Coat protein gene-mediated resistance to Potato virus A in transgenic plants is suppressed following infection with another potyvirus

E. I. Savenkov1 and J. P. T. Valkonen1

Department of Plant Biology, Genetics Centre, SLU, PO Box 7080, S-750 07 Uppsala, Sweden1

Author for correspondence: Jari Valkonen. Fax +46 18 67 3392. e-mail jari.valkonen{at}vbiol.slu.se


   Abstract
Top
Abstract
Main text
References
 
High levels of resistance to Potato virus A (PVA, genus Potyvirus), indicated by absence of detectable infection in inoculated leaves, were attained in Nicotiana benthamiana transformed with a construct expressing the PVA 5'-untranslated region fused with the coat protein (CP)-encoding sequence. Low steady-state levels of the transgene transcripts were detected. Resistance was PVA-specific and did not protect the plants against infection with Potato virus Y (PVY, genus Potyvirus). Consequently, the steady-state levels of the CP-transgene mRNA were greatly elevated in the plants infected with PVY, and plants became susceptible to infection with PVA. These data show that virus resistance obtained by expressing regions of a plant virus genome in transgenic plants may be suppressed following infection with another virus that evades the virus-specific resistance.


   Main text
Top
Abstract
Main text
References
 
The era of genetically engineered resistance to viruses in plants started with the discovery of resistance to Tobacco mosaic virus (TMV) in tobacco plants transformed with the coat protein (CP) gene of TMV (Powell Abel et al., 1986 ). In this particular case, the transgene-encoded CP is believed to inhibit TMV infection by preventing virion disassembly at virus entry (Lu et al., 1998 ; Beachy, 1999 ). Transformation of plants with viral CP genes was soon found to work against many other viruses as well (Lawson et al., 1990 ; Lomonossoff, 1995 ). However, in many cases the highest levels of resistance were associated with low levels or no detectable production of the CP (Lawson et al., 1990 ), and could even be attained using non-translatable or antisense CP gene constructs (Lindbo & Dougherty, 1992 ; Lindbo et al., 1993 ; Smith et al., 1995 ). The evidence for RNA-mediated resistance led to the discovery that transgenic resistance could result from ‘homology-based gene silencing’ (reviewed in Marathe et al., 2000 ), an inducible cellular RNA surveillance mechanism targeted against viruses containing sequences homologous to the transgene (reviewed in Sijen & Kooter, 2000 ). Since the RNA-mediated resistance is sequence-specific, viruses not closely similar to the transgene sequence can circumvent silencing. Furthermore, they can cause reversal of silencing, as revealed by recovered expression of the silenced marker genes in transgenic plants following virus infection (Anandalakshmi et al., 1998 ; Brigneti et al., 1998 ; Kasschau & Carrington, 1998 ; Voinnet et al., 1999 ). The virus counter-defence against silencing is mediated by certain viral proteins (reviewed in Carrington et al., 2001 ), of which among those first identified was the helper-component proteinase (HC-Pro) of Potato virus Y (PVY, genus Potyvirus, family Potyviridae) (Brigneti et al., 1998 ).

Since virus resistance obtained in transgenic plants is usually virus-specific and often based on gene silencing, infection of the plants with other viruses could reduce levels of resistance due to suppression of gene silencing. However, this possibility remains to be tested. Therefore, the aim of this study was to generate CP gene-mediated resistance to Potato virus A (PVA, genus Potyvirus) in transgenic plants, and to test whether the resistance to PVA was affected by infection of the transgenic plants with PVY, another potyvirus known to suppress gene silencing (Brigneti et al., 1998 ; Mäki-Valkama et al., 2000 ).

Nicotiana benthamiana was transformed with the CP gene of PVA (isolate B11) driven by the 35S promoter of Cauliflower mosaic virus fused with the 5'-untranslated region of the PVA genome to enhance transgene expression. N. benthamiana transformed with the glucuronidase (GUS) marker gene under control of the 35S promoter was used as a control in virus experiments. The constructs and plant materials as well as the experimental conditions and protocols used in this study have been described elsewhere in detail (Savenkov & Valkonen, 2001 ). Thirteen CP-transgenic lines were obtained, and all were resistant to PVA-B11, as indicated by absence of detectable infection following mechanical inoculation (data not shown). The transgenic lines were self-pollinated and the T1 progeny of four CP-transgenic lines were tested for PVA resistance. Some of these T1 progenies contained a few non-transgenic segregants which were susceptible to PVA, whereas all transgenic T1 progeny were PVA-resistant, similar to the primary transformants (data not shown). The T1 progeny of one CP-transgenic line (line ab10) and one GUS-transgenic line that do not segregate for the transgene were selected for this study. Plants were grown from seed under conditions described elsewhere (Savenkov & Valkonen, 2001 ).

The upper leaves of uninoculated, 4-week-old plants of line ab10 were tested for expression of PVA CP and the CP-transgene mRNA. CP was tested by DAS-ELISA (Savenkov & Valkonen, 2001 ) and Western analysis (Sambrook et al., 1989 ) using monoclonal antibodies specific to PVA CP and including known amounts of purified virions of PVA for comparison. Development of reaction with substrate was terminated at the time-point when the lowest amount of virions (0·16 ng per well) had reached an ELISA absorbance value (A405) of 0·20 (for buffer wells and GUS-transgenic plants, A405=0·00). No elevation of A405 values was observed for samples from the transgenic plants (values similar to buffer wells and samples from the GUS-transgenic plants) and no CP was detectable by Western analysis. Total RNA was extracted from the leaves and subjected to Northern analysis using the 32P-labelled PVA CP cDNA as a probe, but no signal corresponding to the CP-transgene mRNA was observed. However, RT–PCR carried out on the total RNA (treated with DNase) using PVA CP gene-specific primers produced a product of the expected size from plants of line ab10. No amplification was obtained from the DNase-treated RNA without RT prior to PCR, or from total RNA of the control (GUS-transgenic) plants. These data indicate that the steady-state expression levels of the PVA CP gene were very low, in contrast to expression of GUS mRNA, which was readily detectable in the GUS-transgenic plants (using the histochemical {beta}-glucuronidase assay).

Four-week-old plants of line ab10 and the GUS-transgenic line were mechanically inoculated with PVA-B11 (inoculum concentration ca. 1 µg virions/ml sterile distilled water) the day after samples had been taken for analysis of transgene expression. Two leaves per plant of a total of 10 plants per line were inoculated in three experiments. The inoculated and upper non-inoculated leaves were tested for PVA by DAS-ELISA at 14 days post-inoculation (p.i.). In plants of line ab10, neither the inoculated leaves nor the upper non-inoculated leaves were infected with PVA (A405 values no different from buffer wells) and plants were symptomless. In contrast, the plants of the GUS-transgenic line developed symptoms of severe mosaic and leaf malformation at 8–10 days p.i., and all plants were systemically infected with PVA (>8000 ng PVA CP antigen/g leaf, as determined by ELISA). Sap was extracted from the PVA-inoculated leaves of line ab10, diluted fivefold with distilled water and used for inoculation of healthy seedlings of the GUS-transgenic line, but no inoculated plant was infected at 14 days p.i. These results indicated that line ab10 expressed high levels of CP gene-mediated resistance to PVA, and that no detectable infection occurred in the inoculated plants.

In the next experiment, 25 plants of line ab10 were grown for 2 weeks, and then five plants were sap-inoculated with PVY (isolate UK, ordinary strain group of PVY). Symptoms of severe mosaic and leaf malformation developed in the PVY-inoculated plants at 8–10 days p.i. The symptomatic leaves were tested for PVY by DAS-ELISA using polyclonal antibodies to PVY (Adgen) and including known amounts of purified virions of PVY for comparison. All symptomatic leaves contained high amounts of the PVY CP antigen (>2000 ng/g). These data indicated that the PVA CP gene provided no resistance to PVY in the transgenic line ab10. Taken together, the very low steady-state levels of transgene mRNA, the high levels of resistance to the homologous virus, and the lack of resistance to a heterologous virus suggested that the resistance to PVA in line ab10 was based on homology-dependent gene silencing (Marathe et al., 2000 ).

Total RNA was extracted from the upper leaves of the healthy plants and PVY-infected plants (14 days p.i.) of line ab10 and subjected to quantitative Northern blot analysis for detection of the PVA CP-transgene mRNA. As before, its expression in healthy plants of line ab10 was extremely low or below the detection limit even using a long exposure of the film, whereas it was readily detectable in the PVY-infected plants (Fig. 1). Hence, infection with PVY led to reversal of the PVA CP gene silencing in the transgenic plants, as revealed by the resumption of transgene mRNA accumulation.



View larger version (52K):
[in this window]
[in a new window]
 
Fig. 1. (A) Accumulation of steady-state levels of transgene mRNA in N. benthamiana plants transformed with the PVA 5'-UTR+CP construct. Total RNA was extracted from six upper leaves immediately before inoculation with PVY (samples 1–6) and from the upper leaves of the same plants (samples 1'–6') and from a non-inoculated control plant (c) 14 days after inoculation with PVY. PVY infection of the leaves was verified by ELISA. RNA (25 µg) from each sample was subjected to Northern analysis (Sambrook et al., 1989 ) using 32P-labelled PVA CP cDNA as a probe. Long exposure (48 h) was used and the signals were visualized by a phosphoimager (Molecular Dynamics). Note that distinct bands corresponding to the expected size of transgene mRNA could already be seen after 2 h of exposure in samples 1'–6'. (B) Ethidium bromide staining of ribosomal RNAs showing equal loading of the samples.

 
The following day, the healthy plants and PVY-infected plants of line ab10, as well as healthy and PVY-infected GUS-transgenic control plants, were sap-inoculated with PVA. All control plants were systemically infected with PVA at 17 days p.i., irrespective of whether they had been healthy or PVY-infected at the time of PVA inoculation (Table 1). The symptoms of all plants co-infected with PVY and PVA were severe and similar to the symptoms caused by PVY and PVA alone, but the amounts of PVA in the co-infected plants were lower than in the non-PVY-infected plants (P<0·05; Table 1), suggesting competition between the two viruses (amounts of PVY were not determined). In all the PVY-infected plants of line ab10, the PVA-inoculated leaves and upper non-inoculated leaves were also infected with PVA at 17 days p.i. (as detected by ELISA and Northern analysis) and contained PVA amounts no different (P<0·05) from those in the PVY-infected control plants (Table 1). In contrast, no PVA infection was detectable in the non-PVY-infected plants (Table 1). Therefore, the results indicate that, in the CP gene-transgenic plants infected with PVY, PVA could overcome the CP gene-mediated resistance. In all virus-infected plants, new leaves continued to display the severe symptoms, indicating no recovery from disease up to 90 days p.i.


View this table:
[in this window]
[in a new window]
 
Table 1. Mean amounts of PVA in leaves of N. benthamiana transformed with the CP-encoding sequence of PVA

 
The new upper leaves were tested for viruses with ELISA at 65 days p.i., with results essentially similar to those obtained at 17 days p.i. (Table 1). Both PVY and PVA were readily detected in all plants of line ab10 that had been doubly infected with these viruses according to the previous ELISA test at 17 days p.i. These data suggested that infection with PVY suppressed the CP gene-mediated resistance to PVA in line ab10.

This study has shown that high levels of resistance to PVA were expressed in N. benthamiana transformed with the CP-encoding sequence of PVA. The observed resistance was associated with very low steady-state levels of the transgene mRNA. These findings are consistent with some of the first reports on the CP gene-mediated resistance to potyviruses (Lawson et al., 1990 ; Lindbo & Dougherty, 1992 ; Lindbo et al., 1993 ). While this study describes the first example of CP gene-mediated resistance to PVA, many previous studies have reported similar resistance to other potyviruses (reviewed in Lomonossoff, 1995 ; Mäki-Valkama & Valkonen, 1999 ). Resistance to PVA was homology-dependent and did not protect the plants against infection with PVY (comparison of the CP-encoding region of PVA-B11 to those of 13 PVY isolates retrieved from databases reveals only 53–56% and 58–60% identity at the nucleotide and amino acid sequence level, respectively). Consequently, the steady-state levels of the CP gene mRNA were greatly increased in the plants infected with PVY, which is consistent with suppression of gene silencing (Marathe et al., 2000 ). Therefore, this situation was reminiscent of a previous study where silencing of the green fluorescent marker gene (GFP) in transgenic plants could be suppressed by ectopic expression of the HC-Pro of PVY, resulting in readily detectable expression of GFP (Brigneti et al., 1998 ).

The important and novel finding of this study is that CP gene-mediated virus resistance in transgenic plants may be suppressed by infection of the plants with heterologous viruses that encode suppressors of gene silencing, such as the HC-Pro of PVY. In contrast to healthy plants of the CP gene-transgenic lines, in which no detectable infection with PVA was observed following challenge with a high PVA inoculum dose, all the PVY-infected plants of the same transgenic line were readily infectible with PVA and accumulated moderate titres of PVA CP and RNA in the systemically infected leaves. Since PVY and PVA share only a low level of sequence similarity (see above), cross-protection between these viruses does not occur, and does not prevent superinfection of the PVY-infected plants with PVA. Hence, the practical impact of the negative effects of gene silencing suppression on transgenic virus resistance in the field will depend on the availability of virus sources and vectors determining the chance of co-infections of plants.


   Acknowledgments
 
Financial support from the European Commission (grant BIO4-CT98-0374), the Research Council for Natural Sciences in Sweden (NFR; grant U-AA/ST 12090-302) and The Royal Swedish Academy of Sciences (KVA) is gratefully acknowledged.


   References
Top
Abstract
Main text
References
 
Anandalakshmi, R., Pruss, G. J., Ge, X., Marathe, R., Mallory, A. C., Smith, T. H. & Vance, V. B. (1998). A viral suppressor of gene silencing in plants. Proceedings of the National Academy of Sciences, USA 95, 13079-13084.[Abstract/Free Full Text]

Beachy, R. N. (1999). Coat protein mediated resistance to tobacco mosaic virus: discovery, mechanisms and exploitation. Philosophical Transactions of the Royal Society of London B Biological Sciences 354, 659-664.

Brigneti, G., Voinnet, O., Li, W.-X., Ji, L.-H., Ding, S.-W. & Baulcombe, D. C. (1998). Viral pathogenicity determinants are suppressors of transgene silencing in Nicotiana benthamiana. EMBO Journal 17, 6739-6746.[Abstract/Free Full Text]

Carrington, J. C., Kasschau, K. D. & Johansen, L. K. (2001). Activation and suppression of RNA silencing by plant viruses. Virology 281, 1-5.[Medline]

Kasschau, K. D. & Carrington, J. C. (1998). A counterdefensive strategy of plant viruses: suppression of posttranscriptional gene silencing. Cell 95, 461-470.[Medline]

Lawson, C., Kaniewski, W., Haley, L., Rozman, R., Newell, C., Sanders, P. & Tumer, N. E. (1990). Engineered resistance to mixed virus infection in a commercial potato cultivar: resistance to potato virus X and potato virus Y in transgenic Russet Burbank. Bio/Technology 8, 127-134.[Medline]

Lindbo, J. A. & Dougherty, W. G. (1992). Untranslatable transcripts of tobacco etch virus coat protein gene sequence can interfere with tobacco etch virus replication in transgenic plants and protoplasts. Virology 189, 725-733.[Medline]

Lindbo, J. A., Silva-Rosales, L., Proebsting, W. M. & Dougherty, W. G. (1993). Induction of a highly specific antiviral state in transgenic plants: implications for regulation of gene expression and virus resistance. Plant Cell 5, 1749-1759.[Abstract/Free Full Text]

Lomonossoff, G. P. (1995). Pathogen-derived resistance to plant viruses. Annual Review of Plant Pathology 33, 323-343.

Lu, B., Stubbs, G. & Culver, J. N. (1998). Coat protein interactions involved in tobacco mosaic tobamovirus cross-protection. Virology 248, 188-198.[Medline]

Mäki-Valkama, T. & Valkonen, J. P. T. (1999). Pathogen derived resistance to potato virus Y: mechanisms and risks. Agricultural and Food Science in Finland 8, 493-513.

Mäki-Valkama, T., Valkonen, J. P. T., Kreuze, J. F. & Pehu, E. (2000). Transgenic resistance to PVYO associated with post-transcriptional silencing of the P1 transgene is overcome by PVYN strains that carry highly homologous P1 sequences and recover the transgene expression at infection. Molecular Plant–Microbe Interactions 13, 366-373.

Marathe, R., Anandalakshmi, R., Smith, T. H., Pruss, G. J. & Vance, V. B. (2000). RNA viruses as inducers, suppressors and targets of post-transcriptional gene silencing. Plant Molecular Biology 43, 295-306.[Medline]

Powell Abel, P., Nelson, R. S., De, B., Hoffmann, N., Rogers, S. G., Fraley, R. T. & Beachy, R. N. (1986). Delay of disease development in transgenic plants that express the tobacco mosaic virus coat protein gene. Science 232, 738-743.[Medline]

Sambrook, J., Fritsch, E. F. & Maniatis, T. (1989). Molecular Cloning: A Laboratory Manual, 2nd edn. Cold Spring Harbor, NY: Cold Spring Harbor Laboratory.

Savenkov, E. I. & Valkonen, J. P. T. (2001). Potyviral helper component proteinase expressed in transgenic plants enhances titers of Potato leaf roll virus but does not alleviate its phloem limitation. Virology 282, 285-293.

Sijen, T. & Kooter, J. M. (2000). Post-transcriptional gene silencing: RNAs on the attack or on the defense? BioEssays 22, 520-531.[Medline]

Smith, H. A., Powers, H., Swaney, S. L., Brown, C. & Dougherty, W. G. (1995). Transgenic potato virus Y resistance in potato: evidence for an RNA-mediated cellular response. Phytopathology 85, 864-870.

Voinnet, O., Pinto, Y. M. & Baulcombe, D. C. (1999). Suppression of gene silencing: a general strategy used by diverse DNA and RNA viruses. Proceedings of the National Academy of Sciences, USA 96, 14147-14152.[Abstract/Free Full Text]

Received 4 April 2001; accepted 30 May 2001.