Cellular Targets of Functional and Dysfunctional Mutants of Tobacco Mosaic Virus Movement Protein Fused to Green Fluorescent Protein

doi:10.1128/JVI.74.23.11339-11346.2000

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Journal of Virology, December 2000, p. 11339-11346, Vol. 74, No. 23
0022-538X/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Cellular Targets of Functional and Dysfunctional Mutants of Tobacco Mosaic Virus Movement Protein Fused to Green Fluorescent Protein

Vitaly Boyko, Jessica van der Laak, Jacqueline Ferralli, Elena Suslova, Myoung-Ok Kwon, and Manfred Heinlein^*

Friedrich Miescher Institute, CH-4058 Basel, Switzerland

Received 3 July 2000/Accepted 30 August 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Intercellular transport of tobacco mosaic virus (TMV) RNA involves the accumulation of virus-encoded movement protein (MP)in plasmodesmata (Pd), in endoplasmic reticulum (ER)-derived inclusionbodies, and on microtubules. The functional significance of theseinteractions in viral RNA (vRNA) movement was tested in plantaand in protoplasts with TMV derivatives expressing N- and C-terminaldeletion mutants of MP fused to the green fluorescent protein.Deletion of 55 amino acids from the C terminus of MP did not interferewith the vRNA transport function of MP:GFP but abolished its accumulationin inclusion bodies, indicating that accumulation of MP at theseER-derived sites is not a requirement for function in vRNA intercellularmovement. Deletion of 66 amino acids from the C terminus of MPinactivated the protein, and viral infection occurred only uponcomplementation in plants transgenic for MP. The functional deficiencyof the mutant protein correlated with its inability to associatewith microtubules and, independently, with its absence from Pdat the leading edge of infection. Inactivation of MP by N-terminaldeletions was correlated with the inability of the protein totarget Pd throughout the infection site, whereas its associationswith microtubules and inclusion bodies were unaffected. The observationssupport a role of MP-interacting microtubules in TMV RNA movementand indicate that MP targets microtubules and Pd by independentmechanisms. Moreover, accumulation of MP in Pd late in infectionis insufficient to support viral movement, confirming that intercellulartransport of vRNA relies on the presence of MP in Pd at the leadingedge ofinfection.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Intercellular communication in plants occurs through plasmodesmata (Pd), gatable channels in the cell wall that provide symplasticcontinuity between adjacent cells. Although the size exclusionlimit (SEL) of Pd normally restricts diffusion for molecules largerthan 1 kDa (22, 43, 45, 53), accumulating evidence indicatesthat Pd are dynamic and able to increase the SEL to allow thepassage of macromolecules such as proteins, RNA, and protein-RNAcomplexes (13, 15, 18, 21, 29, 32, 33, 36, 47,53). Most compelling evidence for macromolecular traffickingthrough Pd is provided by viruses which exploit Pd to move theirgenomes from cell to cell and to spread infection (18, 33).The spread of viruses represents an excellent model to study themechanism by which nucleic acid molecules are targeted to Pd.Their trafficking depends on virus-encoded movement proteins (MPs)(12) which can be used to directly probe the intercellular communicationmachinery.

Much of what is known about MPs is derived from studies on the MP of tobacco mosaic virus (TMV). Consistent with its functionin viral movement, this protein is targeted to Pd and increasestheir SEL (37, 53). The protein also binds single-strandednucleic acids in vitro, which results in the formation of elongatedand unfolded complexes (8, 9). Since the virus coat protein(CP) is not required for intercellular spread of TMV infection(10, 42) MP is believed to form a ribonucleoprotein complex(vRNP) with viral RNA (vRNA) and to facilitate its intercellulartransport in nonencapsidated form (9).

To elucidate the mechanism by which MP and vRNA are targeted to Pd, we recently developed recombinant TMV derivatives whichencode MP as a fusion with green fluorescent protein (GFP). Usingthese constructs, it was possible to perform studies in plantaand to directly correlate the cell-to-cell spread of vRNA andthe growth of the fluorescent infection site with the subcellularlocalization of the MP:GFP fusion protein (24, 25, 37).These studies demonstrated that during infection, the virus-encodedMP:GFP fusion protein associates with Pd, with irregularly shapedendoplasmic reticulum (ER)-derived inclusion bodies, as well aswith microtubules (5, 24). The ER-derived inclusion bodiescontain replicase (25) as well as vRNA (34) in addition toMP, thus providing evidence that these bodies represent sitesof virus replication and protein synthesis. During the courseof infection, MP:GFP produced in these sites is conveyed to microtubules(25), indicating a role of microtubules in the transport ofvRNPs from membrane sites of synthesis toward Pd (25). Recentsupport for this hypothesis was provided by in situ hybridizationexperiments which localized TMV RNA to microtubules (34) aswell as by in vivo observations which indicated that the amountof MP:GFP associated with microtubules at the leading edge ofinfection is positively correlated with the efficiency by whichinfection spreads from cell to cell (5). MP also appears tointeract with actin (35). Since actin is a component of Pd (2,14, 52), it may be possible that microfilaments and microtubulesshare synergistic functions in Pd targeting (6, 54).

This study was undertaken to further dissect the functional role of associations of MP with microtubules, ER inclusion bodies,and Pd. Based on the finding that the vRNA transport functionof MP can tolerate large deletions at its C terminus but not atits N terminus (1), we generated a series of TMV derivativesin which we introduced N- and C-terminal deletions into MP fusedto GFP. This generated a series of infectious and noninfectiousvirus derivatives which allowed us to correlate the activity ofwild-type and mutant MP:GFP in viral movement with their subcellulardistribution and to identify those interactions between MP andhost components that are essential or dispensable in vRNA intercellulartransport inplanta.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Constructs. Plasmid pTf5-nx1, used as a template for in vitro mutagenesis, was constructed by substitution of the MluI-KpnI fragment ofplasmid pLA41, a pUC119 derivative with an extended polylinker,with the BamHI-KpnI restriction fragment of pTMV-M:GfusBr (24,25, 37). BalI-SpeI restriction sites were then used to replacemost of the GFP coding sequence by a PCR fragment encoding animproved version of GFP (GFP5, without ER targeting sequences)which is characterized by increased thermostability and by twostabilized excitation absorbance maxima (395 and 473 nm) (41).Unique NruI and XhoI restriction sites were then introduced infront of and behind the MP:GFP5 open reading frame (ORF), resultingin plasmid pTf5-nx1. The BamHI-NotI fragment of pTf5-nx1 was thenused to replace the BamHI-NotI fragment of pTMV-M:GfusBr to createplasmid pTf5-nx2, encoding infectious genomic RNA of TMV-MP:GFP5.It should be noted that "wild-type MP" refers to the MP as expressedfrom the original TMV-M:GfusBr construct (24). In this construct,fusion of the GFP ORF resulted in the deletion of 30 nucleotidesfrom the 3' end of the MP gene sequence. Thus, wild-type MP fusedto GFP lacks amino acids 259 to 268 from its C terminus. Moreover,the MP is derived from a TMV variant that is distinguished fromthe published TMV U1 sequence by a replacement of glutamic acidin position 52 by glycine (27).

In vitro mutagenesis of the MP:GFP5 coding sequence was performed by PCR in the presence of pTf5-nx1 as the template and specificprimer sets for mutagenesis to yield MP sequences encoding MPwith specific N- or C-terminal deletions. The PCR fragments wereblunt ended at the 5' end of the corresponding plus strand andhad an XmaI restriction site at their 3' end, the latter locatedwithin the hinge region between MP and GFP (24). Following XmaIdigestion, the sequences were cloned into plasmid pTf5-nx1 forin-frame fusion of the MP sequences with the GFP ORF, replacingthe NruI-XmaI fragment. The resulting pTf5-nx1 derivative plasmidswere cut with restriction enzymes BamHI and Asp718I to subclonethe fragments in place of the respective fragment in pTf5-nx2.Viral infectious RNA was produced by in vitro transcription ofplasmid pTf5-nx2 (wild-type MP:GFP) and its derivatives (dMP:GFPmutants) by using a MEGAscript T7 kit(Ambion).

Inoculation of plants and protoplasts. Nicotiana tabacum cv. Xanthi nn, N. tabacum cv. Xanthi NN, and N. benthamiana plants (5 to 6 weeks old) were mechanicallyinoculated (in the presence of carborundum) with transcripts derivedfrom in vitro reactions, and the plants were maintained in 70%humidity at 22°C during the 16-h photoperiod and at 20°C duringthe darkperiod.

Protoplasts of tobacco suspension cell line BY-2 were prepared and inoculated by electroporation with infectious transcriptsas described elsewhere (51). Following inoculation, protoplastswere resuspended in 10 ml of medium and cultured as 1-ml aliquotsin 35-mm-diameter petri dishes in the dark at 28°C. ActinomycinD (30 µg/ml) was added to the protoplasts to increase MP expression(3, 25).

Immunoblot analysis. Protoplasts (5 × 10⁵) were harvested at 20 h postinfection from culture medium by low-speed centrifugation, and pellets wereimmediately frozen on dry ice and stored at $-$ 80°C. Proteins from125,000 protoplasts were subjected to sodium dodecyl sulfate-polyacrylamidegel electrophoresis and blotted onto polyvinylidene difluoridemembranes (Amersham, Arlington Heights, Ill.). The membranes wereprobed with affinity-purified rabbit antibodies that were raisedagainst synthetic peptides encompassing amino acid residues 6to 22 (N-terminal anti-MP) or 209 to 222 (C-terminal anti-MP)ofMP.

Immunofluorescent labeling and microscopy. Fixation and immunostaining of protoplasts was performed as described elsewhere (24). Rhodamine-labeled secondary antibodywas from Pierce (Rockford, Ill.). Fluorescence microscopy wasperformed with a Nikon Eclipse E800 microscope equipped with CFIPlan Apochromat objectives (Nikon Corp., Tokyo, Japan) and XF100(Omega Optical, Inc., Brattleboro, Vt.) as well as G-2A (NikonCorp.) filter sets for visualization of GFP and rhodamine fluorescence,respectively. Whole fluorescent infection sites on leaves wereviewed with 2× or 4× lenses. Leaf disks placed on glass slideswere used for high-magnification microscopy using 100× oil immersionobjectives. Protoplasts were analyzed with 60× and 100× oil immersionlenses. Images were acquired and processed using an ORCA-100 progressivescan interline charge-coupled device camera (Hamamatsu Photonics,Hamamatsu City, Japan) and Openlab 2 software (Improvision, Coventry,England). Images were prepared for publication using Adobe Photoshopsoftware (Adobe Systems Inc., Mountain View, Calif.).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

TMV derivatives replicate and produce $Delta$ MP:GFP proteins of expected sizes. The deletion mutations in MP used in this study (Fig. 1A) include two $Delta$ MP:GFP mutants with 3 and 28 amino acids deleted fromthe N terminus (the first two amino acids, N5 and N30, were notdeleted) and four $Delta$ MP:GFP mutants with up to 81 amino acids deletedfrom the C terminus (C35, C55, C66, and C81) of MP. Except forencoding either wild-type MP:GFP or $Delta$ MP:GFP, all viral constructsused in the analysis were identical and derived from TMV-MP:GFP(25). To test whether the viruses replicate and produce authentic $Delta$ MP:GFP mutant proteins, we infected BY-2 protoplasts and confirmedexpression of the $Delta$ MP:GFP proteins by immunoblotting using antibodiesraised against N- and C-subterminal peptides of the MP. As shownin Fig. 1B and C, the $Delta$ MP:GFP fusion proteins were comparableto MP:GFP produced by the wild-type virus with respect to bothamount and stability.

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FIG. 1. (A) Schematic representation of $Delta$ MP:GFP constructs used in this study. MP and GFP sequences are represented by dark grey and white, dashed bars, respectively. MP:GFP (24) is shown at the top, and $Delta$ MP:GFP derivatives are depicted below. The $Delta$ MP:GFP derivatives include mutants with up to 81 amino acids deleted from the C terminus (C35, C55, C66, and C81) and 3 or 28 amino acids deleted from the N terminus (the first two amino acids, N5 and N30, were not deleted) of MP. (B and C) Immunoblot analysis of infected tobacco BY-2 protoplasts expressing wild-type MP:GFP and $Delta$ MP:GFP mutants with antibody directed against amino acids 6 to 22 (B) and 209 to 222 (C) of MP. Mk, mock-infected protoplasts; M, protein size markers (positions are indicated in kilodaltons).

Activity of $Delta$ MP:GFP mutant proteins in intercellular transport of vRNA. It was previously reported that MP can tolerate deletions of up to 55 amino acids at its C terminus, whereas even very smalldeletions within the N terminus destroy the function of MP invRNA transport (1, 20). To test if this activity profileof MP deletion mutants is reflected by our $Delta$ MP:GFP fusion proteins,we tested the infectivity of TMV variants encoding these mutantproteins by inoculation of N. tabacum cv. Xanthi NN plants. N.tabacum cv. Xanthi NN plants harbor the N gene, which triggersa hypersensitive cell death response in infected cells, resultingin the formation of local necrotic lesions (Fig. 2A). As summarizedin Fig. 2B, local lesion formation on leaves of N. tabacum cv.Xanthi NN plants was observed when leaves were inoculated withvirus expressing MP:GFP, C35:GFP, or C55:GFP. Thus, C35:GFP andC55:GFP are functional and, like MP:GFP, can transport vRNA fromcell to cell. In contrast, no lesions were observed on N. tabacumcv. Xanthi NN plants when leaves were inoculated with virus encoding $Delta$ MP:GFP with larger deletion mutations at the C terminus of MP(C66:GFP or C81:GFP). Lesions also did not develop when leaveswere inoculated with virus expressing N5:GFP or N30:GFP. Thus,all mutant viruses except those that produced C35:GFP or C55:GFPwere defective in local movement. Nevertheless, as summarizedin Fig. 2B, the whole series of mutant and wild-type viruses wasinfectious on N. tabacum cv. Xanthi NN plants carrying a transgenefor MP (line 2005 [11]). Thus, all mutant viruses were ableto replicate and to move from cell to cell if complemented bywild-type MP. Collectively, these tests demonstrated that the $Delta$ MP:GFP fusion proteins reflect the activity profiles reportedfor unfused $Delta$ MP mutants (1, 20).

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FIG. 2. Infectivity of TMV derivatives encoding $Delta$ MP:GFP fusion proteins. TMV variants encoding either wild-type MP:GFP or mutant $Delta$ MP:GFP derivatives were inoculated onto leaves of N. tabacum cv. Xanthi NN plants to test for local lesion development (A) in response to local virus movement. (B) Results obtained following inoculation of nontransgenic (NN) and MP-transgenic (NN^MP) plants, showing the presence (+) and absence (--) of local lesion formation. The ability of a virus mutant to induce the formation of lesions on MP-transgenic but not nontransgenic plants indicates that the virus replicates but encodes a $Delta$ MP:GFP fusion protein deficient in TMV RNA transport.

Intracellular targeting of MP:GFP and mutant $Delta$ MP:GFP derivatives. To correlate the activity profiles of mutant $Delta$ MP:GFP proteins with their specific subcellular sites of accumulation, we analyzedinfection sites formed at 22°C on leaves of N. benthamiana, asystemic host of TMV. As expected, viruses encoding C35:GFP orC55:GFP were infectious in N. benthamiana, whereas the other viralmutants were dependent on functional complementation by N. benthamianatransgenic for MP. Since we did not observe any difference insubcellular localization of MP:GFP, C35:GFP, and C55:GFP betweeninfection sites on wild-type and MP-transgenic N. benthamianaplants, subcellular localization of each of the $Delta$ MP:GFP mutants(Fig. 3) was examined in MP-transgenic plants. Nevertheless, tomonitor possible effects of wild-type MP on the subcellular distributionof the $Delta$ MP:GFP mutants, especially those that are impaired infacilitating vRNA movement, we compared the localization patternof the proteins in N. benthamiana with their localization patternin infected, nontransgenic BY-2 tobacco protoplasts. The timecourse of MP:GFP accumulation in epidermal cells and protoplastshas been described in detail elsewhere (25). Therefore, emphasiswas given to the occurrence, absence, or modification of specificpatterns, although a detailed time course analysis was performedfor each of the viral constructs. Infected protoplasts were analyzedat 10, 14, 18, and 22 h postinfection; MP:GFP accumulation patternsin cells of infection sites on N. benthamiana leaves were carefullyexamined at high magnification, starting with cells at the outerleading edge and progressing toward cells within the center ofthe infectionsite.

Consistent with transient expression of MP early during infection (49), infection sites formed in N. benthamiana by virusproducing fluorescent MP:GFP appear in the form of fluorescentrings (24, 25) (Fig. 3, A1). Like in previous studies (25),we observed that the MP:GFP localized to Pd in all cells of theinfection site, including those at its center (Fig. 3, A2 andA3). Moreover, also as described previously, MP:GFP accumulatedin inclusion bodies in cells at or near the leading edge of theinfection site (Fig. 3, A4) and on microtubules in cells in themiddle and at the trailing edge of the infection site (Fig. 3,A5). Association of MP:GFP with microtubules and inclusion bodieswas also seen in infected protoplasts (Fig. 3, A6). Moreover,protoplasts displayed fluorescent puncta at or near the plasmamembrane (25). However, because a clear relationship betweenthese puncta in protoplasts and specific sites of MP:GFP accumulationin epidermal cells could not be established, we decided not tofocus on the puncta.

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FIG. 3. Intracellular targeting of MP:GFP and of mutant $Delta$ MP:GFP derivatives. Wild-type MP:GFP and mutant derivatives encoded by the virus used for infection are indicated on the left. Infection sites in MP-transgenic N. benthamiana are shown in column 1, and the subcellular distribution of the proteins in epidermal cells from these sites is shown in columns 2 to 5. Images in columns 2 and 3 show the presence or absence of the proteins in Pd of epidermal cell walls at the leading edge (LE) and trailing edge (TE) of infection; those in columns 4 and 5 show representative patterns of distribution of the proteins within the cytoplasm of cells at the LE and TE. Localization of the LE and TE of the ring-like infection site is shown in A1. In the cases of infection sites that appeared in the form of expanding disks (F1, G1, and H1), no TE could be defined and pictures were taken from cells close to the center of the infection site. Column 6 displays representative images of the subcellular distribution of the proteins in infected tobacco BY-2 protoplasts which are nontransgenic for MP. The size bar in A1 represents 1 mm and applies to all infection sites shown in column 1; the size bar in A2 represents 5 µm and applies to all images in columns 2 to 5 except for G5 and H5, where the size bar represents 2.5 µm; the size bar in A6 represents 10 µm and applies to all protoplasts shown in column 6.

Infection sites produced by virus encoding C35:GFP appeared as fluorescent rings (Fig. 3, B1) and thus were similar to thoseproduced by virus encoding MP:GFP (Fig. 3, A1). The intracellulardistribution of C35:GFP was also essentially like that of MP:GFPand indicated association of the protein with inclusion bodiesat the leading edge of the ring (Fig. 3, B4), with microtubulesat the trailing edge of the ring (Fig. 3, B5), as well as withPd throughout the infection site (Fig. 3, B2 and B3). However,accumulation of C35:GFP in inclusion bodies was reduced (Fig.3, B5) compared to MP:GFP (Fig. 3, A5). This was especially obviousin protoplasts, where the protein was mostly observed in associationwith microtubules (Fig. 3, B6). C55:GFP accumulated on microtubules(Fig. 3, C5) and in Pd (Fig. 3, C2 and C3) but not in inclusionbodies (Fig. 3, C4). Moreover, unlike MP:GFP and C35:GFP, C55:GFPwas localized to microtubules throughout the infection site, evenin cells at the very leading edge of infection (Fig. 3, C4 andC5). Similar findings were obtained in infected BY-2 protoplasts,where C55:GFP was predominantly found in association with microtubulesthroughout the time course of infection (Fig. 3, C6). Since C55:GFPis active in vRNA transport, these observations indicate thataccumulation of MP:GFP in ER-derived inclusion bodies is not arequirement for itsactivity.

Virus encoding C66:GFP could form infection sites (Fig. 3, D1) only in N. benthamiana transgenic for MP. This was expectedsince this virus also was movement defective in N. tabacum cv.Xanthi NN and gave rise to infection and the formation of locallesions only in the presence of wild-type MP (Fig. 2). The functionaldeficiency of C66:GFP in vRNA movement was correlated with thelack of association of the protein with microtubules in epidermalcells of MP transgenic plants (Fig. 3, D4 and D5) as well as innontransgenic protoplasts (Fig. 3, D6). Instead, the protein appearedin the form of thick bundles of short filaments that accumulatedin the center of the cells (Fig. 3, D4 and D5; Fig. 4). To testif this aberrant localization of C66:GFP was caused by disruptionof microtubules in infected cells, we stained infected protoplastswith antibodies directed against $alpha$ -tubulin. As shown in Fig. 4,green fluorescence of MP:GFP (Fig. 4A) and C55:GFP (Fig. 4D) alignedrhodamine-labeled, red fluorescent microtubules (Fig. 4B and 4E)and gave rise to yellow-stained microtubules when images weremerged (Fig. 4C and F). C66:GFP formed aberrant filaments (Fig.4G) even though microtubules were intact (Fig. 4H and I), confirmingthat C66:GFP does not disrupt microtubules but is deficient inmicrotubule association. In addition to the formation of aberrantfilamentous structures in the center of infected cells, C66:GFPwas also characterized by its lack of accumulation in Pd of cellslocated at the leading front of infection (Fig. 3, D2). The proteinaccumulated normally in Pd of cells at the trailing edge and inthe center of the infection site (Fig. 3, D3), showing that C66:GFPis not defective in Pd targeting per se. However, the deletionmutation in C66:GFP appears either to fully abolish Pd targetingof the protein early during infection or to reduce the rate ofPd targeting, thus prolonging the time required for accumulationand, as infection advances, visualization of the protein in Pdof cells located behind the infection front.

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FIG. 4. Intracellular distribution of MP:GFP (A to C), C55:GFP (D to F), and C66:GFP (G to I) in relation to the pattern of microtubules in infected BY-2 protoplasts. Microtubules were immunostained with antibody directed against $alpha$ -tubulin followed by rhodamine-labeled secondary antibody. Bar = 10 µm. The strong red fluorescence in the center of protoplasts shown in panels B and H may be caused by insufficient fluorescence filtering and bleed-through from areas of very strong GFP fluorescence.

The finding that C55:GFP, but not C66:GFP, interacted with microtubules suggested that amino acids 203 to 213 may be involvedin microtubule association of MP:GFP. To test this possibility,we constructed a virus in which only amino acids 203 to 213 weredeleted from MP (C55-66). Like virus encoding C66:GFP, this viruswas infectious only when inoculated onto plants expressing wild-typeMP, where it formed normal ring-shaped infection sites (Fig. 3,E1). Unexpectedly, in epidermal cells as well as in protoplasts,we observed that C55-66:GFP, unlike C66:GFP, associated with microtubules(Fig. 3, E4, E5, and E6), indicating that amino acids 202 to 213are not essential for microtubule association of MP. However,like C66:GFP, C55-C66:GFP did not accumulate in Pd at the leadingedge of infection (Fig. 3, E2 and E3). We conclude that accumulationof MP in Pd behind the infection front is insufficient for intercellulartransport of vRNA. In contrast, vRNA movement requires the presenceof MP in Pd of cells at the leading front ofinfection.

Like C66:GFP, C81:GFP failed to associate with microtubules and formed short filamentous structures in epidermal cells (Fig.3, F4 and F5) and protoplasts (Fig. 3, F6). However, in contrastto filaments formed by C66:GFP (Fig. 3, D4, D5, and D6), filamentsformed by C81:GFP were more numerous, randomly distributed, anddevoid of bundle formation (Fig. 3, F4, F5, and F6). More importantly,in contrast to C66:GFP, C81:GFP failed to accumulate in Pd anywherewithin the infection site (Fig. 3, F2 and F3), suggesting thatamino acids 188 to 202 contribute to Pd targeting of MP. Moreover,unlike virus expressing wild-type MP:GFP or virus expressing $Delta$ MP:GFPwith deletions of up to 66 amino acids from the C terminus, virusencoding C81:GFP produced disk-shaped rather than ring-shapedinfection sites (Fig. 3, F1). This may suggest that a normal ring-shapedappearance of the infection site is linked to the ability of MPto targetPd.

Like C81:GFP, N5:GFP failed to accumulate in Pd throughout the infection site (Fig. 3, G2 and G3) and produced disk-shapedinfection sites (Fig. 3, G1). However, in contrast to C81:GFP,this mutant had the ability to associate with microtubules (Fig.3, G4 and G6) and inclusion bodies (Fig. 3, G5), indicating thatthese associations are not sufficient for Pd targeting of MP andfor vRNAmovement.

We noted that the intracellular distribution of N5:GFP differed between infected MP-transgenic epidermal cells and infectednontransgenic BY-2 protoplasts. In epidermal cells, N5:GFP tendedto accumulate in the form of very large fluorescent inclusionbodies (Fig. 3, G5). Fluorescent filaments were seen only rarelyand, if present, were aberrantly shaped (faintly visible in Fig.3, G4). In contrast, in protoplasts N5:GFP was associated withmicrotubules and accumulated in inclusion bodies at much lowerlevels if at all (Fig. 3, G6). These findings suggest that N5:GFPmay not be able to compete with the plant-encoded wild-type MPfor binding sites on microtubules and therefore accumulates ininclusion bodies in epidermal cells. It may also be possible thatN5:GFP and plant-encoded MP undergo an incompatible interactionin which wild-type MP and N5:GFP mutually interfere with microtubuleassociation. Such a mechanism could contribute to MP-derived resistancedeveloped by plants transgenic for a defective MP which lacksamino acids 3 to 5 (30; G. Kotlitzky, A. Katz, J. van der Laak,V. Boyko, M. Lapidot, R. N. Beachy, M. Heinlein, and B. L. Epel,submitted for publication) as is the case for N5:GFP.

N30:GFP was also impaired in efficient Pd accumulation (Fig. 3, H2 and H3) and produced disk-shaped infection sites (Fig.3, H1). Like N5:GFP, this protein distributed differently betweenepidermal cells of MP-transgenic plants (Fig. 3, H4 and H5) andnontransgenic BY-2 protoplasts (Fig. 3, H6). However, the patternsobserved in both systems indicate that N30:GFP has the capacityto accumulate in inclusion bodies as well as to interact withmicrotubules.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

This study was undertaken to illuminate the mechanism by which TMV RNA is targeted to Pd for intercellular spread and to investigatethe functional significance of the previously observed associationsbetween TMV MP and subcellular components. We introduced N- andC-terminal deletion mutations into MP fused to GFP and correlatedthe activity of the resulting $Delta$ MP:GFP mutants in mediating vRNAtransport with subcellular localization. With regard to the effectof the deletion mutations on RNA transport, the MP:GFP fusionproteins behaved as expected from studies on unfused MP (1,20). Thus, the GFP is unlikely to account for the subcellulardistribution effects of the mutations reported here. $Delta$ MP:GFP mutantswith deletions of up to 55 amino acids from the C terminus ofthe MP were functional and allowed vRNA to move from cell to cell.In contrast, $Delta$ MP:GFP mutants carrying either N-terminal deletionsor deletions larger than 55 amino acids from the C terminus ofMP were dysfunctional, and vRNAs produced neither lesions on NNtobacco plants nor fluorescent infection sites on leaves of N.benthamiana. The lack of infection sites was due to a defect inthe vRNA transport function of $Delta$ MP:GFP, since the movement-deficientviruses were able to replicate in protoplasts as well as in transgenicplants expressing functional MP. Using these TMV derivatives expressingfunctional and dysfunctional MP:GFP mutants together with immunolabelingof microtubules in protoplasts, this study shows that the vRNAtransport function of the MP is tightly associated with specifictargeting and accumulation of the protein to microtubules andto Pd at the leading edge of infection, thus supporting the involvementof these sites in intercellular transport ofvRNA.

vRNA movement does not depend on accumulation of MP:GFP in ER inclusion bodies. Deletion of the 35 C-terminal amino acids from MP had no effect on the function and subcellular localization of the protein.Deletion of 55 C-terminal amino acids also did not abolish theRNA transport function of the protein but led to a strong reduction,if not absence, of fluorescence in inclusion bodies. This findingindicates that accumulation of MP in ER-derived inclusion bodiesproposed to represent sites of viral replication and protein synthesis(25, 34, 39) does not represent a functional requirementfor intercellular movement of TMV RNA. The distribution of C55:GFPin infected cells was strikingly similar to the distribution ofMP:GFP at elevated temperature (5). In both cases we observedthat the lack of fluorescent bodies in cells at the leading edgeof infection was complemented by the presence of highly fluorescentmicrotubules. In the case of MP:GFP, the association with microtubulesin cells at the leading edge was correlated with a strong increasein the rate of intercellular spread of infection, supporting arole of microtubules in the trafficking of vRNA to Pd (5).These findings indicate that the distribution of MP:GFP betweenreplication sites and microtubules is critical for the efficiencyof viral movement. Since C55:GFP, in contrast to C35:GFP, accumulatedpredominantly on microtubules, this distribution appears to becontrolled by determinants in MP, most likely by the domain encompassingamino acids 214 to 233. This domain is adjacent to C-terminalsequences that harbor phosphorylation sites (50) as well ashost range determinants (17, 19). Moreover, in vivo phosphorylationin the C terminus of the MP was mapped to a peptide composed ofamino acids 212 to 231 (23) as well as to Ser238 within theMP of the closely related tomato mosaic virus (28). The temperature-sensitivedynamics by which the MP associates with microtubules (5) followingsynthesis on the ER may thus be regulated by multiple phosphorylationand dephosphorylation events at the C terminus as well as by host-specificfactors.

vRNA movement depends on accumulation of MP in Pd early in infection. The observation that the inactivating N5 and N30 deletion mutations specifically interfered with the accumulation of the MP:GFPin Pd suggests that the N-terminal portion of the protein is involvedin targeting or anchorage of MP to Pd and confirms that the presenceof the protein in the cell wall channel is essential for intercellularmovement of vRNA. The observations obtained by using these mutationsalso demonstrated that the ability of MP:GFP to accumulate ininclusion bodies and to interact with microtubules is insufficientfor accumulation of the protein in Pd. In fact, microtubules appearnot to be involved in the targeting of MP to Pd, as was shownby temperature-sensitive mutations in MP which interfere withmicrotubule association but not with Pd targeting at nonpermissivetemperatures (4). In addition to the N5 and N30 mutations,accumulation of MP in Pd was also affected by the large C-terminalC66 and C81 deletion mutations, suggesting that almost all domainsof MP, except the C-terminal amino acids 213 to 268, are requiredfor Pd targeting or anchorage of the protein. It appears noteworthythat the C66 and C55-66 mutations interfered with the accumulationof MP:GFP in Pd at the infection front but not at the trailingedge and in the center of the infection site. It is possible thatthe mutations slow down the targeting of MP:GFP to Pd, thus requiringa longer time for detectable accumulation. However, based on thisobservation one could also speculate that targeting of MP to Pdis differentially regulated during early and late stages of infectionand that the mutations specifically interfere with the targetingof MP:GFP to Pd early in infection. The results obtained withviruses encoding C55-C66:GFP and C66:GFP indicate that MP foundin Pd only behind the infection front is unable to compensatefor the lack of MP in Pd at the leading edge of infection. Thus,it is tempting to speculate that the protein may exist in twoforms, an active form that is targeted to Pd early in infectionand able to support viral movement and an inactive form whichis targeted to Pd late in infection and not able to perform thisfunction. This interpretation is consistent with microinjectionstudies which have shown that MP increases the SEL of Pd withinthe fluorescent halo of the infection site but not in its center(37). This view is also consistent with the proposal that MPwhich stays in Pd behind the infection front may be downregulatedto reduce the level of interference of MP with normal intercellularcommunication (7). Regardless of whether active MP is replacedby inactive MP or active MP residing in Pd is downregulated, blockingPd behind the infection front may represent an important strategyevolved by TMV to interfere with the spread of a virus-specificgene-silencing signal (40, 46) and therefore merits furtherinvestigation.

Involvement of microtubules in vRNA transport. The mutants carrying N-terminal deletion mutations demonstrated that accumulation of MP:GFP in Pd is not a prerequisite forassociation of the protein with microtubules. Thus, the inabilityof C66:GFP to associate with microtubules is caused not by disruptionof Pd accumulation at the leading edge of infection but ratherby an independent effect of the mutation. In fact, the two effectscould be separated when the C terminus of the MP was retainedand only amino acids 203 to 213 of MP were deleted from MP:GFP(C55-66). It is intriguing that deletion of amino acids 203 to268 interfered with microtubule association of the protein althoughneither the deletion of amino acids 203 to 213 nor the deletionof amino acids 214 to 268 had this effect. It thus appears thatamino acids 203 to 268 do not provide a microtubule binding activitybut that deletion of this stretch of the protein sequence affectsa microtubule association domain located in another region ofthe MP. This conclusion is consistent with other studies indicatingthat microtubule association is mediated by the core region ofthe protein (4, 27). Nevertheless, the observation that theinactivating C66 mutation interferes with microtubule associationof MP:GFP is consistent with a role of microtubules in intra-andintercellular transport of vRNA. A role of microtubules in vRNAmovement is further supported by (i) temperature-sensitive mutationsin MP that were used to directly correlate microtubule associationof MP with its activity in intercellular movement of vRNA (4),(ii) a positive correlation between the amount of MP:GFP associatedwith microtubules and the efficiency of intercellular transportof vRNA (5), and (iii) the colocalization of viral genomicRNA with microtubules (34).

The appearance of the infection site is linked to the presence or absence of MP:GFP in Pd. During infection, the tobamovirus MPs are transiently produced and then degraded (3, 16, 26, 31, 38, 44, 49),and a ring-shaped infection site develops because infection spreadsradially, away from the origin of infection. We observed thatseveral mutations in the MP gave rise to a change in the appearanceof the infection site from the normal ring shape to a disk shape.Notably, disk-shaped infection sites are formed by viruses encodingdefective MPs that have lost the ability to accumulate in Pd butstill can associate with microtubules and accumulate in inclusionbodies (N5:GFP; N30:GFP, and C81:GFP). This suggests that thedynamics of MP production and degradation may be tightly linkedto the successful targeting and anchorage of MP to Pd. Since theability of MP to move by itself (48) likely contributes to itsdistribution within the infection site, it is also possible thatMP:GFP mutants that have lost the ability to interact with Pdoveraccumulate in infected cells, thus changing the appearanceof the fluorescent infection site. Finally, $Delta$ MP:GFP mutants thatare not targeted to Pd may fail to downregulate Pd conductivitylate in infection, thus perturbing the regulation of macromoleculartrafficking, including that ofvRNA.

	ACKNOWLEDGMENTS

We thank Barbara Hohn, Witold Filipowicz, Ueli Grossniklaus, and Gertraud Orend for critically reading the manuscript beforesubmission. We are also grateful to Sjoerd van Eeden and MarkusBriker for continuous greenhousesupport.

This work was supported by the Novartis ResearchFoundation.

	FOOTNOTES

^* Corresponding author. Mailing address: Friedrich Miescher Institute, Maulbeerstrasse 66, CH-4058 Basel, Switzerland. Phone:41-61-697-8517. Fax: 41-61-697-3976. E-mail: heinlein{at}fmi.ch.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

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1.	Berna, A., R. Gafny, S. Wolf, W. J. Lucas, C. A. Holt, and R. N. Beachy. 1991. The TMV movement protein: role of the C-terminal 73 amino acids in subcellular localization and function. Virology 182:682-689[CrossRef][Medline].
2.	Blackman, L. M., and R. L. Overall. 1998. Immunolocalization of the cytoskeleton to plasmodesmata of Chara corallina. Plant J. 14:733-741[CrossRef].
3.	Blum, H., H. J. Gross, and H. Beier. 1989. The expression of the TMV-specific 30-kDa protein in tobacco protoplasts is strongly and selectively enhanced by actinomycin. Virology 169:51-61[CrossRef][Medline].
4.	Boyko, V., J. Ferralli, J. Ashby, P. Schellenbaum, and M. Heinlein. 2000. Function of microtubules in intercellular transport of plant virus RNA. Nat. Cell Biol. 2:826-832[CrossRef][Medline].
5.	Boyko, V., J. Ferralli, and M. Heinlein. 2000. Cell-to-cell movement of TMV RNA is temperature-dependent and corresponds to the association of movement protein with microtubules. Plant J. 22:315-325[CrossRef][Medline].
6.	Carrington, J. C., K. D. Kasschau, S. K. Mahajan, and M. C. Schaad. 1996. Cell-to-cell and long distance transport of viruses in plants. Plant Cell 8:1669-1681[CrossRef][Medline].
7.	Citovsky, V. 1999. Tobacco mosaic virus: a pioneer of cell-to-cell movement. Philos. Trans. R. Soc. Lond. B 354:637-643[Abstract/Free Full Text].
8.	Citovsky, V., D. Knorr, G. Schuster, and P. Zambryski. 1990. The P30 movement protein of tobacco mosaic virus is a single-stranded nucleic acid binding protein. Cell 60:637-647[CrossRef][Medline].
9.	Citovsky, V., M. L. Wong, A. L. Shaw, B. V. Venkataram Prasad, and P. Zambryski. 1992. Visualization and characterization of tobacco mosaic virus movement protein binding to single-stranded nucleic acids. Plant Cell 4:397-411[Abstract/Free Full Text].
10.	Dawson, W. O., P. Bubrick, and G. L. Grantham. 1988. Modifications of the tobacco mosaic virus coat protein gene affecting replication, movement, and symptomatology. Phytopathology 78:783-789[CrossRef].
11.	Deom, C. M., S. Wolf, C. A. Holt, W. J. Lucas, and R. N. Beachy. 1991. Altered function of the tobacco mosaic virus movement protein in a hypersensitive host. Virology 180:251-256[CrossRef][Medline].
12.	Deom, M. C., M. Lapidot, and R. N. Beachy. 1992. Plant virus movement proteins. Cell 69:221-224[CrossRef][Medline].
13.	Ding, B. 1998. Intercellular protein trafficking through plasmodesmata. Plant Mol. Biol. 38:279-310[CrossRef][Medline].
14.	Ding, B., M.-O. Kwon, and L. Warnberg. 1996. Evidence that actin filaments are involved in controlling the permeability of plasmodesmata in tobacco mesophyll. Plant J. 10:157-164[CrossRef].
15.	Ding, B., M. O. Kwon, R. Hammond, and R. Owens. 1997. Cell-to-cell movement of potato spindle tuber viroid. Plant J. 12:931-936[CrossRef][Medline].
16.	Epel, B. L., H. S. Padgett, M. Heinlein, and R. N. Beachy. 1996. Plant virus movement protein dynamics probed with a GFP-protein fusion. Gene 173:75-79[CrossRef][Medline].
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