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American Society of Plant Physiologists Production of 6-Methylsalicylic Acid by Expression of a Fungal Polyketide Synthase Activates Disease Resistance in TobaccoPioneer Hi-Bred International, Inc., P.O. Box 552, 7250 NW 62nd Avenue, Johnston, Iowa, 50131-0552 1 To whom correspondence should be addressed. E-mail yalpanin{at}phibred.com; fax 515-334-4755
Salicylic acid (SA) has been shown to act as a signal molecule that is produced by many plants subsequent to the recognition of potentially pathogenic microbes. Increases in levels of SA often trigger the activation of plant defenses and can result in increased resistance to subsequent challenge by pathogens. We observed that the polyketide 6-methylsalicylic acid (6-MeSA), a compound that apparently is not endogenous to tobacco, can mimic SA. Tobacco leaves treated with 6-MeSA show enhanced accumulation of the pathogenesis-related (PR) proteins PR1,  -1,3-glucanase, and chitinase and also develop increased resistance to tobacco mosaic virus. We transformed tobacco with 6msas, the 6-methylsalicylic acid synthase (6MSAS) gene from Penicillium patulum, to generate plants that constitutively accumulate 6-MeSA. Analysis of primary transformants and the first generation progeny of 6MSAS tobacco revealed that plants can be engineered to accumulate significant amounts of 6-MeSA as a conjugate. Levels of total 6-MeSA increased with plant age. Increased 6-MeSA accumulation correlated with increased levels of PR1 and chitinase proteins and resulted in enhanced resistance of NN genotype 6MSAS tobacco to tobacco mosaic virus. Our results demonstrate that a multistep biosynthetic pathway can be engineered into plants using a single fungal polyketide synthase gene. The functional expression of 6msas can be used to activate disease resistance pathways that normally are induced by SA.
The importance of salicylic acid (SA) as a signal molecule in plant disease resistance responses is well documented and has been the subject of a number of reviews (Raskin, 1992  ; Durner et al., 1997; Mauch-Mani and Métraux, 1998; Dempsey et al., 1999; Scott et al., 1999; Klessig et al., 2000). In many plants, tissue levels of SA increase upon invasion by certain incompatible pathogens and exposure to certain chemicals or environmental stresses (Yalpani et al., 1994; Leôn et al., 1995). This increase may occur not only around the site of inoculum penetration but in more distant tissues as well. Increases in SA frequently induce increased resistance to subsequent challenge by a spectrum of viral, bacterial, or fungal pathogens. SA can induce the expression of several classes of pathogenesis-related (PR) protein gene families (Ward et al., 1991; Van Loon and Van Strien, 1999). Although some, such as -1,3-glucanases and chitinases, have antimicrobial hydrolytic activities, it remains unclear how most SA-induced PR proteins contribute to disease resistance. Other evidence indicates that SA may contribute to resistance by affecting the sensitivity of the triggers for defense activation (Shirasu et al., 1997). Although there is little doubt that SA has a key role in resistance, recent reports indicate that in certain plant–microbe interactions, jasmonic acid, ethylene, nitric oxide, and possibly other molecules also may be involved in the activation of local and systemic defenses (Pieterse and van Loon, 1999; Klessig et al., 2000). Additional work indicates that SA may play a regulatory role in other developmental processes. For example, it has been shown that SA may affect alternative oxidase activity, chilling resistance, stomatal opening, senescence, and cell growth (Raskin, 1992; Janda et al., 1999; Rate et al., 1999; Morris et al., 2000).
In plants, SA most likely is formed by 2-hydroxylation of benzoic acid or benzoyl conjugates. These are likely products of the
Compelling evidence for the importance of SA in disease resistance was obtained from work with plants expressing the Pseudomonas putida gene for SA hydroxylase (nahG). Tobacco and Arabidopsis plants expressing this enzyme constitutively display reduced resistance against viral, bacterial, and fungal pathogens (Gaffney et al., 1993
Here, we present a novel approach to the manipulation of SA response pathways using a fungal polyketide synthase (PKS) gene. Prokaryotic and eukaryotic PKSs form a wide variety of biomolecules, including long-chain fatty acids, pigments, immunosuppressants, and antibiotics (Monaghan and Tkacz, 1990
Among the PKSs, aromatic PKSs consist of a group of iteratively used active sites contained either on a group of separate proteins encoded by a cluster of genes, as in bacteria, or on a large single protein, as in fungi. 6-Methylsalicylic acid synthase (6MSAS) is a well-characterized fungal aromatic PKS from Penicillium patulum Bainier (anamorph P. griseofulvum Dierckx). The 6msas gene, the first fungal PKS gene cloned (Beck et al., 1990
All active sites for the 11 transformations required to produce 6-MeSA are carried on the single multifunctional protein. Catalysis involves the repeated use of some of these active sites. The expression of functional P. patulum 6msas in bacteria and yeast was demonstrated by Bedford et al. (1995)
6-MeSA Treatment Activates Resistance Mechanisms in Tobacco The polyketide product of the reactions catalyzed by 6MSAS from P. patulum shows structural resemblance to SA. To determine if 6-MeSA can mimic SA in planta and trigger similar defense responses, we infiltrated leaves of NN genotype, nontransgenic tobacco plants, with buffer in the absence or presence of either 2.5 mM SA or 2.5 mM 6-MeSA. As expected, by 7 days after infiltration, antiserum raised against acidic PR1, glucanase, and chitinase of tobacco allowed the detection of a significant accumulation of SA-induced proteins (Figure 1) . 6-MeSA also induced these proteins, although not as strongly as SA. When an NN genotype tobacco cultivar is inoculated with TMV, it responds hypersensitively, and spread of the virus is restricted. Enhanced resistance in such plants is reflected by the reduced size of virus-induced necrotic lesions (Holmes, 1938 ).
Consistent with its effect on PR proteins, 6-MeSA also induced enhanced resistance to TMV when leaves were inoculated 7 days after infiltration (Figure 2) . The mean area of individual TMV lesions on leaves that had been pretreated with 6-MeSA was 0.66 ± 0.01 mm2, 55% of the area of lesions on buffer-treated control leaves. Again, SA appeared to be a more potent inducer than 6-MeSA. Although the lesions were smaller in the SA-treated leaves, the results indicate that 6-MeSA induces resistance to TMV. The difference in the efficacy of 6-MeSA compared with SA could be due to dissimilarities in bioactivity, the presence of impurities in the 6-MeSA preparation used, or the differential uptake, transport, or metabolism of the compounds. Using HPLC analysis, we confirmed that the 6-MeSA used was not contaminated by SA. We also determined that 6-MeSA treatment did not affect the levels of SA accumulation in tobacco significantly (data not shown). These results with exogenously applied 6-MeSA suggested that this compound could activate defense mechanisms similar to those activated by SA.
Transgenic 6MSAS Tobacco Accumulates 6-MeSA Even though the results of the leaf infiltration experiments needed to be viewed with caution, we were encouraged sufficiently to try to generate transgenic tobacco expressing 6MSAS. To this end, the binary transformation vector pPHP12424 was constructed. The 6msas and nptII genes in this construct were designed for high level constitutive expression in plants using the SCP1 and UCP3 promoters, respectively, each with the  ' translation enhancement sequence. Because its substrates acetyl-CoA, malonyl-CoA, and NADPH were expected to be available in plastids, a ribulose bisphosphate carboxylase targeting sequence from petunia was used to direct the accumulation of 6MSAS protein to plastids. Primary leaf explants of NN and nn genotype tobacco were inoculated with Agrobacterium strain EHA105/PHP12424 and then cocultivated and selected on kanamycin-containing callus initiation medium. Fast-growing, kanamycin-resistant calli were transferred to selective regeneration medium for the production of transgenic tobacco shoots. Reverse transcription–mediated polymerase chain reaction analysis of callus lines was performed to verify the transcription of the 6msas gene (data not shown). Transgenic shoots initially were identified using NPTII ELISA of leaf samples. NPTII-positive shoots were established in the greenhouse, and developing transgenic plants were assayed for the maintenance of NPTII expression. Compared with nontransformed controls, the primary transgenic plants (T0 generation) had a normal phenotype.
HPLC analysis of hydrolyzed extracts of leaf samples taken at flowering time identified a large number of T0 tobacco events that produced a metabolite that cochromatographed with authentic 6-MeSA (Figure 3)
. This substance was not detectable in untransformed tobacco and was identical to 6-MeSA, as confirmed by its fluorescence emission, its UV light absorption spectrum, and gas chromatography–mass spectral analysis (Figure 4)
. Four of these 6-MeSA–accumulating lines were in an NN genotype background. The levels of total 6-MeSA in leaves of some of the plants exceeded 20 µg/g fresh weight. 6-MeSA appears to accumulate primarily as a conjugate. For plant 917287, we measured 0.078 ± 0.002 µg of free 6-MeSA per gram fresh weight. This was near the fluorescence detection limit for 6-MeSA and insufficient to be confirmed by diode array analysis. Base hydrolysis followed by acid hydrolysis of tissue extracts (Enyedi et al., 1992
Accumulation of 6-MeSA is a heritable trait. The T0 plants were self-pollinated. Seed from the selfed plants were surface sterilized and sown on kanamycin-containing germination medium to select transgenic T1 individuals. Kanamycin-resistant, NPTII-positive T1 plants were tested for 6-MeSA, and five of seven selected events produced progeny that accumulated the compound. Of the 16 individual plants from event 911403 that were tested, 15 had detectable levels of 6-MeSA, whereas no 6-MeSA was detected in leaves of untransformed control NN genotype plants (Figure 5) . Four weeks after transplanting to soil, 6-MeSA levels in fully expanded leaves of the transgenic plants ranged from less than 0.1 to nearly 9 µg/g fresh weight. By 8 weeks after transplanting, the levels had increased in all plants and reached as much as 53.3 ± 1.91 µg/g fresh weight. These results reveal that progeny from plants transformed with 6msas can inherit the trait of 6-MeSA accumulation and that levels of this compound can increase with plant age. It is unclear why the T1 selection 911403-9 accumulated exceptionally high levels of 6-MeSA.
Activation of Disease Resistance Mechanisms in 6MSAS Tobacco Extracts of leaf samples from NN genotype event 870856 were subjected to protein gel blot analysis to examine the effect of 6-MeSA accumulation on PR proteins. There appeared to be a rough correlation between total 6-MeSA levels and the accumulation of PR1 and chitinase proteins (Figure 6) . To study the effect of 6-MeSA accumulation on disease resistance, we inoculated T1 plants derived from line 870955 and additional T1 selections from event 911403 with TMV. The mean area of individual lesions that developed subsequently was determined 5 days later and compared with 6-MeSA levels in a lower leaf of the same plant. The results shown in Figure 7A for derivatives of 911403 demonstrate an inverse relation between mean lesion area and levels of 6-MeSA. The mean area of individual TMV-induced lesions on the transgenic plant that accumulated 0.29 ± 0.01 µg of 6-MeSA per gram fresh weight was 43.4 ± 1.0 mm2, nearly three times larger than the 14.7 ± 0.4 mm2 lesions on the plant that accumulated 4.33 ± 0.21 µg of 6-MeSA per gram fresh weight. Six plants derived from line 870955 accumulated lower levels of 6-MeSA than plants from event 911403. Nevertheless, the plants that accumulated more than 0.23 ± 0.01 µg of 6-MeSA per gram fresh weight displayed increased TMV resistance (Figure 7B). Leaves of untransformed tobacco accumulated levels of total SA similar to those in 6MSAS-tobacco lines (0.10 ± 0.01 versus 0.08 ± 0.01 µg of total SA per gram fresh weight, respectively). Therefore, it is unlikely that the increased TMV resistance of the transgenic plants resulted from a breakdown of 6-MeSA to SA. The data obtained with the 6MSAS plants are consistent with the results of the leaf infiltration experiments and suggest that 6-MeSA acts as an inducer of defense proteins and a trigger of increased resistance to TMV infection.
Effect of 6-MeSA on Plant Phenotype T0 generation transgenic tobacco plants had a normal morphology and produced viable seed. All T1 generation plants looked normal until just before flowering. However, NN genotype T1 plants produced from three events (870955, 870956, and 911403) developed an odd leaf-curling phenotype on leaves that were forming as the floral bud appeared (Figure 8) . As the inflorescence emerged, subsequent leaves looked normal. No abnormal morphology was observed with nn genotype T1 transgenic plants. Additional transgenic 6MSAS tobacco of the NN genotype will need to be generated to determine if the effect on leaf morphology is a transformation artifact or an effect of 6MSAS expression.
In this work, we demonstrated successful plant transformation with a multifunctional fungal polyketide synthase gene. A complex biosynthetic pathway was introduced into tobacco using a single gene from P. patulum. Tobacco transformed with 6msas constitutively accumulated significant amounts of 6-MeSA. This trait is heritable. Results from treatment of leaves with 6-MeSA and work with 6MSAS transgenic plants indicated that 6-MeSA accumulation induces enhanced defense protein levels and virus resistance, probably by mimicking but not acting through SA, a natural defense hormone in tobacco. It is expected that the defense mechanisms that were activated by heterologous 6MSAS expression can affect resistance to other phytopathogenic taxa and can be exploited in other crops as well.
Although we were unable to detect 6MSAS protein by protein gel blot analysis (data not shown), transformed plants appeared to have sufficient functional enzyme activity to allow the production and accumulation of 6-MeSA in leaf tissues. Leaf 6-MeSA levels increased progressively with plant age, primarily in the form of conjugates (Figure 5). Further work is needed to determine the identity of the conjugates. At this time, we do not know if 6-MeSA conjugates have the ability to induce PR protein accumulation or if defenses are activated by free 6-MeSA only. Venkatasubbaiah and Chilton (1992)
The substrates for 6MSAS (acetyl-CoA, malonyl-CoA) and NADPH are expected to be available in chloroplasts. Therefore, we targeted 6MSAS protein to plastids by linking the signal sequence from the petunia ribulose bisphosphate carboxylase small subunit gene to the 6msas gene. However, it is likely that for 6-MeSA to activate defense gene expression, it has to leave the plastids. By analogy to the fate of 4-hydroxybenzoic acid (Siebert et al., 1996
Work by Kealey et al. (1998)
Phosphopantetheinylation of the acyl carrier domains of apo-6MSAS may be achieved by endogenous enzymes that are involved in catalyzing this reaction on the acyl carrier protein(s) of fatty acid biosynthesis. Interestingly, among the microbial phosphopantetheinyl transferases studied, the protein encoded by the B. subtilis sfp gene appears to be outstanding. Although most phosphopantetheinyl transferases seem to have a narrow substrate recognition spectrum, Sfp can efficiently phosphopantetheinylate a number of peptidyl carrier proteins, acyl carrier domains, or subunits of fatty acid synthases and polyketide synthases (Lambalot et al., 1996
Plant Material and Treatments Tobacco (Nicotiana tabacum) cv Xanthi-nc (NN genotype) and cv Xanthi (nn genotype) (seed kindly provided by Prof. Ilya Raskin, Rutgers University, New Brunswick, NJ) was raised in a greenhouse under conditions similar to those described by Simmons et al. (1998) . Regenerated plants were self-pollinated. To study the effect of 6-methylsalicylic acid (6-MeSA) on pathogenesis-related (PR) proteins and tobacco mosaic virus (TMV) resistance, we syringe infiltrated the uppermost fully expanded leaves of 8-week-old plants with 5 mM bis-tris buffer, pH 6.5, in the absence or presence of 2.5 mM 6-MeSA or 2.5 mM salicylic acid (SA). Seven plants were used for each treatment. An additional set of plants were not subjected to infiltration and were used as controls. Seven days later, leaf tissue from two plants per treatment was sampled and pooled for analysis of PR protein accumulation, and control and treated leaves from the remaining plants were inoculated with a suspension of TMV (strain U1). The area of individual TMV-induced lesions was determined 5 days after inoculation. No visible phytotoxicity was associated with these treatments. All reagents used were of the highest purity available.
Construction of the Transformation Vector
The resulting clone, pPHP11028, was used for subsequent cloning into transformation vectors. By means of subcloning and intermediate vectors, the 19.9-kb transformation vector pPHP12424 (SCP1::
Plant Transformation and Regeneration
Analysis of Salicylates and PR Proteins in Leaf Extracts For gas chromatography–mass spectrometry analysis, 100 µL of the hydrolyzed tobacco extracts used for HPLC analysis was dried in limited volume autosampler vials using a SpeedVac (Savant Instruments, Holbrook, NY). The dried residue was resuspended subsequently in 100 µL of bis(trimethylsilyl)trifluroacetamide (Supelco, Bellafonte, PA), and the vials were capped and incubated at 50°C for 15 min. Samples were analyzed using a Hewlett-Packard 5890 gas chromatograph interfaced to a model 5972 mass spectrometer. One-microliter samples were injected (splitless, 250°C inlet) into a 30-m Hewlett-Packard 5MS column with 0.25-mm i.d. and 0.25-µm film thickness. The column conditions were as follows: 170°C for 5 min, with the temperature increased at 5°C/min to 180°C. Finally, the temperature was increased at 20°C/min to 250°C and held for 2 min. The 50 to 550 mass-to-charge ratio range was scanned. The identity of 6-MeSA in tobacco extracts was confirmed by matching the mass spectrum with that of the authentic standard, which coeluted at 7.9 min.
Protein gel blot analysis of the accumulation of PR proteins was as described by Simmons et al. (1998)
The 6msas gene was kindly provided by Prof. Eckhardt Schweizer, and a sample of the 6-MeSA standard was obtained from Prof. Chaitan Khosla (Stanford University, Stanford, CA). Numerous people at Pioneer Hi-Bred International provided critical technical and other support. Among these we particularly thank Kelli Van Waus and Joni Heller for running protein gel blot analysis and Dr. Jan Hazebroek for operating the mass spectrometer. We also are indebted to Alejandra Pascal and her colleagues for expert support with nursing the plants in the greenhouse, and we thank Drs. Jon Duvick and Carl A. Maxwell for providing a critical review of the manuscript. Received January 11, 2001; accepted April 5, 2001.
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Abstract
INTRODUCTION
740 kD (Spencer and Jordan, 1992
