Interaction of the Trans-Frame Potyvirus Protein P3N-PIPO with Host Protein PCaP1 Facilitates Potyvirus Movement

A small open reading frame (ORF), pipo, overlaps with the P3 coding region of the potyviral polyprotein ORF. Previous evidence suggested a requirement for pipo for efficient viral cell-to-cell movement. Here, we provide immunoblotting evidence that the protein PIPO is expressed as a trans-frame protein consisting of the amino-terminal half of P3 fused to PIPO (P3N-PIPO). P3N-PIPO of Turnip mosaic virus (TuMV) fused to GFP facilitates its own cell-to-cell movement. Using a yeast two-hybrid screen, co-immunoprecipitation assays, and bimolecular fluorescence complementation (BiFC) assays, we found that P3N-PIPO interacts with host protein PCaP1, a cation-binding protein that attaches to the plasma membrane via myristoylation. BiFC revealed that it is the PIPO domain of P3N-PIPO that binds PCaP1 and that myristoylation of PCaP1 is unnecessary for interaction with P3N-PIPO. In PCaP1 knockout mutants (pcap1) of Arabidopsis, accumulation of TuMV harboring a GFP gene (TuMV-GFP) was drastically reduced relative to the virus level in wild-type plants, only small localized spots of GFP were visible, and the plants showed few symptoms. In contrast, TuMV-GFP infection in wild-type Arabidopsis yielded large green fluorescent patches, and caused severe stunting. However, viral RNA accumulated to high level in protoplasts from pcap1 plants indicating that PCaP1 is not required for TuMV RNA synthesis. In contrast to TuMV, the tobamovirus Oilseed rape mosaic virus did not require PCaP1 to infect Arabidopsis plants. We conclude that potyviral P3N-PIPO interacts specifically with the host plasma membrane protein PCaP1 to participate in cell-to-cell movement. We speculate that PCaP1 links a complex of viral proteins and genomic RNA to the plasma membrane by binding P3N-PIPO, enabling localization to the plasmodesmata and cell-to-cell movement. The PCaP1 knockout may contribute to a new strategy for recessive resistance to potyviruses.     

Quantitative and Qualitative Involvement of P3N-PIPO in Overcoming Recessive Resistance against Clover Yellow Vein Virus in Pea Carrying the cyv1 Gene

In pea carrying cyv1, a recessive gene for resistance to Clover yellow vein virus (ClYVV), ClYVV isolate Cl-no30 was restricted to the initially infected cells, whereas isolate 90-1 Br2 overcame this resistance. We mapped the region responsible for breaking of cyv1-mediated resistance by examining infection of cyv1 pea with chimeric viruses constructed from parts of Cl-no30 and 90-1 Br2. The breaking of resistance was attributed to the P3 cistron, which is known to produce two proteins: P3, from the main open reading frame (ORF), and P3N-PIPO, which has the N-terminal part of P3 fused to amino acids encoded by a small open reading frame (ORF) called PIPO in the +2 reading frame. We introduced point mutations that were synonymous with respect to the P3 protein but nonsynonymous with respect to the P3N-PIPO protein, and vice versa, into the chimeric viruses. Infection of plants with these mutant viruses revealed that both P3 and P3N-PIPO were involved in overcoming cyv1-mediated resistance. Moreover, P3N-PIPO quantitatively affected the virulence of Cl-no30 in cyv1 pea. Additional expression in trans of the P3N-PIPO derived from Cl-no30, using White clover mosaic virus as a vector, enabled Cl-no30 to move to systemic leaves in cyv1 pea. Susceptible pea plants infected with chimeric ClYVV possessing the P3 cistron of 90-1 Br2, and which were therefore virulent toward cyv1 pea, accumulated more P3N-PIPO than did those infected with Cl-no30, suggesting that the higher level of P3N-PIPO in infected cells contributed to the breaking of resistance by 90-1 Br2. This is the first report showing that P3N-PIPO is a virulence determinant in plants resistant to a potyvirus.     

ANK, a host cytoplasmic receptor for the Tobacco mosaic virus cell-to-cell movement protein, facilitates intercellular transport through plasmodesmata

Plasmodesma (PD) is a channel structure that spans the cell wall and provides symplastic connection between adjacent cells. Various macromolecules are known to be transported through PD in a highly regulated manner, and plant viruses utilize their movement proteins (MPs) to gate the PD to spread cell-to-cell. The mechanism by which MP modifies PD to enable intercelluar traffic remains obscure, due to the lack of knowledge about the host factors that mediate the process. Here, we describe the functional interaction between Tobacco mosaic virus (TMV) MP and a plant factor, an ankyrin repeat containing protein (ANK), during the viral cell-to-cell movement. We utilized a reverse genetics approach to gain insight into the possible involvement of ANK in viral movement. To this end, ANK overexpressor and suppressor lines were generated, and the movement of MP was tested. MP movement was facilitated in the ANK-overexpressing plants, and reduced in the ANK-suppressing plants, demonstrating that ANK is a host factor that facilitates MP cell-to-cell movement. Also, the TMV local infection was largely delayed in the ANK-suppressing lines, while enhanced in the ANK-overexpressing lines, showing that ANK is crucially involved in the infection process. Importantly, MP interacted with ANK at PD. Finally, simultaneous expression of MP and ANK markedly decreased the PD levels of callose, β-1,3-glucan, which is known to act as a molecular sphincter for PD. Thus, the MP-ANK interaction results in the downregulation of callose and increased cell-to-cell movement of the viral protein. These findings suggest that ANK represents a host cellular receptor exploited by MP to aid viral movement by gating PD through relaxation of their callose sphincters.     

The actin cytoskeleton is involved in the regulation of the plasmodesmal size exclusion limit

Plasmodesmata (PD) are the communication channels which allow the trafficking of macromolecules between neighboring cells. Such cell-to-cell movement of macromolecules is regulated during plant growth and development; however, little is known about the regulation mechanism of PD size exclusion limit (SEL). Plant viral movement proteins (MPs) enhance the invasion of viruses from cell to cell by increasing the SEL of the PD and are therefore a powerful means for the study of the plasmodesmal regulation mechanisms. In a recent study, we reported that the actin cytoskeleton is involved in the increase of the PD SEL induced by MPs. Microinjection experiments demonstrated that actin depolymerization was required for the Cucumber mosaic virus (CMV) MP-induced increase in the PD SEL. In vitro experiments showed that CMV MP severs actin filaments (F-actin). Furthermore, through the analyses of two CMV MP mutants, we demonstrated that the F-actin severing ability of CMV MP was required to increase the PD SEL. These results are similar to what has been found in Tobacco mosaic virus MP. Thus, our data suggest that actin dynamics may participate in the regulations of the PD SEL.Key words: plasmodesmata, size exclusion limit, movement protein, actin filaments, F-actin severing     

Isolation of an Arabidopsis thaliana Mutant in Which the Multiplication of both Cucumber Mosaic Virus and Turnip Crinkle Virus Is Affected

During the systemic infection of plants by viruses, host factors play an important role in supporting virus multiplication. To identify and characterize the host factors involved in this process, we isolated an Arabidopsis thaliana mutant named RB663, in which accumulation of the coat protein (CP) of cucumber mosaic virus (CMV) in upper uninoculated leaves was delayed. Genetic analyses suggested that the phenotype of delayed accumulation of CMV CP in RB663 plants was controlled by a monogenic, recessive mutation designated cum2-1, which is located on chromosome III and is distinct from the previously characterized cum1 mutation. Multiplication of CMV was delayed in inoculated leaves of RB663 plants, whereas the multiplication in RB663 protoplasts was similar to that in wild-type protoplasts. This suggests that the cum2-1 mutation affects the cell-to-cell movement of CMV rather than CMV replication within a single cell. In RB663 plants, the multiplication of turnip crinkle virus (TCV) was also delayed but that of tobacco mosaic virus was not affected. As observed with CMV, the multiplication of TCV was normal in protoplasts and delayed in inoculated leaves of RB663 plants compared to that in wild-type plants. Furthermore, the phenotype of delayed TCV multiplication cosegregated with the cum2-1 mutation as far as we examined. Therefore, the cum2-1 mutation is likely to affect the cell-to-cell movement of both CMV and TCV, implying a common aspect to the mechanisms of cell-to-cell movement in these two distinct viruses.     

DEVELOPMENTALLY REGULATED PLASMA MEMBRANE PROTEIN of Nicotiana benthamiana Contributes to Potyvirus Movement and Transports to Plasmodesmata via the Early Secretory Pathway and the Actomyosin System

The intercellular movement of plant viruses requires both viral and host proteins. Previous studies have demonstrated that the frame-shift protein P3N-PIPO (for the protein encoded by the open reading frame [ORF] containing 5′-terminus of P3 and a +2 frame-shift ORF called Pretty Interesting Potyviridae ORF and embedded in the P3) and CYLINDRICAL INCLUSION (CI) proteins were required for potyvirus cell-to-cell movement. Here, we provide genetic evidence showing that a Tobacco vein banding mosaic virus (TVBMV; genus Potyvirus) mutant carrying a truncated PIPO domain of 58 amino acid residues could move between cells and induce systemic infection in Nicotiana benthamiana plants; mutants carrying a PIPO domain of seven, 20, or 43 amino acid residues failed to move between cells and cause systemic infection in this host plant. Interestingly, the movement-defective mutants produced progeny that eliminated the previously introduced stop codons and thus restored their systemic movement ability. We also present evidence showing that a developmentally regulated plasma membrane protein of N. benthamiana (referred to as NbDREPP) interacted with both P3N-PIPO and CI of the movement-competent TVBMV. The knockdown of NbDREPP gene expression in N. benthamiana impeded the cell-to-cell movement of TVBMV. NbDREPP was shown to colocalize with TVBMV P3N-PIPO and CI at plasmodesmata (PD) and traffic to PD via the early secretory pathway and the actomyosin motility system. We also show that myosin XI-2 is specially required for transporting NbDREPP to PD. In conclusion, NbDREPP is a key host protein within the early secretory pathway and the actomyosin motility system that interacts with two movement proteins and influences virus movement.The movement of viruses in plants can be divided into three stages: intracellular, intercellular, and long-distance movement (Nelson and Citovsky, 2005; Benitez-Alfonso et al., 2010). Plasmodesmata (PD) are plasma membrane-mediated channels in cell walls that control the intercellular trafficking of micromolecules and macromolecules, including plant viruses (Boevink and Oparka, 2005; Lucas et al., 2009). Plant viruses encode movement proteins (MPs) that can regulate the size exclusion limit (SEL) of PD and mediate virus trafficking between cells (Lucas, 2006; Raffaele et al., 2009; Amari et al., 2010; Ueki et al., 2010). Based on the functions of MPs during virus movement, the viral MPs are divided into three major groups. The first group of MPs is represented by the 30-kD protein of Tobacco mosaic virus (TMV). The 30-kD proteins can interact with single-stranded RNAs and transport viral ribonucleoprotein complexes to cell walls, where they modify the SEL of PD to allow viruses to traverse the cell walls (Olesinski et al., 1996; Tzfira et al., 2000; Kawakami et al., 2004). The second group of MPs is known to form tubular structures that extend across the PD and allow virus to traverse. Viruses that encode this group of MPs include Cowpea mosaic virus, Grapevine fan leaf virus (GFLV), Cauliflower mosaic virus, and Tomato spotted wilt virus (Ritzenthaler and Hofmann, 2007; Amari et al., 2011). The third group of MPs is known as triple gene block proteins (TGBps), encoded by overlapping triple gene blocks. The three TGBps (TGBp1, TGBp2, and TGBp3) function coordinately to transport viral genomes to and through PD (Verchot-Lubicz, 2005; Jackson et al., 2009; Lim et al., 2009; Tilsner et al., 2013). Viruses that encode TGBps belong to the genera Potexvirus, Hordeivirus, and Pomovirus (Verchot-Lubicz et al., 2010). Potyviruses are different from the above viruses and lack a dedicated MP. To date, multiple potyviral proteins, including COAT PROTEIN, CYLINDRICAL INCLUSION (CI), HELPER COMPONENT PROTEINASE (HC-Pro), and VIRAL GENOME-LINKED PROTEIN, have been shown to function in the cell-to-cell movement of potyviruses (Nicolas et al., 1997; Rojas et al., 1997; Carrington et al., 1998; Wei et al., 2010).Viruses of Potyvirus (family Potyviridae), the largest genus of plant-infecting viruses, cause great economic losses to world agriculture production (Fauquet et al., 2005). The potyviral genome is a positive sense, single-stranded RNA of approximately 10 kb in length. It contains a large open reading frame (ORF) encoding a polyprotein that is later processed into 10 mature proteins by three virus-encoded proteinases (Riechmann et al., 1992; Fauquet et al., 2005). A +2 frame-shift Pretty Interesting Potyviridae (PIPO) ORF that is embedded within the P3 ORF was recently identified and proposed to produce a P3N-PIPO (for the protein encoded by 5′-terminus of P3 and frame-shift PIPO) fusion (Chung et al., 2008; Vijayapalani et al., 2012). The P3N-PIPOs of Turnip mosaic virus (TuMV) and Tobacco etch virus were previously shown to localize at PD, interact with CI in planta, and transport CI to PD in a CI:P3N-PIPO ratio-dependent manner (Wei et al., 2010). Soybean mosaic virus with a mutant PIPO domain failed to cause systemic infection in its host plant (Wen and Hajimorad, 2010). Therefore, the potyvirus P3N-PIPO has been suggested as the classical MP (Tilsner and Oparka, 2012; Vijayapalani et al., 2012).Viruses recruit host factors for their movement in plants (Chen et al., 2000; Raffaele et al., 2009; Amari et al., 2010; Ueki et al., 2010). Compared with the progresses on viral MP characterization, identifications of MP-interacting host proteins are much behind (Chen et al., 2000; Oparka, 2004; Raffaele et al., 2009; Amari et al., 2010). To date, about 20 host proteins have been identified to interact with specific viral MPs (Pallas and García, 2011). For example, the pectin methylesterase interacted with TMV MP, increased the SEL of PD, and facilitated TMV movement between cells (Chen et al., 2000); an ankyrin repeat-containing protein (ANK) interacted with TMV MP at PD, down-regulated callose formation, and aided viral movement (Ueki et al., 2010); the Arabidopsis (Arabidopsis thaliana) PLASMODESMATA-LOCALIZED PROTEIN1 (AtPDLP1) was reported to interact with GFLV MP and mediate tubule assembly during GFLV cell-to-cell movement in plants (Amari et al., 2010, 2011). TuMV P3N-PIPO was shown to interact with AtPCaP1, a plasma membrane cation-binding protein of Arabidopsis, and colocalize with this host protein at the PD. Knockout of AtPCaP1 expression resulted in a significant reduction of TuMV infection in Arabidopsis (Vijayapalani et al., 2012).Many viral MPs have been shown to traffic within plant cells via the early secretory pathway and/or along the actin filaments or microtubules. For example, the early secretory pathway and microtubules were required for GFLV MP trafficking to PD (Laporte et al., 2003). TuMV P3N-PIPO and CI were reported to utilize the early secretory pathway rather than the actomyosin motility system for their trafficking to PD (Wei et al., 2010). Several plant myosin motor proteins have been reported to participate in virus intracellular movement (Wei and Wang, 2008; Harries et al., 2010). Myosins VIII-1, VIII-2, and VIII-B were shown to transport a HEAT SHOCK PROTEIN70 homolog of Beet yellows virus to PD (Avisar et al., 2008a), but only myosin VIII-1 was needed for the nonstructural protein encoded by viral complementary strand of RNA4 (NSvc4) of Rice stripe virus traffic to PD (Yuan et al., 2011). A more recent study has indicated that both the secretory pathway and myosins XI-2 and XI-K were required for TuMV cell-to-cell movement (Agbeci et al., 2013). However, it remains largely unknown how the MP-interacting host factor(s) reach their target sites in cells.Tobacco vein banding mosaic virus (TVBMV) is a distinct potyvirus mainly infecting solanaceous crops (Tian et al., 2007; Yu et al., 2007; Zhang et al., 2011). In this article, we provide evidence showing the length requirements of the PIPO domains for its function in mediating TVBMV movement and the restoration of the movement-defective TVBMV mutants. We also show the interactions between TVBMV P3N-PIPO and CI and NbDREPP, a developmentally regulated plasma membrane protein in Nicotiana benthamiana, and the route by which NbDREPP traffics to PD. Silencing of NbDREPP expression in N. benthamiana significantly impeded the cell-to-cell movement of TVBMV.     

Reduced levels of class 1 reversibly glycosylated polypeptide increase intercellular transport via plasmodesmata

Maize and Arabidopsis thaliana class 1 reversibly glycosylated polypeptides (^C1RGPs) are plasmodesmata-associated proteins. Previously, overexpression of Arabidopsis ^C1RGP AtRGP2 in Nicotiana tabacum was shown to reduce intercellular transport of photoassimilate, resulting in stunted, chlorotic plants, and inhibition of local cell-to-cell spread of tobacco mosaic virus (TMV). Here, we used virus induced gene silencing to examine the effects of reduced levels of ^C1RGPs in Nicotiana benthamiana. Silenced plants show wild-type growth and development. Intercellular transport in silenced plants was probed using fluorescently labeled TMV and its movement protein, P30. P30 shows increased cell-to-cell movement and TMV exhibited accelerated systemic spread compared with control plants. These results support the hypothesis that ^C1RGPs act to regulate intercellular transport via plasmodesmata.     

Cell-to-cell movement of potato potexvirus X is dependent on suppression of RNA silencing

RNA silencing in transgenic and virus-infected plants involves a mobile silencing signal that can move cell-to-cell and systemically through the plant. It is thought that this signal can influence long-distance movement of viruses because protein suppressors of silencing encoded in viral genomes are required for long-distance virus movement. However, until now, it was not known whether the mobile signal could also influence short-range virus movement between cells. Here, through random mutation analysis of the Potato Potexvirus X (PVX) silencing suppressor P25, we provide evidence that it does. All mutants that were defective for silencing suppression were also non-functional in viral cell-to-cell movement. However, we identified mutant P25 proteins that were functional as silencing suppressors but not as movement proteins and we conclude that suppression of silencing is not sufficient to allow virus movement between cells: there must be a second P25 function that is independent of silencing but also required for cell-to-cell movement. Consistent with this hypothesis, we identified two classes of suppressor-inactive P25 mutants. One class of these mutants is proposed to be functional for the accessory function because their failure to support PVX movement could be complemented by heterologous suppressors of silencing. The second class of P25 mutants is considered defective for both the suppressor and second functions because the heterologous silencing suppressors did not restore virus movement. It is possible, based on analyses of short interfering RNA accumulation, that P25 suppresses silencing by interfering with either assembly or function of the effector complexes of RNA silencing.     

The ER-Membrane Transport System Is Critical for Intercellular Trafficking of the NSm Movement Protein and Tomato Spotted Wilt Tospovirus

Plant viruses move through plasmodesmata to infect new cells. The plant endoplasmic reticulum (ER) is interconnected among cells via the ER desmotubule in the plasmodesma across the cell wall, forming a continuous ER network throughout the entire plant. This ER continuity is unique to plants and has been postulated to serve as a platform for the intercellular trafficking of macromolecules. In the present study, the contribution of the plant ER membrane transport system to the intercellular trafficking of the NSm movement protein and Tomato spotted wilt tospovirus (TSWV) is investigated. We showed that TSWV NSm is physically associated with the ER membrane in Nicotiana benthamiana plants. An NSm-GFP fusion protein transiently expressed in single leaf cells was trafficked into neighboring cells. Mutations in NSm that impaired its association with the ER or caused its mis-localization to other subcellular sites inhibited cell-to-cell trafficking. Pharmacological disruption of the ER network severely inhibited NSm-GFP trafficking but not GFP diffusion. In the Arabidopsis thaliana mutant rhd3 with an impaired ER network, NSm-GFP trafficking was significantly reduced, whereas GFP diffusion was not affected. We also showed that the ER-to-Golgi secretion pathway and the cytoskeleton transport systems were not involved in the intercellular trafficking of TSWV NSm. Importantly, TSWV cell-to-cell spread was delayed in the ER-defective rhd3 mutant, and this reduced viral infection was not due to reduced replication. On the basis of robust biochemical, cellular and genetic analysis, we established that the ER membrane transport system serves as an important direct route for intercellular trafficking of NSm and TSWV.     

Cucumber Mosaic Virus Movement Protein Severs Actin Filaments to Increase the Plasmodesmal Size Exclusion Limit in Tobacco

Plant viral movement proteins (MPs) enable viruses to pass through cell walls by increasing the size exclusion limit (SEL) of plasmodesmata (PD). Here, we report that the ability of Cucumber mosaic virus (CMV) MP to increase the SEL of the PD could be inhibited by treatment with the actin filament (F-actin)–stabilizing agent phalloidin but not by treatment with the F-actin–destabilizing agent latrunculin A. In vitro studies showed that CMV MP bound globular and F-actin, inhibited actin polymerization, severed F-actin, and participated in plus end capping of F-actin. Analyses of two CMV MP mutants, one with and one without F-actin severing activities, demonstrated that the F-actin severing ability was required to increase the PD SEL. Furthermore, the Tobacco mosaic virus MP also exhibited F-actin severing activity, and its ability to increase the PD SEL was inhibited by treatment with phalloidin. Our data provide evidence to support the hypothesis that F-actin severing is required for MP-induced increase in the SEL of PD. This may have broad implications in the study of the mechanisms of actin dynamics that regulate cell-to-cell transport of viral and endogenous proteins.     

Identification and study of tobacco mosaic virus movement function by complementation tests

The phenomenon of trans-complementation of cell-to-cell movement between plant positive-strand RNA viruses is discussed with an emphasis on tobamoviruses. Attention is focused on complementation between tobamoviruses (coding for a single movement protein, MP) and two groups of viruses that contain the triple block of MP genes and require four (potato virus X) or three (barley stripe mosaic virus) proteins for cell-to-cell movement. The highlights of complementation data obtained by different experimental approaches are given, including (i) double infections with movement-deficient (dependent) and helper viruses; (ii) infections with recombinant viral genomes bearing a heterologous MP gene; (iii) complementation of a movement-deficient virus in transgenic plants expressing the MP of a helper virus; and (iv) co-bombardment of plant tissues with the cDNAs of a movement-dependent virus genome and the MP gene of a helper virus.     

Aluminum-induced 1-->3-beta-D-glucan inhibits cell-to-cell trafficking of molecules through plasmodesmata. A new mechanism of aluminum toxicity in plants

Symplastic intercellular transport in plants is achieved by plasmodesmata (PD). These cytoplasmic channels are well known to interconnect plant cells to facilitate intercellular movement of water, nutrients, and signaling molecules including hormones. However, it is not known whether Al may affect this cell-to-cell transport process, which is a critical feature for roots as organs of nutrient/water uptake. We have microinjected the dye lucifer yellow carbohydrazide into peripheral root cells of an Al-sensitive wheat (Triticum aestivum cv Scout 66) either before or after Al treatment and followed the cell-to-cell dye-coupling through PD. Here we show that the Al-induced root growth inhibition is closely associated with the Al-induced blockage of cell-to-cell dye coupling. Immunofluorescence combined with immuno-electron microscopic techniques using monoclonal antibodies against 1-->3-beta-D-glucan (callose) revealed circumstantial evidence that Al-induced callose deposition at PD may responsible for this blockage of symplastic transport. Use of 2-deoxy-D-glucose, a callose synthesis inhibitor, allowed us to demonstrate that a reduction in callose particles correlated well with the improved dye-coupling and reduced root growth inhibition. While assessing the tissue specificity of this Al effect, comparable responses were obtained from the dye-coupling pattern in tobacco (Nicotiana tabacum) mesophyll cells. Analyses of the Al-induced expression of PD-associated proteins, such as calreticulin and unconventional myosin VIII, showed enhanced fluorescence and co-localizations with callose deposits. These results suggest that Al-signal mediated localized alterations to calcium homeostasis may drive callose formation and PD closure. Our data demonstrate that extracellular Al-induced callose deposition at PD could effectively block symplastic transport and communication in higher plants.     

The conserved aromatic residue W122 is a determinant of potyviral coat protein stability,replication, and cell-to-cell movement in plants

Coat proteins (CPs) play critical roles in potyvirus cell-to-cell movement. However, the underlying mechanism controlling them remains unclear. Here, we show that substitutions of alanine, glutamic acid, or lysine for the conserved residue tryptophan at position 122 (W¹²²) in tobacco vein banding mosaic virus (TVBMV) CP abolished virus cell-to-cell movement in Nicotiana benthamiana plants. In agroinfiltrated N. benthamiana leaf patches, both the CP and RNA accumulation levels of three W¹²² mutant viruses were significantly reduced compared with those of wild-type TVBMV, and CP accumulated to a low level similar to that of a replication-deficient mutant. The results of polyprotein transient expression experiments indicated that CP instability was responsible for the significantly low CP accumulation levels of the three W¹²² mutant viruses. The substitution of W¹²² did not affect CP plasmodesmata localization or virus particle formation; however, the substitution significantly reduced the number of virus particles. The wild-type TVBMV CP could complement the reduced replication and abolished cell-to-cell movement of the mutant viruses. When the codon for W¹²² was mutated to that for a different aromatic residue, phenylalanine or tyrosine, the resultant mutant viruses moved systemically and accumulated up to 80% of the wild-type TVBMV level. Similar results were obtained for the corresponding amino acids of W¹²² in the watermelon mosaic virus and potato virus Y CPs. Therefore, we conclude that the aromatic ring in W¹²² in the core domain of the potyviral CP is critical for cell-to-cell movement through the effects on CP stability and viral replication.     

Role of the alfalfa mosaic virus movement protein and coat protein in virus transport

The movement protein (MP) and coat protein (CP) encoded by Alfalfa mosaic virus (AMV) RNA 3 are both required for virus transport. RNA 3 vectors that expressed nonfused green fluorescent protein (GFP), MP:GPF fusions, or GFP:CP fusions were used to study the functioning of mutant MP and CP in protoplasts and plants. C-terminal deletions of up to 21 amino acids did not interfere with the function of the CP in cell-to-cell movement, although some of these mutations interfered with virion assembly. Deletion of the N-terminal 11 or C-terminal 45 amino acids did not interfere with the ability of MP to assemble into tubular structures on the protoplast surface. Additionally, N- or C-terminal deletions disrupted tubule formation. A GFP:CP fusion was targeted specifically into tubules consisting of a wild-type MP. All MP deletion mutants that showed cell-to-cell and systemic movement in plants were able to form tubular structures on the surface of protoplasts. Brome mosaic virus (BMV) MP did not support AMV transport. When the C-terminal 48 amino acids were replaced by the C-terminal 44 amino acids of the AMV MP, however, the BMV/AMV chimeric protein permitted wild-type levels of AMV transport. Apparently, the C terminus of the AMV MP, although dispensable for cell-to-cell movement, confers specificity to the transport process.     

Long-distance movement factor: a transport function of the potyvirus helper component proteinase.

Transport of viruses from cell to cell in plants typically involves one or more viral proteins that supply dedicated movement functions. Transport from leaf to leaf through phloem, or long-distance transport, is a poorly understood process with requirements differing from those of cell-to-cell movement. Through genetic analysis of tobacco etch virus (TEV; potyvirus group), a novel long-distance movement factor was identified that facilitates vascular-associated movement in tobacco. A mutation in the central region of the helper component proteinase (HC-Pro), a TEV-encoded protein with previously described activities in aphid-mediated transmission and polyprotein processing, inactivated long-distance movement. This mutant virus exhibited only minor defects in genome amplification and cell-to-cell movement functions. In situ histochemical analysis revealed that the mutant was capable of infecting mesophyll, bundle sheath, and phloem cells within inoculated leaves, suggesting that the long-distance movement block was associated with entry into or exit from sieve elements. The long-distance movement defect was specifically complemented by HC-Pro supplied in trans by a transgenic host. The data indicate that HC-Pro functions in one or more steps unique to long-distance transport.     

Genetic evidence for an essential role for potyvirus CI protein in cell‐to‐cell movement

The potyvirus cylindrical inclusion (CI) protein, an RNA helicase required for genome replication, was analyzed genetically using alanine-scanning mutagenesis. Thirty-one mutations were introduced into the CI protein coding region of modified tobacco etch virus (TEV) genomes expressing either β-glucuronidase or green fluorescent protein reporters. Twelve of the mutants were replication-defective in protoplast inoculation assays. Among the 19 replication-competent mutants, several possessed cell-to-cell or long-distance movement defects in tobacco plants. Two mutants, AS1 and AS8, were restricted to single cells in inoculated leaves despite genome amplification levels that were equivalent to that of parental virus. Other mutants, such as AS9 and AS14, were able to move cell to cell slowly but were debilitated in long-distance movement. These data provide genetic evidence for a direct role of CI protein in potyvirus intercellular movement, and for distinct roles of the CI protein in genome replication and movement. In combination with high-resolution ultrastructural analyzes and previous genetic data, these results support a model in which CI protein interacts directly with plasmodesmata and capsid protein-containing ribonucleoprotein complexes to facilitate potyvirus cell-to-cell movement.     

Estimation of the Size of Genetic Bottlenecks in Cell-to-Cell Movement of Soil-Borne Wheat Mosaic Virus and the Possible Role of the Bottlenecks in Speeding Up Selection of Variations in trans-Acting Genes or Elements

Genetic bottlenecks facilitate the fixation and extinction of variants in populations, and viral populations are no exception to this theory. To examine the existence of genetic bottlenecks in cell-to-cell movement of plant RNA viruses, we prepared constructs for Soil-borne wheat mosaic virus RNA2 vectors carrying two different fluorescent proteins, yellow fluorescent protein (YFP) and cyan fluorescent protein (CFP). Coinoculation of host plant leaves with the two RNA2 vectors and the wild-type RNA1 showed separation of the two vector RNA2s, mostly within seven to nine cell-to-cell movements from individual initially coinfected cells. Our statistical analysis showed that the number of viral RNA genomes establishing infection in adjacent cells after the first cell-to-cell movement from an initially infected cell was 5.97 ± 0.22 on average and 5.02 ± 0.29 after the second cell-to-cell movement. These results indicate that plant RNA viruses may generally face narrow genetic bottlenecks in every cell-to-cell movement. Furthermore, our model suggests that, rather than suffering from fitness losses caused by the bottlenecks, the plant RNA viruses are utilizing the repeated genetic bottlenecks as an essential element of rapid selection of their adaptive variants in trans-acting genes or elements to respond to host shifting and changes in the growth conditions of the hosts.Plant RNA viruses change their genomes so rapidly that variant viruses with altered biological properties are often found after prolonged growth of infected plants or after serial mechanical inoculations (26, 33). Furthermore, inoculation of less-fit artificial mutants produces revertants or pseudo-revertants even after short infection times (12, 14). The rapid evolution of plant RNA viral genomes is achieved not only by high mutation rates due to error-prone replication by the nonproofreading viral RNA-dependent RNA polymerase (19) but also by rapid selection and strong genetic drift. Generally, narrow genetic bottlenecks facilitate the fixation and extinction of variants in populations (15), and viral populations are no exception to this theory.Plant RNA viruses are known to face many narrow genetic bottlenecks during their life cycles (23). The life cycles of most plant RNA viruses are as follows: After replicating in cells, viruses move from cell to cell through plasmodesmata, which connect the cytoplasms of adjacent cells separated by cell walls in plant tissue. Following the establishment of infection in cells and cell-to-cell movements, the viruses expand their infected regions, spreading to the veins and moving through the vascular system and infecting the plant systemically. Some plant RNA viruses are transmitted through the seeds or via mechanical injuries, but most are transmitted from plant to plant by biological vectors such as insects, nematodes, and fungi. Previous studies have found that genetic bottlenecks occur during the transfer from lower leaves to upper leaves in systemic infections of Wheat streak mosaic virus (WSMV) (11), Tobacco mosaic virus (TMV) (24), and Cucumber mosaic virus (CMV) (18) and during the transfer from one tiller to another tiller of WSMV (11). Vector transmissions were also shown to act as genetic bottlenecks for WSMV (11), CMV (1, 3), and Potato virus Y (PVY) (20). With the exception of PVY, the typical method for detecting genetic bottlenecks has been to observe the spatial separation of closely related strains or artificial synonymous mutants inoculated as mixed populations: the narrower the genetic bottleneck, the more frequently the spatial separation should be observed. Using this idea with mathematical analyses, WSMV was estimated to infect a new tiller starting with four genomes (9), TMV was estimated to infect the upper leaves starting with 10 genomes (24), and CMV was estimated to infect a new plant starting with one to two particles after aphid transmission (3). Studies of PVY using sets of host plant cultivars with or without resistance genes and mixed strains of viruses with or without resistance-breaking abilities also estimated the number of virus particles transmitted by an aphid vector to be 0.5 to 3.2 on average (20).However, genetic bottlenecks in cell-to-cell movement of viruses have not been well characterized, although these occurrences are likely (11) and have been expected to be important for understanding the life cycle and population dynamics of plant RNA viruses. The size of genetic bottlenecks in cell-to-cell movement can be referred to as “multiplicity of infection (MOI) in plant tissue colonization,” and only a recent study showing that the estimated MOI of TMV is between 6 and 1 to 2 (10) indicates the occurrence and the size of genetic bottlenecks in cell-to-cell movement of a plant RNA virus. In this paper, we also show the occurrence of narrow genetic bottlenecks during cell-to-cell movement of a plant RNA virus, Soil-borne wheat mosaic virus (SBWMV, type species of the genus Furovirus), by observing the spatial separation of RNA2 vectors carrying different fluorescent proteins, yellow fluorescent protein (YFP) and cyan fluorescent protein (CFP). Both of the fluorescent proteins were expressed as fusion proteins to the N-terminal nuclear localization signal (NLS) peptide from Simian virus 40 (SV40) large T antigen, which enabled us to observe and count the infected cells accurately using nuclear fluorescence. Numerical data were analyzed to estimate the size of bottlenecks. We also carried out a simulation to show that, due to the narrow genetic bottlenecks, rapid selection occurs even on trans-acting elements in plant RNA virus genomes, overcoming the negative effect of complementation among adaptive and defective genomes in each intracellular population. We discuss the possible roles of the bottlenecks in the life cycle and evolution mechanisms of plant RNA viruses.