PLANT BREEDING, GENETIC RESOURCES AND MOLECULAR BIOLOGY Received for publication: 11 February, 2011. Accepted for publication: 29 June, 2012. 1 Faculty of Sciences, Universidad Nacional de Colombia. Medellin(Colombia). estorresv@gmail.com 2 Plant Biotechnology, Corporación para Investigaciones Biológicas (CIB). Medellin (Colombia). Agronomía Colombiana 30(2), 163-171, 2012 Development of transgenic lines from a male-sterile potato variety, with potential resistance to Tecia solanivora Povolny Desarrollo de líneas transgénicas de una variedad androestéril de papa, potencialmente resistentes a Tecia solanivora Povolny Emy Shilena Torres1, 2, Javier Torres1, 2, Claudia Moreno1, and Rafael Arango1, 2 ABSTRACT RESUMEN Male sterility is a very important characteristic for environ- mental safety in genetically modified (GM) plants, particularly in the release of transgenic plants in the centers of origin or high biodiversity areas. In order to contribute to the develop- ment of environmentally safe agricultural technologies that allow the proper use of transgenic potato crops in Colombia, this project developed transgenic potato cry1Ac of Bacillus thuringiensis (Bt), lines that are potentially resistant to T. so- lanivora, from the male-sterile variety Pastusa Suprema (PS) (Solanum tuberosum ssp. andigena). Modifications were made to the Agrobacterium tumefaciens mediated-transformation protocol which allowed the genetic transformation of leaves of in vitro plants, with transformation efficiencies of 22 and 37%. Cry1Ac protein levels in transgenic leaves ranged from 88 to 639 ng mg-1 of fresh leaf tissue, suggesting a better potential plant resistance. This is the first report on transgenic lines with potential resistance to T. solanivora from a male-sterile variety of S. tuberosum ssp. andigena. La androesterilidad es una característica de importancia en la bioseguridad ambiental de las plantas modificadas gené- ticamente para la liberación de éstas en los centros de origen o en áreas de alta biodiversidad de los cultivos. Como una contribución al desarrollo de tecnologías agrícolas medioam- bientalmente seguras, que permitan el uso adecuado de cultivos transgénicos de papa en Colombia, en este trabajo se desarro- llaron líneas transgénicas de papa con el gen cry1Ac de Bacillus thuringiensis (Bt), potencialmente resistentes a T. solanivora, a partir de la variedad androestéril, Pastusa Suprema (PS) (Solanum tuberosum ssp. andigena). Modificaciones realizadas con Agrobacterium tumefaciens mediante el protocolo que permitieron la transformación genética de hojas de plántulas in vitro, con eficiencias de transformación de 22 y 37%. En las plántulas transgénicas se obtuvieron niveles de expresión de la proteína Cry1Ac, con valores entre 88 a 639 ng mg-1 de tejido foliar fresco, lo cual sugiere un buen potencial de resistencia de las plantas. Este es el primer reporte de líneas transgénicas, con resistencia potencial a T. solanivora, a partir de una variedad androestéril de S. tuberosum ssp. andigena. Key words: Solanum tuberosum, Agrobacterium tumefaciens, genetic transformation, Bacillus thuringiensis, Guatemalan potato moth. Palabras clave: Solanum tuberosum, Agrobacterium tumefa- ciens, transformación genética, Bacillus thuringiensis, polilla guatemalteca de la papa. Introduction Potatoes (Solanum tuberosum L.) are grown in 125 coun- tries and consumed by more than one billion people world- wide, and are the fourth most important food crop, after wheat, rice and maize. Its annual production is more than 320 million t and constitutes an important dietary source of fiber, carbohydrates, protein, vitamins C, minerals and trace elements (Mullins et al., 2006; FAOSTAT, 2010). In Colombia, this crop ranks fourth in agricultural produc- tion, with 2.2 to 3.0 million t per year, and the ninth in size, with about 128,701 ha (Agronet, 2009). Tecia solanivora Povolny, commonly known as the guate- malan potato moth, is one of the principal entomological pests of economic importance for the potato; found mainly in Central and South America, and in parts of southeast Europe (Child, 2004; EPPO, 2006;). This insect has become a serious pest in Colombian agriculture, as it attacks tubers in the field and in storage, causing losses of up to 100% of total production (Osorio et al., 2001). To control the moth, farmers use indiscriminate applications of chemical pesti- cides which contribute to the selection of resistant insects, mortality of non-target species and destruction of natural enemies. Additionally, these substances generate pollution and adversely affect human health (Arévalo, 2003). 164 Agron. Colomb. 30(2) 2012 Integrated pest management programs (IPMP) of the potato have not had enough success in the field, due to serious dif- ficulties in implementing the management practices for this pest. Genetically modified potato plants carrying Bacillus thuringiensis (Bt) genes constitute a viable alternative to produce plants which are resistant to moths (Meiyalaghan et al., 2006; Estrada et al., 2007; Kumar et al., 2010). In previous studies, the transformation of Colombian potato varieties (S. tuberosum ssp. andigena) has been re- ported (Valderrama et al., 2007). Potato lines of Colombian varieties Diacol Capiro and Parda Pastusa expressing 0.02 to 17 µg g-1, Cry1Ac protein in tubers and fresh tissue were shown to be able to cause 87 to 100% mortality of T. sola- nivora larvae under laboratory and greenhouse conditions (Torres, 2010; Valderrama et al., 2007). Although these transgenic potato lines represent a promis- ing future for control of the Guatemalan potato moth, in general, the release of genetically modified (GM) organisms for agricultural production has generated considerable debate, particularly among the general public, biotech- nologists, international food safety organizations and government officials (Nap et al., 2003). The concerns are related to the possible risk that GM plants may present to the environment. Among the main biological risks that have been cited are: horizontal gene transfer mainly of antibiotic resistance, possible adverse effects in the host organism, negative effects on non-target species, insect resistance, increased invasive weeds, and impact on bio- diversity (Conner et al., 2003; Chaparro, 2011). One of the most important concerns is associated with the potential risk of gene flow from GM crops to neighboring plants of the same or related species, which may generate plants that invade agricultural or natural habitats and adversely affect biodiversity (Conner et al., 2003). As part of the evaluation of the biosafety of transgenic potato plants for release in centers of origin and diversity, studies have been conducted to measure the flow of genes from wild to cultivated potatoes (Celis et al., 2004). A solution for the problem of possible gene flow is the use of male-sterile transgenic potato lines. Celis et al. (2004) suggested the use of male-sterile varieties as a basis for field testing in the Andean region. They report the use of a transgenic male-sterile potato variety called revolution (S. tuberosum ssp. tuberosum × S. tuberosum ssp. andigena) that is resistant to Globodera pallida. In Colombia, the only male-sterile potato variety that has been produced by conventional breeding is the so called Pastusa Suprema variety. This variety was the result of the interspecific hybridization of a clone of Solanum stoloniferum 230490 × Solanum phureja (Juz. et. Buk) var. Yema de huevo, as the maternal parent and Solanum tuberosum ssp. andigena var. Parda Pastusa as the paternal parent. This new variety has high resistance to Phytoph- thora infestans, the causal agent of gout and also has high commercial potential in Colombian markets (Segura et al., 2006; López and Chaparro, 2007; Ñústez, 2011). The present study reports of development of transgenic potato lines of this male-sterile variety with potential resis- tance to T. solanivora. For this purpose, an Agrobacterium transformation system for the variety was optimized, using a transformation vector carrying a cassette containing the Cry1Ac gene of Bacillus thuringiensis. Materials and methods Plant material Plantlets of S.tuberosum ssp. andigena variety Pastusa Su- prema were provided by Universidad Nacional de Colom- bia, Bogotá. The plantlets were aseptically micropropagated using internodal cuts in polypropylene vials containing a solid propagation medium (MP) consisting of Murashige and Skoog salts (MS) supplemented with 2.0 mg L-1 of D-pantothenic acid, 0.4 mg L-1of thiamine, mg.L-1 of myo- inositol, 20.0 g L-1 of sucrose, 1.7 g L-1 of phytagel (pH 5.7) and 12 μM of silver thiosulfate (STP) sterilized by filtration (Rodriguez et al., 2000). The plant material was grown at an average temperature of 20±2°C, relative humidity of 60-70%, light intensity of 3,000 lux and a photoperiod of 12 h. The plantlets were subcultured every month, and the leaves were used for transformation experiments and kanamycin selection. Transformation vector and Agrobacterium The p1AcPRD vector was obtained from University of Ottawa, under a material transfer agreement (MTA). This plasmid carries two constructs: a selection marker cassette containing the nptII gene under regulation of the nos promoter and nos terminator, and a cassette of interest, which carries a sybnthetic cry1Ac gene together with the 2X CaMV35S promoter and the nos terminator (Fig. 1). The vector was transferred to the Agrobacterium tumefa- ciens LBA4404 strain by the method described by Hofgen and Willmitzer (1988). The transformed Agrobacterium strain was grown in 50 mL of liquid LB medium supple- mented with 100 mg L-1 of kanamycin and 25 mg L-1 of strep- tomycin, for 16 h at 28°C in an orbital shaker at 200 rpm 165Torres, Torres, Moreno, and Arango: Development of transgenic lines from a male-sterile potato variety, with potential resistance to Tecia solanivora Povolny to an optical density (OD 600) of 0.6. The culture was then centrifuged at 1,000 gn for 30 min at 4°C, the supernatant was discarded and the bacterial pellet was kept on ice for the explant co-culture. The transformation experiments were carried out follow- ing the protocol described by Trujillo et al. (2001) with some modifications generating two new protocols. In the first protocol (Trujillo modified 1), acetosyringone was added to 100 μM final concentration to AB medium MS salts (supplemented with 1% sucrose) and RM media were used in the activation, infection and co-cultivation steps respectively. In the second protocol (Trujillo modified 2), the bacterial infection medium MIB which consisted in 50 mL AB salts, 5 g glucose, 0.24 g NaH2PO4, 3.9 g de MES (Sigma-Aldrich, St. Louis, MO) and 100 µM acetosyringone finally adjusted to pH 5.6), MIB medium (Gelvin et al., 1989; Ramírez et al., 2009) was used as the infection medium and the infection time was prolonged for 1 h. Transformation controls were treated in the same manner but without Agrobacterium. The transformation experiments were conducted under a completely randomized design where each treatment (transformation protocol) was done with five experimental units. Each experimental unit was a petri dish with 10 leaf explants of the Pastusa Suprema variety. Response variables evaluated were: callus formation, shoot regeneration and root formation. Molecular characterization PCR analysis. Total genomic DNA of the in vitro plantlets (corresponding to the independent putative transformants) and control plants was extracted using the protocol des- cribed by the International Potato Center (CIP) (Ghislain et al., 1997). PCR was done to detect the cry1Ac gene by specific amplification of a 766 pb fragment. The primers used were: CRYC1 (5’-ATCTTCACCTCAGCGTGCTT-3’) and CRYC2 (5’-GGCACATTGTTGTTCTGTGG-3’) (Val- derrama et al., 2007). Each PCR reaction was adjusted to a final volume of 25 µL containing 1X PCR buffer (50 mM of and cryopreserved at -70°C for use in the transformation experiments. Determination of the optimal concentration of kanamycin for the selection of transformed explants To estimate the optimum concentration of kanamycin for the selection of transformed explants, its effect on callus and shoot formation and viability was evaluated as follows: leaves approximately 5x5 mm in size from 4-week-old in vitro plantlets were cut and placed in basal and apical contact with the beam with a regeneration medium (RM) which consisted of MS salts supplemented with 3% sucrose (w/v), 0.05% casein enzymatic hydrolyzate, 1 mg L-1 of GA3, 40 mg L-1 of ascorbic acid, 1 mg L-1 of IAA and 3 mg L-1 of zeatine riboside ZR (Rodríguez et al., 2000) supplemented with different concentrations of kanamycin (0, 25, 50, 100 and 150 mg L-1). For each concentration of kanamycin, 6 petri dishes with 10 leaf explants were used. The explants were incubated in the dark for 15 d at 20±2°C to allow callus formation. Afterwards, during eight weeks, under a photo- period of 12 h, the explants were transferred every 15 d to fresh RM medium with the corresponding concentration of kanamycin. The number of viable explants and/or calli and shoots was then determined. The evaluation of the response variables was done under an experimental design of randomized blocks with 30 experimental units. The explants were considered as vi- able when they remained green with no signs of necrosis or chlorosis, and as non-viable when the explants were necrotic or chlorotic in appearance. Transformation and plant regeneration For the plant transformation experiments, 50 mL of AB liquid medium which consisted of 5 g L-1 glucose; 50 mL of Buffer AB (20x) (60 g L-1 K2HPO4, 20 g L-1 NaH2PO4, 6 g L-1 MgSO4·7H2O); and 50 mL of AB salts (20x) (3 g L-1 KCl, 20 g L-1 NH4Cl, 6 g L-1 MgSO4·7H2O, 0.2 g L-1 CaCl·7H2O and 0.72 g L-1 NaFe-EDTA supplemented with 50 mg L-1 of kanamycin were inoculated with 100 µL of aLBA4404 strain culture carrying the p1AcPRD vector and grown Pnos nptII T nos CaMV35S-2X Cry1Ac T nos PmeI NheI HindIII EcoRI BstBI BamHI FIGURE 1. Linear map of the cassette containing nptII and cry1Ac genes. RB, right border of the T-DNA region; LB, left border of the T-DNA region; CaMV35S-2X, Cauliflower mosaic virus 2 x promoter; P nos, nopalin sintetase promoter; T nos, nopalin sintetase terminator; nptII, neomycin fos- fotransferase gene; cry1Ac, B. thuringiensis cry1Ac gene. RB LB 166 Agron. Colomb. 30(2) 2012 KCl, 10 mM of Tris-HCl, pH 8.3), 1.5 mM of MgCl2, 0.2 mm of dNTPs, 0.4 µM of each primer, 1.5 U of Taq polymerase and 100-200 ng of genomic DNA. DNA amplifications were performed in an iCycler™ (Bio- Rad, Hercules, CA) thermocycler using the following temperature profile: an initial step of 94°C for 3 min, 25 amplification cycles of 1 min, denaturation at 94°C, 1 min annealing at 55°C and 1 min extension at 72°C, followed by an additional extension cycle of 10 min at 72°C. The PCR products (5 µL) were mixed with 6X DNA Loading Dye and ran in a 1% (w/v) agarose gel at 70 V for 45 min. The DNA bands were observed using a UV transiluminator. DAS-ELISA assay. For this assay, extracts of leaves of in vitro plantlets were prepared. The presence of the Cry1Ac protein was detected using an ELISA kit Bt-Cry1Ab/1Ac® (Agdia, Elkhart, IN). The ELISA protocol was performed following the manufacturer’s instructions. Readings were done at 650 nm in an ELISA Bio-Rad (Model 680) Microplate-Reader (Molecular Devices, Sunnyvale, CA). To quantitate the amount of Cry1Ac protein in µg mL-1, a standard curve was constructed using the control provided in the kit. To determine the percentage of Cry1Ac (% Cry- 1Ac), the total protein concentration was estimated using the Bradford method (Bradford, 1976). The OD was read in each microplate and the ratio of μg of Cry1Ac protein per µg of total protein was estimated for each transgenic line. Additionally, we calculated: µg Cry1Ac per mg of fresh leaf tissue. Statistical analysis Results were analyzed using SAS® 9.1 statistical software (SAS Institute, 2003). The association between each con- centration of kanamycin and response variables (callus formation, shoot regeneration and viability) was determi- ned by logistic regression analysis. The effect of transformation protocols on callus formation, regeneration of shoots and root formation was determined by one-way ANOVA and Duncan test. Likewise, for each modified protocol, the regeneration frequency and the transformation efficiency were calculated. The first was calculated as the number of explants that formed shoots divided by the total number of treated explants and the second as the number of PCR and DAS-ELISA positive plantlets divided by the total number of treated explants. To determine significant differences between the percent- ages of Cry1Ac protein expression of transformed plantlets, an ANOVA and a Duncan test for comparison of means were performed. Results and discussion Effect of kanamycin on explant regeneration and viability Callus formation was found to be decreased with increa- sing concentrations of kanamycin. Callous formation of leaf explants exposed to 0 and 25 mg L-1 of kanamycin was 100 and 94%, respectively, while at 50, 100 and 150 mg L-1, callous formation was 70, 5 and 0%, respectively (Fig. 1). The effect of kanamycin on shoot regeneration was obser- ved on leaf explants cultured in kanamycin concentrations equal to or greater than 50 mg L-1. The percentage of shoot regeneration at this concentration was 0% (Fig. 1). Addi- tionally, 99% of the explants were not viable at 50 mg L-1 of kanamycin. This was evidenced by the calli not being able to produce shoots and by the appearance of the explants, which became oxidized and necrotic. ( Fig. 2). FIGURE 2. Effects of kanamycin concentrations on the callus formation and regeneration of explants. The vertical bars indicate standard de- viation. The Pastusa Suprema variety was able to tolerate levels of kanamycin of 25 mg L-1, with explants remaining green at this dose, with many calluses and high percentages of shoot regeneration at week 3 of the culture . Furthermore, concentrations equal to or above 50 mg L-1 were toxic to the explants, drastically inhibiting shoot formation. Analysis of these data allowed for the selection of the con- centration of 100 mg L-1 of kanamycin for the selection of transformed leaf explants. Higher antibiotic concentrations were not used because they could exert strong selection pressure and cause the loss of transformed explants by oxidation due to necrosis or chlorosis of non-transformed tissues (Quissen et al., 2009). The effect of kanamycin on callus formation and regenera- tion has been extensively studied in S. tuberosum. In most studies, concentrations above 50 mg L-1 have been used and 100 mg L-1 is the most common concentration used for the selection of transformed leaf explants (De Block, 1988; Tavazza et al., 1988 Wenzler et al., 1989; Visser et al., 1991; Beaujean et al., 1998; Trujillo et al., 2001; Banerjee et al., 2006). The toxic effect of kanamycin observed at these 0 20 40 60 80 100 120 0 25 50 100 150 Ex pl an ts ( % ) Kanamycin (mg L-1) Callus formation Regeneration 167Torres, Torres, Moreno, and Arango: Development of transgenic lines from a male-sterile potato variety, with potential resistance to Tecia solanivora Povolny concentrations is explained by its direct action on mito- chondria and chloroplast ribosomes of plant cells, resulting in inhibition of protein synthesis. This causes failures in the synthesis of chlorophyll evidenced by chlorosis and growth inhibition (Brasileiro and Aragão, 2001). Transformation and regeneration of the potato lines Comparison of transformation protocols showed that the method by Trujillo et al. (2001) produced 9% callus forma- tion but no shoot regeneration. Friable calli were produced but they became oxidized. The Trujillo modified 1 protocol gave 38% callus formation and 28% shoot regeneration frequency. When Trujillo modified 2 Protocol was used, 52% of explants formed callus and 44% regenerated shoots (Tab.1 and Fig. 3). In both protocols, all regenerating shoots were transferred to a MP medium supplemented with kana- mycin, in order to form rooted plantlets. Statistical analysis showed that callus formation, shoot formation and root formation differed significantly in the modified protocols with respect to the original protocol by Trujillo et al. (2001), with Trujillo modified 2 being significantly better. The results show that the protocol published by Trujillo et al. (2001) is less efficient for the transformation of PS. However, the success of this protocol for transformation of other varieties of S. tuberosum ssp. andigena (Diacol Capiro and Parda Pastusa, among others) suggests an influence by the genotype on the regeneration efficiency, and transformation (Dale and Harnpson, 1995; Heeres et al., 2002). This is especially important when considering that PS is an interspecific hybrid, unlike the Parda Pastusa and Diacol Capiro varieties, and therefore there may have a marked influence from the genotype. The results of this study, together with other reports in the literature, favor the dependency relationship between genotype and transfor- mation, although others claim that transformation is inde- pendent of genotype (De Block, 1988; Kumar et al., 1995). The large difference between the transformation efficiency of the original protocol of Trujillo et al. (2001) and the modified protocols is probably due to the addition of ace- tosyringone to all the culture media used for transforma- tion, as this substance acts as a transcriptional activator of the vir genes, which encode proteins responsible for transfer of T-DNA into the plant genome (Stachel et al., 1986; Gelvin, 2006). This is in agreement with reports by Hamdi et al. (2003) who had higher rates of transforma- tion and regeneration when acetosyringone was added at a concentration of 10 mg L-1 to a co-culture medium during A. tumefaciens mediated genetic transformation of the S. tuberosum var. Desirée. Henzi et al. (2000) were also able to observe increases in the efficiency of transformation of Brasica oleracea L. var. Italics, with the addition of aceto- syringone to the infection medium. Moreover, the difference between the frequencies of trans- formation in the Trujillo modified 1 and Trujillo modified 2 protocols might have been influenced by the parameters: time of infection and infection medium, since these were the basic differences between the two protocols. The infection medium MIB (Gelvin et al., 1989) used in Trujillo modified 2 contains substances that activate the FIGURE 3. Regeneration of transformed Pastusa Suprema leaf explants in regeneration medium RM media supplemented with kanamycin 100 mg L-1 A, Calli produced 3 weeks after transformation. B, Regeneration of shoots at 5 weeks after transformation. C, Stems grown at 6 weeks. D, Regene- ration after 8 weeks. Source photographs: Torres, E.S. TABLE 1. Regeneration and transformation frequency obtained in the transformation protocols. Treatments % Explants with callus (mean±SD) % Explants with shoots (mean±SD) % Shoots with roots (mean±SD) % Regeneration frequencya % Transformation efficiencyb Trujillo 9.0±2.9 0 0 0 0 Trujillo M1 38.0±4.0 28.0±4.0 28.0±4.0 28 22 Trujillo M2 52.0±3.3 44.0±4.6 44.0±4.6 44 37 a Regeneration frequency was calculated as the number of explants that formed shoots divided by the total number of treated explants. b Transformation efficiency was calculated as the number of PCR, DAS-ELISA positive seedlings divided by the total number of treated explants. Trujillo M1, acetosyringone in AB medium MS salts and regeneration medium for activation, infection and co-cultivation steps respectively. Trujillo M2, the bacterial infection medium MIB and acetosyringone prolonged 1 h. A B C D 168 Agron. Colomb. 30(2) 2012 virulence of Agrobacterium: glucose and acetosyringone (Doty et al., 1993; Gelvin, 2003; Gelvin, 2006; Higgins et al., 1992), and compounds which act as buffers or pH stabiliz- ers: sodium dihydrogen phosphate (NaH2PO4), morpholino ethanesulfonic acid (MES) (Gelvin, 2006). Glucose may also be involved in stimulating the virulence of Agrobacterium. Monosaccharides such as glucose, fucose, arabinose and acids such as D-glucuronic acid and D-galacturonic have been identified as inducers of vir genes of Agrobacterium. The ChvE gene is required for the induction of the vir genes by sugars (Doty et al., 1993; He et al., 2009). Peng et al. (1998) and Ramírez et al. (2009) reported that an important condition for achieving high vir gene induction is the presence of glucose in the infection medium. Glucose is generally substituted for sucrose in the activation and infection media. However, this substance is not as effective as the co-inducer of vir genes (Gelvin, 2006). NaH2PO4 and MES can affect vir gene expression due to the interactions that occur between the pH, temperature and inorganic phosphate levels (Gelvin, 2006). In some cases, the environment surrounding wounded plant cells is inhibitory to bacteria because of acid exudates of plant cells (Gelvin, 2006). It is necessary to ensure that Agro- bacterium is in an environment or culture medium with good buffering capacity, to help facilitate transformation (Kanemoto et al., 1989). The MES concentration appears to be critical to determine the transformation efficiency. Ramírez et al. (2009) used the culture media MIB, PIM2 (Aldemita and Hodges, 1996) and Gelvin-Liu (Gelvin and Liu, 1994) for infec- tion and co-cultivation in the genetic transformation of the tomato var. Unapal-Arreboles. These media differed only in the concentration of MES (20, 75 and 50 mM, respectively). Transient expression of the β-glucuronidase gene (GUS) used was increased when the MIB medium was used. For the influence of the time of infection in the frequen- cies of transformation, it has been reported that successful transformation of explants can depend on the time of ex- posure with the inoculum; if it is very long, high-mortality of plant cells occurs due to bacterial infection and if it is very short, only transient expression might be observed (Ramírez et al., 2009). Most research in potato transfor- mation (S. tuberosum spp.) proposes inoculation times between 2 and 15 min (Gustafson et al., 2006; Trujillo et al., 2001). However López and Chaparro (2007) inoculated explants for 30 min, while others, like De Block (1988), per- formed a single inoculation and co-culture for 2 d. Finally, others, like Hamdi et al. (2003) and as in the present study, had success using 1 h of infection in darkness. Molecular characterization The presence of the cry1Ac gene was evaluated by PCR in 38 putative transformants, showing the expected band of 766 bp corresponding to the amplification product of the cry1Ac gene in 31 plants. The non-transformed control plant was PCR negative (Fig. 4). All 31 PCR positive lines were tested by ELISA to determine Cry1Ac protein expression. All lines expressed Cry1Ac protein. The Cry1Ac protein percentage ranged between 2.5 and 6.4% of the soluble proteins extracted from the leaf tissue of in vitro plants, corresponding to expression levels between 88 and 639 ng mg-1 of fresh-leaf tissue (Tab. 2). TABLE 2. Bt transgenic lines of the Pastusa Suprema variety with the highest Cry1Ac protein expressions. Plants grown in kanamycin Cry1Acng protein / mg of leaf tissue PS 40.10 614 PS 40.13 573 PS 40.14 575 PS 40.17 492 PS 40.18 491 PS 40.23 469 PS 40.24 463 PS 40.27 639 According to the PCR and DAS-ELISA analysis, the transformation protocols Trujillo modified 1 and Trujillo modified 2 were effective for regenerating transgenic po- tato shoots. Transformation efficiencies were 22 and 37%, respectively. The difference between these efficiencies 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 FIGURE 4. Amplification of the cry1Ac gene by PCR in putative trans- formed plantlets. Lane 1, 100 bp molecular weight marker; lanes 2-11, putative transformed plants; lane 12, negative control (non-transformed plantlet); lane 13, positive control (transgenic line 40.7 a DC); lane 14, p1AcPRD vector; lane 15, absolute control (no DNA mix). 169Torres, Torres, Moreno, and Arango: Development of transgenic lines from a male-sterile potato variety, with potential resistance to Tecia solanivora Povolny confirms the effectiveness of the changes made in the Trujillo modified 2 protocol to induce Agrobacterium viru- lence and consequently increase the number of transgenic shoots. The obtained transformation efficiencies are higher than those reported by López and Chaparro (2007), who obtained initial transformation efficiencies of 31.0±2.5%, expressed in the formation of callus and a final eficiency of 30%, based on the GUS assay. The difference in the level of expression of Cry1Ac protein in the transgenic plants obtained in this study (88 to 639 ng mg-1 of leaf tissue) can be explained by the fact that such variation in expression is common between popula- tions that are independently transformed with the same transgene (Meiyalaghan et al., 2006; Estrada et al., 2007). This unpredictability of transgene expression is usually attributed to differences in the integration site of the T- DNA into the plant genome (Conner and Christie, 1994; Davidson et al., 2004) and or differences in the number of gene copies (Hobbs et al., 1993). Therefore, further work is required for the determination of the number of cry1Ac gene copies by Southern blot or real time PCR, in order to relate the differences found in the cry1Ac gene expression with the gene copy number. These results are similar to those obtained in other studies of genetic transformation of plants with cry genes, includ- ing transgenic lines with cry genes under the regulation of the CaMV35S promoter (Meiyalaghan et al., 2006; Estrada et al., 2007; Valderrama et al., 2007; Jacobs et al., 2009; Kumar et al., 2010). The levels of protein expression in vitro in our study (639 ng mg-1 of leaf tissue) are comparable with those reported by Torres (2010) on the expression of the Cry1Ac protein in DC variety in vitro plantlets (to 620 ng/mg of leaf tis- sue), also under the control of the CaMV35S 2X promoter. Nevertheless, they are superior to those obtained by Es- trada et al. (2007) in greenhouse plants, resulting from the transformation of the potato ND5873 line with the cry1Ac gene under regulation of the CaMV35S promoter-1X (up to 0.58 ng/mg of leaf tissue). This difference in Cry1Ac expres- sion may be due, among other factors, to the variety used for each study, the transformation vector (the promoter having great influence), the plant tissue and the growth condition (in vitro or greenhouse) (Valderrama et al., 2007; Torres, 2010; Vanegas et al., 2010). Of the above factors, the most important factor is probably the use of the 2X CaMV35S promoter. The results of several studies suggest greater activity of the CaMV35S 2X promoter for protein expression compared to the single promoter (1X) (Torres, 2010; Vanegas et al., 2010). In a study on Cry1Ab protein expression in potato tubers, it was found that the amount of this protein was three to four times higher under the CaMV35S 2X promoter compared to the single promoter (Cañedo et al., 1998). The high Cry1Ac protein expression in the leaves of the transgenic plantlets obtained in this study could sug- gest a potential high expression in tubers. Valderrama et al. (2007), who also transformed varieties of potato S. tuberosum ssp. andigena with the cry1Ac gene under regulation of the 2X CaMV35S promoter, found Cry1Ac protein expression levels between 0.02 and 17.00 ng g-1 of tuber tissue. Additionally, Torres (2010) reported increased levels of Cry1Ac protein expression in fresh tuber tissue (up to 1528 ng/mg of tuber tissue) as compared to the levels obtained in in vitro leaves (210-620 ng/mg tissue). Other studies have also reported a correlation between the Cry protein expression in leaves and tubers (Cañedo et al., 1998; Estrada et al., 2007; Jacobs et al., 2009; Kumar et al., 2009; Meiyalaghan et al., 2006). Since high levels of cry1Ac gene expression were obtained in the PS transgenic lines developed in this study (88 to 639 ng mg-1), it is possible that the resistance to T. solanivora of these lines is good, considering that tubers from transgenic plants that express similar quantities of Cry1Ac protein in leaf tissue have shown between 80 and 100% larval mortal- ity (Valderrama et al., 2007; Torres, 2010). Conclusions In this study, two protocols were optimized for the genetic transformation of the male-sterile Colombian potato vari- ety Pastusa Suprema. These protocols allowed the transfor- mation of this variety with transformation efficiencies 22 to 37% better than other protocols previously reported by other authors. The availability of these protocols allows the possibility of introducing other agronomically important genes, such as those conferring resistance to other pests and/or abiotic stress. The transgenic Pastusa Suprema male-sterile variety pro- vides a basis for solving the problem of gene flow in potato in the Andean region. The possibility of using these lines in national markets will require safety assessments of the phenotypic characteristics of substantial equivalence and productivity as well as biosafety trials under greenhouse and field conditions. This is the first report to our knowl- edge on the development of cry1Ac transgenic potato lines potentially resistant to T. solanivora, developed from a male-sterile variety. 170 Agron. Colomb. 30(2) 2012 Acknowledgements We want to thank the Colombian Ministerio de Agricultura y Desarrollo Rural (MADR) for financial support that hel- ped to carry out this study. We thank Professor Guillermo Correa of the National University of Colombia, Medellin and Wilmer Cuervo for statistical advice. Literature cited Aldemita, R.R. and T.K. Hodges. 1996. 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