN/Yuxi 5 UTR, the vector of pChiVMV d15 -GFP was constructed. This was identical to pChiVMV-GFP, but lacked the 15 nt sequence. The infectious clones pChiVMV-GFP and pChiVMV d15 -GFP were transformed into A. tumefaciens and then delivered to N. benthamiana plantlets by infiltration. At 5 dpi, UV lamp examination showed GFP fluorescence in the inoculated leaves of pChiVMV-GFP infected plants. At 7 dpi, GFP fluorescence was observed in the upper non-inoculated leaves of pChiVMV-GFP infected plants, but not in those infected by pChiVMV d15 -GFP ( Figure 4A). Western blots also showed that the coat protein and GFP could be detected in the new non-inoculated leaves, but only those of pChiVMV-GFP-infected plants ( Figure 4B). pChiVMVd15-GFP were transformed into A. tumefaciens and then delivered to N. benthamiana plantlets by infiltration. At 5 dpi, UV lamp examination showed GFP fluorescence in the inoculated leaves of pChiVMV-GFP infected plants. At 7 dpi, GFP fluorescence was observed in the upper non-inoculated leaves of pChiVMV-GFP infected plants, but not in those infected by pChiVMVd15-GFP ( Figure 4A). Western blots also showed that the coat protein and GFP could be detected in the new non-inoculated leaves, but only those of pChiVMV-GFP-infected plants ( Figure 4B). To further confirm the function of the additional 15 nt and to investigate the significance of the A residues, another three mutant infectious clones were constructed ( Figure  S1D). In pChiVMVMutC-GFP, the A bases were all replaced with C, while the other clones underwent the addition or deletion of an A residue at the N-terminus (pChiVMVAdd1A-GFP and pChiVMVdelete1A-GFP, respectively). pChiVMV-GFP and the three mutant infectious clones were delivered to N. benthamiana plantlets by A. tumefaciens. At 7 dpi, GFP fluorescence was observed in the upper non-inoculated leaves of plants infected with pChiVMV-GFP and pChiVMVAdd1A-GFP ( Figure 5A). At 8 dpi, GFP fluorescence was observed in 3/3 upper non-inoculated leaves of plants infected with pChiVMV-GFP or pChiVMVAdd1A-GFP, in 1/3 leaves of those infected with pChiVMVMutC-GFP, but not in those inoculated with pChiVMVdelete1A-GFP ( Figure 5A,B). Western blots confirmed that there were significant differences in the accumulation levels of virus proteins in the order: pChiVMV-GFP > pChiVMVAdd1A-GFP > pChiVMVMutC-GFP > pChiVMVdelete1A-GFP ( Figure  5). By 12 dpi, the GFP fluorescence was observed in all the infected plants. The results show that these 15 nt of the 5′ UTR are crucial for infection by ChiVMV-YunN/Yuxi. To further confirm the function of the additional 15 nt and to investigate the significance of the A residues, another three mutant infectious clones were constructed ( Figure S1D). In pChiVMV MutC -GFP, the A bases were all replaced with C, while the other clones underwent the addition or deletion of an A residue at the N-terminus (pChiVMV Add1A -GFP and pChiVMV delete1A -GFP, respectively). pChiVMV-GFP and the three mutant infectious clones were delivered to N. benthamiana plantlets by A. tumefaciens. At 7 dpi, GFP fluorescence was observed in the upper non-inoculated leaves of plants infected with pChiVMV-GFP and pChiVMV Add1A -GFP ( Figure 5A). At 8 dpi, GFP fluorescence was observed in 3/3 upper non-inoculated leaves of plants infected with pChiVMV-GFP or pChiVMV Add1A -GFP, in 1/3 leaves of those infected with pChiVMV MutC -GFP, but not in those inoculated with pChiVMV delete1A -GFP ( Figure 5A,B). Western blots confirmed that there were significant differences in the accumulation levels of virus proteins in the order: pChiVMV-GFP > pChiVMV Add1A -GFP > pChiVMV MutC -GFP > pChiVMV delete1A -GFP ( Figure 5). By 12 dpi, the GFP fluorescence was observed in all the infected plants. The results show that these 15 nt of the 5 UTR are crucial for infection by ChiVMV-YunN/Yuxi.

Discussion
Molecular criteria are often used in the taxonomy of potyviruses. Isolates of different species typically have sequence identities of their large ORF (or, if necessary, the CP-coding region) < 76% (nt) and <82% (aa) [24]. Thresholds for other coding regions, ranging from 58% (P1 coding region) to 74-78% (in other regions), have become commonly accepted [25]. In this study, we have identified a novel recombinant ChiVMV isolate taken from S. nigrum. There are significant sequence differences among the 21 ChiVMV isolates, but the variation remains within the limits expected for isolates of the same species. The genetic variations were not distributed evenly among the different regions of the ChiVMV genome, with the greatest diversity seen in the P1, P3 and 6K2 coding regions. Recombination is important in the evolution, sequence diversity and complex genotyping system of potyviruses [26]. Earlier investigations demonstrated that the CP to 3 UTR region was a hotspot for recombination in ChiVMV isolates [7,8]. In this study, recombination events were identified in most of the genomic regions of ChiVMV, with a higher frequency in the P1 to HC-Pro and 6K2 to VPg regions (Table S3) and a significant recombination hotspot in the P1 region (3/10 events). P1 may be under lesser evolutionary constraints than the other proteins, making it a mutational hotspot in ChiVMV.
Previous studies show that the 5 UTRs of potyviruses can significantly increase gene expression in plant cells. The SL structures and last 55 nt of the 5 UTR are necessary for this enhancement [16]. In this study, the first 15 nt of ChiVMV-YunN/Yuxi RNA promoted efficient viral infection (Figures 4 and 5). However, there were no predicted significant secondary RNA structures in the first 48 nt ( Figure S4), suggesting that secondary structure is not a factor in this effect. Previous studies showed that the first 16 bases of PVY (potato virus Y) RNA have an essential function in the initiation of translation. Antisense oligonucleotide A (16-1) mediated the inhibition of translation, even when the concentration of A (16-1) was reduced to 25/1 of the transcript 5 PVY-GUS [1]. The first 15 nt of ChiVMV-YunN/Yuxi RNA appear to play a crucial role in viral infection, but the mechanism of enhancement is unclear and may play a similar role to the PVY (1-16 nt).
In the protein translation of potyviruses in general, the viral VPg, rather than the canonical 5 cap, interacts with eukaryotic translation initiation factor 4E (eIF4E) or its isoform iso 4E [eIF(iso)4E] [27]. Previous studies have shown that the ChiVMV VPg interacted with both eIF4E and eIF(iso)4E and that silencing of eIF4E and eIF(iso)4E decreased the accumulation of ChiVMV [28]. The translation of potyviruses may be stimulated by a collaboration between the 5 UTR and VPg. The cap structure at the 5 ends of mRNAs has been shown to play an important role in the initial ribosome entry and may also protect RNAs against exonuclease degradation. When the 5 PVY-GUS was capped, the translation efficiency was sixfold higher than in conditions with uncapped mRNA [29]. We next plan to assess whether the first 15 bases to help link to the VPg or canonical cap structure to promote translation.

Supplementary Materials:
The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/v15071428/s1, Figure S1: (A) Genome organization ChiVMV; (B-C) Diagram showing how the full-length sequence was constructed by overlap extension RT-PCR; (D) Diagram showing the structure of the full-length cDNA clone and mGFP-tagged cDNA clone; Figure S2: Phylogenetic analysis of 5 and 3 part of ChiVMV isolates; Figure S3: Multiple alignment analysis of 5 UTR of ChiVMV isolates; Figure S4: RNA secondery structure analysis of 5 UTR of ChiVMV isolates; Table S1: Primers used in this study; Table S2: Accession numbers of potyviruses used for phylogenetic analysis; Table S3: Summary of possible recombination events among 26 genome sequences of ChiVMV isolates used by RDP5.