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Inheritance of resistance to Meloidogyne incognita race 3 in cotton accession TX 25

Herança da resistência do acesso TX 25 de algodoeiro a Meloidogyne incognita raça 3

ABSTRACT.

Cotton producers worldwide suffer with the losses caused by the presence of phytonematodes. The aim of the present study was to investigate the inheritance of resistance to Meloidogyne incognita race 3 in Gossypium hirsutum variety punctatum accession TX 25. Accessions of Gossypium sp. were obtained from the germplasm bank of Embrapa Cotton. Two experiments were performed in two consecutive years. In the first experiment, a susceptible parental line, FiberMax 966, a resistant parental line, TX 25, and their F1, F2 and backcross generations were tested. In the second experiment, parental lines FiberMax 966 and TX 25, their F2 generation, and genotypes M315 (resistant), LA887 and DeltaOpal (moderately resistant) were tested. In both experiments, plants were inoculated with 2000 eggs and J2 of M. incognita race 3. The gall index, egg mass index and reproduction factor were evaluated 120 days following inoculation. In the first experiment, plants from the F1 and backcross generations were susceptible. Plants from the F2 generation presented a 3:1 resistant-to-susceptible ratio in the two experiments, indicating oligogenic resistance.

Keywords:
Gossypium hirsutum; gall nematode; gene segregation

RESUMO.

Os cotonicultores do mundo inteiro sofrem com as perdas causadas pela presença de fitonematoides nas lavouras. Assim o objetivo deste trabalho foi estudar a herança da resistência do acesso TX 25 de Gossypium hirsutum raça punctatum a Meloidogyne incognita raça 3. Foram utilizados acessos de Gossypium sp. pertencentes ao Banco de Germoplasma da Embrapa Algodão. Foram realizados dois experimentos em dois anos consecutivos. No primeiro ano foram testados FiberMax 966 e TX 25 como parentais suscetível e resistente, respectivamente, e as gerações F1, F2 e retrocruzamento. No segundo experimento foram testados os parentais FiberMax 966 e TX 25, a geração F2 além dos genótipos M315 (resistente) LA887 e DeltaOpal (moderadamente resistentes). Em ambos experimentos as plantas foram inoculadas com 2000 ovos e J2 de M. incognita raça 3. As avaliações ocorreram aos 120 dias após a inoculação, e avaliou-se índice de galhas, índice de massa de ovos e fator de reprodução. No primeiro experimento as plantas da geração F1 e do retrocruzamento se mostraram suscetíveis, As plantas da geração F2 nos dois experimentos apresentaram uma proporção de três plantas resistentes para uma suscetível indicando resistência de caráter oligogênico.

Palavras-chave:
Gossypium hirsutum; nematoide de galhas; segregação gênica

Introduction

In spite of their high productivity, cotton producers suffer crop losses due to the presence of phytonematodes. Main are of cotton plant-parasitic nematode species Meloidogyne incognita (Kofoid & White, 1919, Chitwood, 1949), Rotylenchulus reniformis (Linford & Oliveira, 1940) Pratylenchus brachyurus (Godfrey, 1929) Filipjev & Sch. Sttekhoven, 1941 (Galbieri et al. (2009Galbieri, R., Fuzatto, M. G., Cia, E., Lüders, R. R., Machado, A. C. Z., & Boldt, A. F. (2009). Reação de cultivares de algodoeiro a Meloidogyne incognita em condições de campo e casa de vegetação no estado de Mato Grosso. Tropical Plant Pathology, 34(1), 018-023. ) evaluated the resistance of 22 cotton genotypes against M. incognita and observed that 21 genotypes allowed nematode reproduction. The most affected genotypes generated a 65% loss of production when compared to the resistant genotypes.

The use of resistant cultivars is the most affordable method for the control of nematodes, because it do not increase production costs, do not interfere with the environment, and do not lead to environmental imbalances (Davis & Stetina, 2016Davis, R. F., & Stetina, S. R. (2016). Resistance and tolerance to nematodes in cotton. In R. Galbieri & J. L. Belot (Ed.), Nematoides fitoparasitas do algodoeiro nos cerrados brasileiros: Biologia e medidas de controle (p. 166-243). Mato Grosso, MT: IMAMT.). Genetic resistance is therefore the safest method for decreasing damages caused by M. incognita to cotton crops (Barbosa et al., 2009Barbosa, A. E. A. D., Fragoso, R. R., Souza, D. S. L., Freire, E., Oliveira Neto, O. B., Viana, A. A. B., & Grossi-de-Sá, M. F. (2009). Differentially expressed genes in cotton plant genotypes infected with Meloidogyne incognita. Plant Science, 177(5), 492-497. ). In Brazil, however, there are currently no cotton varieties that combine interesting agronomical characteristics and a level of resistance against this nematode. It is therefore important to identify and characterize sources of resistance and include them in improved germplasm.

Cotton cultivars with moderate resistance to the gall nematode have been previously identified, but are not used on a commercial scale because of their low production potential (Ogallo, Goodell, Eckert, & Roberts, 1997Ogallo, J. L., Goodell, P. B., Eckert, J., & Roberts, P. A. (1997). Evaluation of NemX, a new cultivar of cotton with high resistance to Meloidogyne incognita. Journal of Nematology, 29(4), 531-537.). In the USA, there are three commercial cultivars with moderate resistance to M. incognita. The first source of resistance, Acala NemX, and the second source of resistance, Clevewilt 6, are considered only moderately resistant, and these sources are now used as commercial cultivars. The third source of resistance, Wild Jack Jones, did not become a commercial cultivar but was used to produce cultivar Auburn 623 (cross between Clevewilt 6 and Will Jack Jones), which is highly resistant (Shen et al., 2006Shen, X., Becelare, G.V., Kumar, P., Davis, R. F., May, O. L., & Chee, P. (2006). QTL mapping for resistance to root knot nematode in the M-120 RNR Upland cotton line (Gossypium hirsutum L.) of Auburn 623 RNR source. Theoretical and Aplied Genetics, 13(8), 1539-1549.). Subsequently, the commercial cultivars Stoneville LA887 and Paymaster 1560 were generated from the second resistance source. Of these three sources, only Acala NemX continues to be used by cotton producers in the USA. The remaining two sources are considered obsolete because their agronomic characteristics do not meet the productivity and quality standards of the current market (Robinson et al., 2001Robinson, A. F., Bowman, D. T., Cook, C. G., Jenkins, J. N., Jones, J. E., May, L. O., … Stewart, J. M. (2001). Nematode resistance. In T. L. Kirkpatrick, & C. S. Rothrock (Eds.), Compendium of Cotton Diseases (p. 68-72). St. Paul, MN: The American Phytopathological Society. ).

In Brazil, the Agronomy Institute of Campinas (Instituto Agronômico de Campinas - IAC) introduced a resistant cultivar, IAC 20, originating from the cross between Auburn 56, which is resistant to the Fusarium sp. and root-knot nematode disease complex, and GH 11-9-75 (Carneiro, Neves, Falcão, Paes, Cia, & Sá, 2005Carneiro, R. M. D. G., Neves, D. I., Falcão, R., Paes, N. S., Cia, E., & Sá, M. F. G. (2005). Resistência de genótipos de algodoeiro a Meloidogyne incognita raça 3: Reprodução e histopatologia. Nematologia Brasileira, 29(1), 1-10.). This cultivar was introduced in 1983 and grown until 1996. The IAC later introduced cultivars 96/414, IAC 22 and IAC 23, all of which are IAC 20 hybrids and originated from the Auburn 56 source of resistance. Thus, sources of resistance are scarce and present resistance mechanisms that are similar and therefore easy to overcome (Carneiro et al., 2005Carneiro, R. M. D. G., Neves, D. I., Falcão, R., Paes, N. S., Cia, E., & Sá, M. F. G. (2005). Resistência de genótipos de algodoeiro a Meloidogyne incognita raça 3: Reprodução e histopatologia. Nematologia Brasileira, 29(1), 1-10.).

The continued use of varieties with the same resistance sources can accelerate the nematodes selection pressure and compromise the durability of resistance. Therefore, it is essential to search for new sources, preferably combining different resistance genes.

Recently were identified two main cotton genes that confer resistance to M. incognita. These genes were identified from the RNR Auburn 623. The source of resistance genes are on chromosomes 11 and 14 and appear to have different mode of action, resulting in a resistance mechanism with two stages. While the gene present on chromosome 11 do not prevent the penetration of the second-stage juveniles, however, soon after penetration prevents the development of these juveniles (Gutierrez et al., 2010Gutiérrez, O. A., Jenkins, J. N., Mccarty, J. C., Wubben, M. J., Hayes, R. W., & Callahan, F. E. (2010). SSR markers closely associated with genes for resistance to root-knot nematodes on chromosomes 11 and 14 of upland cotton. Theoretical and Applied Genetics, 121(7), 1323-1337. ; He et al., 2014He, Y., Kumar, P., Shen, X., Davis, R. F., Van Becelaere, G., May, O. L., Nichols, R. L., & Chee, P. W. (2014). Re-evaluation of the inheritance for root-knot nematode resistance in the Upland cotton germplasm line M-120 RNR revealed two epistatic QTLs conferring resistance. Theoretical and Applied Genetics , 127(6), 1343-1351.). Already this gene on chromosome 14, expresses the resistance later form. Not prevent the formation of galls, but prevents or reduces the production of eggs (Gutierrez et al., 2010Gutiérrez, O. A., Jenkins, J. N., Mccarty, J. C., Wubben, M. J., Hayes, R. W., & Callahan, F. E. (2010). SSR markers closely associated with genes for resistance to root-knot nematodes on chromosomes 11 and 14 of upland cotton. Theoretical and Applied Genetics, 121(7), 1323-1337. ; He et al., 2014He, Y., Kumar, P., Shen, X., Davis, R. F., Van Becelaere, G., May, O. L., Nichols, R. L., & Chee, P. W. (2014). Re-evaluation of the inheritance for root-knot nematode resistance in the Upland cotton germplasm line M-120 RNR revealed two epistatic QTLs conferring resistance. Theoretical and Applied Genetics , 127(6), 1343-1351.). Thus these two genes are complementary to allow the cotton presents a resistance response to M. incognita.

Another study of cotton genotypes CIR 1348 and TX-25, which have common ancestors known Auburn 623 RNR, was resistant to two similar stages. A hypersensitive response during the first week after infection M. incognita which stopped the development of the nematode and consequently the formation of galls. It also showed a delayed resistance reaction, about two to three weeks after infection, allowed the formation of larger giant cells galls, and development of nematodes, however prevented nematodes progressed to adult females (Mota et al., 2013Mota, F. C., Alves, G. C. S., Giband, M., Gomes, A. C. M. M., Sousa, F. R., Mattos, V. S., … Carneiro, R. M. D. G. (2013). New sources of resistance to Meloidogyne incognita race 3 in wild cotton accessions and histological characterization of the defence mechanisms. Plant Pathology, 62(5), 1173-1183.).

Given the reduced number of resistant genotypes and the increase in areas contaminated with nematodes, especially M. incognita, studies focused on identifying new resistance sources and evaluating the possibility of their introduction into genetic improvement programs for the development of new cultivars are essential. The aim of this study was to investigate the resistance of wild cotton accession TX 25 to M. incognita race 3.

Material and methods

Two experiments were conducted using Gossypium hirsutum accessions obtained from the germplasm bank of Embrapa Cotton. The species used and their origins are presented on Table 1. The nematodes M. incognita race 3 inoculum was obtained from roots of tomato (Solanum lycopersicum) cultivar Santa Clara from the Santa Cruz group. The inoculum, with nematodes previously identified by species and race, was supplied by the Laboratory of Nematology of Embrapa Genetic Resources (Embrapa Recursos Genéticos - Cenargen).

The first experiment was conducted in a greenhouse. Seeds were sown in 5-L plastic pots containing a mix of soil, sand and commercial substrate (1:1:1) that was previously autoclaved. One seed was sown per pot. The experiment consisted of twenty backcross (BC), seven F1, two hundred F2, seven TX 25, and seven FiberMax 966 plants in a completely randomized experimental design (Table 1).

Table 1
Origin and response of Meloidogyne incognita race 3 on Gossypium sp. genotypes tested in two experiments conducted in 2011 and 2012. Goiania, Goiás State, 2015.

When plants were approximately 20 cm high, which occurred on average twenty days after emergence, 5 mL of a suspension containing 5,000 eggs and J2 were inoculated per plant. The experiment was conducted between June and November at 2011. Plants were watered daily. Fertilization and pest control were performed as needed.

Evaluations were performed 120 days after inoculation. The plants were removed from the pots, the shoots were discarded, and the roots were taken to the laboratory where they were washed and the root fresh weight was measured. The roots were then stained by immersion in 0.15 g L-1 Phloxine B dye (dissolved in water) for twenty minutes and then washed to remove the excess.

Following staining, the gall index and egg mass index were quantified according to Hartman and Sasser (1985Hartman, K. M., & Sasser, J. N. (1985). Identification of Meloidogyne species on basis of differential host test and perineal-pattern morphology. In: K. R. Barker, C. C. Carter, & J. N. Sasser (Eds.), An advanced treatise on Meloidogyne (Vol. 2, p. 525-543). Raleigh, NC: University Graphics, ): 0 = no galls or egg masses; 1 = 1-2 galls or egg masses, 2 = 3 to 10 galls or egg masses; 3 = 11 to 30 galls or egg masses; 4 = 31 to 100 galls or egg masses; and 5 = more than 100 galls or egg masses. The total number of eggs per plant was quantified according to Hussey and Barker (1973Hussey, R. S., & Barker, K. R. (1973). A comparison of methods of collecting inocula of Meloidogyne spp. including a new technique. Plant Disease Reporter, 57(12 ), 1.025-1.028.). The reproduction factor (RF) was calculated for each plant by dividing the total number of eggs per plant (PF) by the number of eggs inoculated (PI = 5,000).

The second experiment was also conducted in a greenhouse. The treatments consisted of five plants of each genotype: FiberMax 966, TX 25, DeltaOpal, M315 and LA887. Cultivars DeltaOpal, LA887 and M315 The genotypes DeltaOpal, M315 and LA887. Cultivars DeltaOpal, LA887 and M315 were included in the experiment because their behavior against M. incognita is well-known, thereby enhancing the reliability of the results. A Federer's augmented block experimental design was used (Federer, 1956Federer W. T. (1956) Augmented (hoonuiaku) designs. Hawaian Planters’ Record, 55(1), 191-208, ) with six blocks. Each block consisted of 34 F2 plants and one plant of each of the controls Delta Opal, FiberMax 966, LA887, M315 and TX 25 for a total of 39 plants. Each block therefore included 34 plants with unknown behavior and five with known behavior.

Seeds were placed in 2-L plastic seedling bags. The substrate, sowing conditions, experimental period since inoculation, and evaluations were performed as described for the first experiment.

The data obtained from the first experiment were subjected to a Pearson's chi-squared test to measure the discrepancy between the observed and expected frequencies under the proposed hypothesis. A goodness of fit test was used to test for monogenic inheritance, double recessive epistasis, and oligogenic or polygenic character in the F2 genotypes by testing the following distributions at p < 0.01: 3S:1R, 1S:2MR:1R, 9S:7R and 9S:3MR:4S. The hypotheses were accepted or rejected based on the χ2 test.

To better visualize of the behavior of the F2 generation plants, histograms were plotted using the RF data obtained for the two experiments. Nematode reproduction in the F2 generation genotypes were compared to a standard susceptible cultivar and classified as resistant, moderately resistant or susceptible according to the method of Starr and Mercer (2010Starr, J. L., & Mercer, C. F. (2010). Development of Resistant Varieties. In R. N. Perry, M. Moens, & J. L. Starr (Eds.), Root-Knot nematodes (p. 326-337). Wallingford, EN: CAB International. ). Plants with a nematode multiplication of 0 to 5%, 5 to 25%, 25 to 50%, and greater than 50% relative to the standard susceptible cultivar were considered highly resistant, resistant, moderately resistant, and susceptible, respectively.

Results and discussion

Cultivar FiberMax 966 was confirmed to be susceptible, presenting a high gall index, egg mass index and nematode RF in both experiments (Tables 2 and 3). The RF values for this cultivar were 24.5 and 59.5 for experiments 1 and 2, respectively, indicating a high susceptibility. Genotype TX 25 presented the lowest gall index and egg mass index and an RF of less than 1, thereby confirming the resistance of this genotype (Oostenbrink, 1966Oostenbrink, M. (1966). Major characteristics of the relation between nematodes and plants. Mendelingen Landbouwhogeschool Wageningen, 66(1), 46.). Genotype TX 25 was highly resistant when compared to the standard susceptible control, FiberMax 966, according to the Starr and Mercer (2010Starr, J. L., & Mercer, C. F. (2010). Development of Resistant Varieties. In R. N. Perry, M. Moens, & J. L. Starr (Eds.), Root-Knot nematodes (p. 326-337). Wallingford, EN: CAB International. ) classification (Table 2).

Table 2
Average gall index (GI), egg mass index (EMI), reproduction factor (RF), and percentage decrease in the percentage decrease in the reproduction factor (PD) of M. incognit a race 3 in different Gossypium hirsutum genotypes in the fisrt experiment. Goiania, Goiás State, 2015.
Table 3
Average gall index (GI), egg mass index (EMI), reproduction factor (RF), and percentage decrease in the reproduction factor (PD) of M. incognita race 3 in different Gossypium hirsutum genotypes in the second experiment. Goiania, Goiás State, 2015.

Plants from the F1 generation were 100% resistant according to the Star and Mercer (2010Starr, J. L., & Mercer, C. F. (2010). Development of Resistant Varieties. In R. N. Perry, M. Moens, & J. L. Starr (Eds.), Root-Knot nematodes (p. 326-337). Wallingford, EN: CAB International. ) classification. According to the Oostenbrink (1966Oostenbrink, M. (1966). Major characteristics of the relation between nematodes and plants. Mendelingen Landbouwhogeschool Wageningen, 66(1), 46.) classification, the F1 generation was susceptible, as it presented a high egg mass index and gall index and an RF greater than 1 (Table 2), showing that female reproduction was affected. Plants originating from backcrossing were susceptible, presenting a high gall index and egg mass index, an RF of 13.6 (Table 2) and an average percentage decrease in RF of 55.65%. These results were expected because the F1 generation used for backcrossing was backcrossed with a susceptible parental line. Plants from the F2 generation presented a decrease in RF of 24.72%, being classified as resistant to M. incognita race 3 according to the classification of Star and Mercer (2010Starr, J. L., & Mercer, C. F. (2010). Development of Resistant Varieties. In R. N. Perry, M. Moens, & J. L. Starr (Eds.), Root-Knot nematodes (p. 326-337). Wallingford, EN: CAB International. ).

The results of the second experiment also confirmed the known behavior of the genotypes used as controls (Table 3). Cultivar FiberMax 966 was susceptible to M. incognita and presented the highest RF (59.48). The genotype TX 25 and M315 presented the lowest RF values (0.2 and 0.4, respectively) and a 99% decrease in nematode reproduction relative to FiberMax 966. The resistance of genotype M315 is known to effectively control of M. incognita race 3. This resistance is conferred by two genes, one dominant gene, MiC 11, derived from accession Auburn 623 and located in chromosome 11 (Gutierrez et al., 2010Gutiérrez, O. A., Jenkins, J. N., Mccarty, J. C., Wubben, M. J., Hayes, R. W., & Callahan, F. E. (2010). SSR markers closely associated with genes for resistance to root-knot nematodes on chromosomes 11 and 14 of upland cotton. Theoretical and Applied Genetics, 121(7), 1323-1337. ; Shen et al., 2010), and one recessive gene, MiC 07, derived from the moderately resistant cultivar Clevewilt 6-1 and located in chromosome 7 (Shen et al., 2006Shen, X., Becelare, G.V., Kumar, P., Davis, R. F., May, O. L., & Chee, P. (2006). QTL mapping for resistance to root knot nematode in the M-120 RNR Upland cotton line (Gossypium hirsutum L.) of Auburn 623 RNR source. Theoretical and Aplied Genetics, 13(8), 1539-1549.).

Although genotype TX 25 presented intermediate root gall index and egg mass index values (3,66 and 1,83, respectively), it had a low RF (0.2) (Table 3). This indicates that the resistance mechanism present in this genotype interferes with the biology of female nematodes, decreasing their fecundity.

A resistance mechanism that affects the penetration, development and fecundity of female nematodes has been previously reported for other TX genotypes, also originating from Mexico (Faske & Starr, 2009Faske, T. R., & Starr, J. L. (2009). Mechanism of resistance to Meloidogyne incognita in resistant cotton genotypes. Nematropica, 39(2), 281-288. ). However, this is a slow mechanism, which allows nematodes to penetrate and become established in the root, and the decrease in nematode population occurs gradually over several nematode generations. Genotypes TX 25 and M315 are highly resistant to M. incognita (Starr & Mercer, 2010Starr, J. L., & Mercer, C. F. (2010). Development of Resistant Varieties. In R. N. Perry, M. Moens, & J. L. Starr (Eds.), Root-Knot nematodes (p. 326-337). Wallingford, EN: CAB International. ) and efficient in decreasing nematode populations.

According to Mendel’s first law, if the F1 generation is phenotypically similar to one of the genitors, that genitor is dominant relative to the other (Griffiths, Wessler, Lewontin, & Caroll, 2016Griffiths, A. J. S., Wessler, S., Lewontin, R., & Caroll, S. (2016) Herança monogênica. In A. J. S. Griffiths, S. Wessler, R. Lewontin, & S. Caroll (Eds.), Introdução a genética (p. 27-76). Rio de Janeiro, RJ: Guanabara Koogan. ). Segregation in the F1 generation occurs because the resistance in genitor TX 25 is associated with two alleles, and the haploid cells formed during gamete formation possess only one allele of each pair, half of the information of genitor TX 25 and half the information of genitor FiberMax 966. These results indicate that genotype TX 25 is dominant relative to FiberMax 966, resulting in an F1 generation that is 100% resistant. Resistance may therefore be monogenic. However, none of the ratios tested using the chi-squared test, were significant (Table 4). This may be due to the low number of plants in the F1 generation: seven plants do not appear to be sufficient to confirm the behavior of a generation. Therefore, the possibility of monogenic inheritance should not be discarded based only on the analysis of the results for the F1 generation.

According to the goodness-of-fit test, the phenotypic segregation for F2 did not fit a 3:1 or 1S:2MR:1R ratio and, therefore, does not indicate monogenic resistance (Table 4). The F2 generation fit a 9R:3MR:4S ratio, indicating oligogenic inheritance.

Table 4
Chi-squared (χ2) test for F1 and F2, originated in parental FiberMax 966 (♀) x TX 25(♂) segregation patterns based on the reproduction factor, considering one or two genes involved in the control of resistance, in the first experiment. Goiania, Goiás State, 2013.

The behavior of the F2 generation is presented in Figure 1. Most genotypes were classified as resistant, with RF values between 0.01 and six. Genotypes with RF values between 6.1 and 12 were classified as moderately resistant, and those with RF values greater than 12 were considered susceptible.

Figure 1
Frequency of reproduction factor of Meloidogyne incognita plants in the F2 generation cotton genotypes in the first experiment. Goiania, Goias State, 2015. *Genotypes with RF values between 0.01 and 1 = highly resistant; genotypes with RF values between 1.1 and 6.0 = resistant; genotypes with RF values between 6.1 and 12 = moderately resistant, and those with RF values greater than 12 were considered susceptible.

Cultivars LA887 and DeltaOpal have been previously classified as moderately resistant (Mota et al., 2013Mota, F. C., Alves, G. C. S., Giband, M., Gomes, A. C. M. M., Sousa, F. R., Mattos, V. S., … Carneiro, R. M. D. G. (2013). New sources of resistance to Meloidogyne incognita race 3 in wild cotton accessions and histological characterization of the defence mechanisms. Plant Pathology, 62(5), 1173-1183.). However, according to the classification of Starr and Mercer (2010Starr, J. L., & Mercer, C. F. (2010). Development of Resistant Varieties. In R. N. Perry, M. Moens, & J. L. Starr (Eds.), Root-Knot nematodes (p. 326-337). Wallingford, EN: CAB International. ) adopted in this study, these cultivars were classified as resistant, presenting percentage decrease in the reproduction factor of 8.34 and 14.12% for LA887 and DeltaOpal, respectively (Table 3).

The genes for M. incognita resistance in cotton are located on chromosome 11 (Wang, Ulloa, & Roberts, 2006Wang, C., Ulloa, M., & Roberts, P. A. (2006). Identification and mapping of microsatellite markers linked to a root-knot nematode resistance gene (rkn1) in Acala NemX cotton (Gossypium hirsutum L.). Theoretical and Applied Genetics , 112(4), 770-777. ) and chromosome 14 (Ynturi, Jenkins, Mccarty, Gutiérrez, & Sasha, 2006Ynturi, P., Jenkins, J. N., Mccarty, J. C., Gutiérrez, O. A., & Sasha, S. (2006). Association of root knot nematode resistance gene with simple sequence repeat markers on two chromosomes in cotton. Crop Science, 46(3), 2670-2674.). The gene on chromosome 14 plays a role in polygenic resistance expression (Ynturi et al., 2006). The resistance mechanism in DeltaOpal is slow, as it allows nematode juveniles to penetrate the roots, establish their feeding site, inject the toxins responsible for cell hyperplasia and hypertrophy, cause galls, and cause disease to some degree. In LA887 this moderate resistance originates from accession Clevewilt 6, which presents a recessive resistance gene (Robinson, Bridges, & Percival, 2004Robinson, A. F.; Bridges, A. C., & Percival, A. E. (2004). New sources of resistance to the reniform (Rotylenchulus reniformis) and root-knot (Meloidogyne incognita) nematode in upland (Gossypium hirsutum) and sea island (G. barbadense) cotton. Journal of Cotton Science, 8(3), 191-197.). Although M315 and LA 887 had one genitor in common, they presented different behaviors.

It was recently demonstrated that cotton plants that were sensitive to M. incognita induced to express the MIC-3 protein (Meloidogyne Induced Cotton 3), become resistant to M. incognita and reduced egg production, although galls have not been reduced compared with the sensitive plants (Wubben, Callahan, Velten, Burke, & Jenkins, 2015Wubben, M. J., Callahan, F. E., Velten, J., Burke, J. J., & Jenkins, J. N. (2015). Overexpression of MIC-3 indicates a direct role for the MIC gene family in mediating Upland cotton (Gossypium hirsutum) resistance to root-knot nematode (Meloidogyne incognita). Theoretical and Applied Genetics 128(2), 199-209.). The reduction of egg production without a concomitant reduction in the galls, suggest that the MIC 3 is somehow mediated resistance gene on chromosome 14 (Wubben et al., 2015), which has a similar effect. This protein seems to be comum or exclusive the genus Gossypium (Wubben, Callahan, Hayes, & Jenkins, 2008). The quantity of MIC-3 protein produced in the tissue increases the infected root according to the increased resistance to M. incognita level (Davis & Stetina, 2016Davis, R. F., & Stetina, S. R. (2016). Resistance and tolerance to nematodes in cotton. In R. Galbieri & J. L. Belot (Ed.), Nematoides fitoparasitas do algodoeiro nos cerrados brasileiros: Biologia e medidas de controle (p. 166-243). Mato Grosso, MT: IMAMT.).

The mechanism of action of the MIC-3 explains the behavior of the LA887 and M315 genotypes in this study. For these genotypes showed lower rates of eggs index and higher galls index, probably showing that the MIC-3 is present in the LA 887 and M315 in moderate amounts, then have moderate resistance.

Similar to the observed results in the first experiment, most genotypes from the F2 generation in the second experiment were found to be highly resistant (Figure 2). The histograms plotted for the two experiments (Figures 1 and 2), together with the goodness-of-fit test performed in the first experiment, indicate that the plants present oligogenic inheritance. Considering that there are two genes involved in the control of resistance and that they are located on different chromosomes, an independent distribution of these two genes can be expected.

Figure 2
Frequency of reproduction factor of Meloidogyne incognita in plants in the F2 generation cotton genotypes in the second experiment. Goiania, Goiás State, 2015. *Genotypes with RF values between 0.01 and 1 = highly resistant; genotypes with RF values between 1.1 and 6.0 = resistant; genotypes with RF values between 6.1 and 12 = moderately resistant, and those with RF values greater than 12 were considered susceptible.

Polygenic and oligogenic resistance are interesting and necessary tools for plant disease management. Although they result in different levels of resistance, from high susceptibility to high resistance, they are more stable than monogenic resistance.

Assuming the same environmental and genetic conditions, genetic changes in several pathogenicity loci are needed for pathogens to overcome plant resistance and become virulent. The cotton genotypes tested in this study likely present oligogenic resistance, which tends to decrease disease severity in cultivated areas, and their inclusion in improvement programs is recommended.

Conclusion

Genotype TX 25 presents resistance against M. incognita race 3. Genotype M315 presents resistance against M. incognita race 3. The genetic control of M. incognita race 3 resistance in genotype TX 25 is predominantly oligogenic. The F2 generation genotypes present oligogenic resistance to M. incognita.

Acknowledgements

We thank the National Council for Scientific and Technological Development (Conselho Nacional de Desenvolvimento Científico e Tecnológico - CNPq) for granting a scholarship. We thank Prof. Dr. João Batista Duarte for help with the statistical analyses. We thank Dra Regina M.D.G Carneiro for being co-supervisor of this work. We thanks American Journal Experts for revised and edited this manuscript. We also thanks the Instituto Federal Goiano - Campus Urutaí for financial support.

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Publication Dates

  • Publication in this collection
    Sept 2017

History

  • Received
    04 July 2016
  • Accepted
    25 Oct 2016
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