Characterization of the soybean genome in regions surrounding two loci for resistance to soybean mosaic virus

Hayes, Alec J.

11 August 1998

Soybean mosaic virus (SMV), has been the cause of numerous and often devastating disease epidemics, causing reduction in both the quality and quantity of soybeans worldwide. Two important genes for resistance to SMV are Rsv1 and Rsv4. Alleles at the Rsv1 locus have been shown to control resistance to all but the most virulent strain of SMV. This locus has been mapped previously to the soybean F linkage group. Rsv4 is an SMV resistance locus independent of Rsv1 and confers resistance to all strains of SMV. This locus has not been mapped previously. The purpose of this study is to investigate the two genomic regions that contain these vitally important resistance genes. A population of 281 F2 individuals that had previously been genotyped for reaction to SMV was evaluated in a mapping study which combined bulk segregant analysis with Amplified Fragment Length Polymorphism (AFLP). A Rsv4-linked marker, R4-1, was identified that mapped to soybean linkage group D1b using a reference mapping population. More than 40 markers were mapped in the Rsv4 segregating population including eleven markers surrounding Rsv4. This will provide the necessary framework for the fine mapping of this important genetic locus. Previous work has located Rsv1 to a genomic region containing several important resistance genes including Rps3, Rpg1, and Rpv. An RFLP probe, NBS5, whose sequence closely resembles that of several cloned plant disease resistance genes has been mapped to this chromosomal region. The efficacy of using this sequence to identify potential disease resistance genes was assessed by screening a cDNA library to uncover a candidate disease resistance gene which corresponds to this NBS5 sequence. Two related sequence classes were identified that correspond to NBS5. Interestingly, one class corresponds to a full length gene closely resembling other previously cloned disease resistance genes offering evidence that this NBS5-derived clone is a candidate disease resistance gene. A new marker technique was developed by combining the speed and efficiency of AFLP with DNA sequence information from cloned disease resistance genes. Using this strategy, three new markers tightly linked to Rsv1 were identified. One of these markers, which maps 0.6 cM away from Rsv1, has motifs consistent with other cloned disease resistance genes, providing evidence that this approach is an efficient method for targeting genomic regions where disease resistance genes are located. / Ph. D.

gene cloning

gene mapping

plant disease resistance

AFLP

nucleotide binding site (NBS)

leucine rich repeat (LRR)

Indução de resistência em plantas de berinjela e tomate por Lentinula edodes e Agaricus blazei contra bactérias causadoras de murcha (Ralstonia solanacearum) e cancro (Clavibacter michiganensis subsp. michiganensis) / Induced resistance by Lentinula edodes and Agaricus blazei in tomato plant and eggplant against bacterial wilt (Ralstonia solanacearum) solanacearum) and bacterial canker (Clavibacter michiganensis subsp. michiganensis)

Silva, Ricardo Ferrari

20 April 2007

Devido ao aumento da preocupação com o impacto dos agrotóxicos no meio ambiente e na saúde humana, busca-se uma agricultura sustentável. É no âmbito dessa questão que a resistência induzida torna-se uma ferramenta fundamental no manejo integrado de doenças e indispensável para uma nova agricultura, mais racional e sustentável. Dentre os diversos agentes bióticos e abióticos, utilizados em trabalhos de indução de resistência de plantas a patógenos, os cogumelos Lentinula edodes e Agaricus blazei vem sendo pesquisados. Desse modo, este trabalho teve como objetivos avaliar o efeito de diferentes isolados de L. edodes e A. blazei e do acibenzolar-S-metil (aSm) in vitro contra as bactérias e o controle de doenças de importância econômica para as culturas do tomate e da berinjela, em casa-de-vegetação. Depois de obtida a proteção, estudar os possíveis mecanismos bioquímicos ativados nas plantas através do uso dos extratos dos cogumelos e buscar a purificação parcial destes extratos, a fim de identificar o(s) princípio(s) ativo(s). No patossistema berinjela/Ralstonia, os extratos aquosos dos cogumelos não exerceram nenhum efeito direto sobre o patógeno, sendo que os isolados Abl-11 e Abl-28 de de A. blazei reduziram significativamente a ocorrência de folhas murchas das plantas em casa-devegetação, em relação aos demais tratamentos. Ocorreu um aumento na atividade da peroxidase, fenilalanina amônia-liase e polifenoloxidase nas folhas tratadas. O preciptado 60-80% obtido pela precipitação com sulfato de amônia e a fração 4 da cromatografia de troca aniônica (CTA) de Abl-28 reduziram a ocorrência de folhas murchas, sendo que a separação eletroforética revelou a presença de uma banda no gel com aproximadamente 29 kDa nesta fração. Em tomate, os extratos aquosos dos isolados dos cogumelos e o acibenzolar-S-metil não exerceram nenhum efeito inibitório in vitro no crescimento de Ralstonia solanacearum e Clavibacter michiganensis subsp. michiganensis. Porém, os isolados Abl-26 de A. blazei, Le-96/17 de L. edodes e aSm foram os que conferiram maior proteção das plantas de tomates contra os patógenos, diminuindo a ocorrência de folhas murchas, proporcionando um aumento na atividade da peroxidase no patossistema tomate/Ralstonia e um aumento na atividade de peroxidase, quitinase, fenilalanina amônia-liase e polifenoloxidase no patossistema tomate/Clavibacter. O preciptado 40-80% de Le-96/17 foi submetido à CTA, obtendo-se seis frações protéicas. As frações 3 e 4, junto com aSm e o extrato aquoso de Le-96/17 reduziram a ocorrência de folhas murchas. A separação eletroforética destas frações da CTA, do preciptado 40-80% e do extrato aquoso de Le-96/17 revelaram a presença de mais de uma banda no gel na fração 3 e 4 da CTA, no preciptado 40-80% e no extrato aquoso bruto de Le-96/17. Com base nos resultados, os cogumelos A. blazei e L. edodes apresentam compostos que induziram resistência em plantas berinjela e tomate, podendo auxiliar no controle de doenças. / Because the increase of the impact of chemical products in the environment and in human health, a search by sustainable agriculture is needed. It is in the scope of this problem that the induced resistance becomes a tool in the integrated management of pests and diseases and indispensable for a new agriculture, more rational and sustainable. Among the biotic and abiotic agents used to induce resistance, the mushrooms Lentinula edodes and Agaricus blazei have being studied. Thus, the objectives of the present work were evaluate the effects of different isolates of L. edodes and A. blazei and of the acibenzolar-S-methyl (aSm) on in vitro bacterial growth and the control of the diseases in tomato and eggplant under greenhouse conditions. The studies also tried to elucidate the mode of action of the extracts from the fruiting bodies and partially purify them. In eggplant plants, the aqueos extracts from the different mushroom isolates did not have any direct effect on the pathogen. The isolates Abl-11 and Abl-28 of A. blazei reduced the wilt in eggplant leaves, under greenhouse conditions, and increased peroxidase, phenylalanine ammonia-lyase and polyphenoloxidase activities in treated leaves. The fraction of aqueous extract of A. blazei (Abl-28) obtained with ammonium sulfhate and fraction 4 from anion exchange chromatography reduced bacterial wilt and a protein fraction exhibiting molecular mass around 29 kDa was obtained. In tomato plants, the aqueos extracts from the different mushrooms and the acibenzolar-S-methyl did not inhibit in vitro growth of Ralstonia solanacearum and Clavibacter michiganensis subsp. michiganensis. However, the isolates Abl-26 of A. blazei, Le-96/17 of L. edodes and aSm protected tomato plants against the bacterial pathogens, reducing the wilt and causing an increase in peroxidase activity in the tomato/Ralstonia interaction and an increase in peroxidase, chitinase, phenylalanine ammonialyase and polyphenoloxidase activities in the tomato/Clavibacter interaction. The ammonium sulphate fraction of Le-96/17 was submitted to anion exchange chromatography, and the proteins from fractions 3 and 4, aSm and the aqueous extract of Le-96/17 reduced the occurrence of wilt in the leaves. A protein fraction exhibiting proteins with molecular mass around 29, 37 and 45 kDA was obtained in fractions 3 and 4. Thus, the results showed that the mushrooms A. blazei and L. edodes edodes have substances that induce resistance in eggplant and tomato plants.

Bactérias fitopatogênicas

Berinjela

Canker (plant disease - resistance)

Chromatography

Cogumelos comestíveis

Cromatografia

Edible mushrooms

Eggplant

Phytopathogenic bacteria

Tomate

Tomato

Wilt (plant disease - resistance)

Indução de resistência em plantas de berinjela e tomate por Lentinula edodes e Agaricus blazei contra bactérias causadoras de murcha (Ralstonia solanacearum) e cancro (Clavibacter michiganensis subsp. michiganensis) / Induced resistance by Lentinula edodes and Agaricus blazei in tomato plant and eggplant against bacterial wilt (Ralstonia solanacearum) solanacearum) and bacterial canker (Clavibacter michiganensis subsp. michiganensis)

Ricardo Ferrari Silva

20 April 2007

Devido ao aumento da preocupação com o impacto dos agrotóxicos no meio ambiente e na saúde humana, busca-se uma agricultura sustentável. É no âmbito dessa questão que a resistência induzida torna-se uma ferramenta fundamental no manejo integrado de doenças e indispensável para uma nova agricultura, mais racional e sustentável. Dentre os diversos agentes bióticos e abióticos, utilizados em trabalhos de indução de resistência de plantas a patógenos, os cogumelos Lentinula edodes e Agaricus blazei vem sendo pesquisados. Desse modo, este trabalho teve como objetivos avaliar o efeito de diferentes isolados de L. edodes e A. blazei e do acibenzolar-S-metil (aSm) in vitro contra as bactérias e o controle de doenças de importância econômica para as culturas do tomate e da berinjela, em casa-de-vegetação. Depois de obtida a proteção, estudar os possíveis mecanismos bioquímicos ativados nas plantas através do uso dos extratos dos cogumelos e buscar a purificação parcial destes extratos, a fim de identificar o(s) princípio(s) ativo(s). No patossistema berinjela/Ralstonia, os extratos aquosos dos cogumelos não exerceram nenhum efeito direto sobre o patógeno, sendo que os isolados Abl-11 e Abl-28 de de A. blazei reduziram significativamente a ocorrência de folhas murchas das plantas em casa-devegetação, em relação aos demais tratamentos. Ocorreu um aumento na atividade da peroxidase, fenilalanina amônia-liase e polifenoloxidase nas folhas tratadas. O preciptado 60-80% obtido pela precipitação com sulfato de amônia e a fração 4 da cromatografia de troca aniônica (CTA) de Abl-28 reduziram a ocorrência de folhas murchas, sendo que a separação eletroforética revelou a presença de uma banda no gel com aproximadamente 29 kDa nesta fração. Em tomate, os extratos aquosos dos isolados dos cogumelos e o acibenzolar-S-metil não exerceram nenhum efeito inibitório in vitro no crescimento de Ralstonia solanacearum e Clavibacter michiganensis subsp. michiganensis. Porém, os isolados Abl-26 de A. blazei, Le-96/17 de L. edodes e aSm foram os que conferiram maior proteção das plantas de tomates contra os patógenos, diminuindo a ocorrência de folhas murchas, proporcionando um aumento na atividade da peroxidase no patossistema tomate/Ralstonia e um aumento na atividade de peroxidase, quitinase, fenilalanina amônia-liase e polifenoloxidase no patossistema tomate/Clavibacter. O preciptado 40-80% de Le-96/17 foi submetido à CTA, obtendo-se seis frações protéicas. As frações 3 e 4, junto com aSm e o extrato aquoso de Le-96/17 reduziram a ocorrência de folhas murchas. A separação eletroforética destas frações da CTA, do preciptado 40-80% e do extrato aquoso de Le-96/17 revelaram a presença de mais de uma banda no gel na fração 3 e 4 da CTA, no preciptado 40-80% e no extrato aquoso bruto de Le-96/17. Com base nos resultados, os cogumelos A. blazei e L. edodes apresentam compostos que induziram resistência em plantas berinjela e tomate, podendo auxiliar no controle de doenças. / Because the increase of the impact of chemical products in the environment and in human health, a search by sustainable agriculture is needed. It is in the scope of this problem that the induced resistance becomes a tool in the integrated management of pests and diseases and indispensable for a new agriculture, more rational and sustainable. Among the biotic and abiotic agents used to induce resistance, the mushrooms Lentinula edodes and Agaricus blazei have being studied. Thus, the objectives of the present work were evaluate the effects of different isolates of L. edodes and A. blazei and of the acibenzolar-S-methyl (aSm) on in vitro bacterial growth and the control of the diseases in tomato and eggplant under greenhouse conditions. The studies also tried to elucidate the mode of action of the extracts from the fruiting bodies and partially purify them. In eggplant plants, the aqueos extracts from the different mushroom isolates did not have any direct effect on the pathogen. The isolates Abl-11 and Abl-28 of A. blazei reduced the wilt in eggplant leaves, under greenhouse conditions, and increased peroxidase, phenylalanine ammonia-lyase and polyphenoloxidase activities in treated leaves. The fraction of aqueous extract of A. blazei (Abl-28) obtained with ammonium sulfhate and fraction 4 from anion exchange chromatography reduced bacterial wilt and a protein fraction exhibiting molecular mass around 29 kDa was obtained. In tomato plants, the aqueos extracts from the different mushrooms and the acibenzolar-S-methyl did not inhibit in vitro growth of Ralstonia solanacearum and Clavibacter michiganensis subsp. michiganensis. However, the isolates Abl-26 of A. blazei, Le-96/17 of L. edodes and aSm protected tomato plants against the bacterial pathogens, reducing the wilt and causing an increase in peroxidase activity in the tomato/Ralstonia interaction and an increase in peroxidase, chitinase, phenylalanine ammonialyase and polyphenoloxidase activities in the tomato/Clavibacter interaction. The ammonium sulphate fraction of Le-96/17 was submitted to anion exchange chromatography, and the proteins from fractions 3 and 4, aSm and the aqueous extract of Le-96/17 reduced the occurrence of wilt in the leaves. A protein fraction exhibiting proteins with molecular mass around 29, 37 and 45 kDA was obtained in fractions 3 and 4. Thus, the results showed that the mushrooms A. blazei and L. edodes edodes have substances that induce resistance in eggplant and tomato plants.

Bactérias fitopatogênicas

Berinjela

Cogumelos comestíveis

Cromatografia

Tomate

Canker (plant disease - resistance)

Chromatography

Edible mushrooms

Eggplant

Phytopathogenic bacteria

Tomato

Wilt (plant disease - resistance)

Polimorfismos de seqüência nucleotídica em fragmentos genômicos de cana-de-açúcar homólogos a genes de resistência. / Single nucleotide polymorphims in genomic fragments of sugarcane homologous to resistance genes.

Quirino, Mariana Senna

06 June 2003

Este trabalho objetivou investigar a existência de polimorfismos de seqüência nucleotídica (SNPs "single nucleotide polymorphisms") em fragmentos genômicos de cana-de-açúcar homólogos a genes de resistência. Para tal, iniciadores sintéticos homólogos às extremidades de uma seqüência expressa identificada (ESTs "expressed sequence tag") como homóloga ao gene Xa1 de arroz (EST SCCCCL3080E03.g) e outra ao gene Rp1-D de milho (EST SCCCCL3080B03.g) foram utilizados para amplificar, em duplicata, fragmentos genômicos de variedades de cana-de-açúcar. Em seguida, os fragmentos foram clonados e seqüenciados. No caso do primeiro EST, foram obtidas seqüências de 119 insertos de uma variedade resistente (SP804966) e 156 de uma variedade suscetível (SP80180) a Xanthomonas albilineans. No segundo caso, foram obtidas seqüências de 167 insertos de uma terceira variedade resistente (R570) e 135 de outra suscetível (SP811763) a Puccinia melanocephala. Para cada EST considerado, as seqüências foram comparadas por meio do programa DNA Sequencher 3.0 (Gene Codes Corporation, Ann Arbor, MI). Nesta análise, somente foram consideradas seqüências reproduzíveis, isto é, que ocorreram nas duas repetições. No caso de ambos ESTs, a comparação de seqüências entre variedades possibilitou a identificação de quatro a seis fragmentos distintos. A comparação entre variedades, por sua vez, revelou a existência de até duas seqüências comuns. Presume-se que estas seqüências reproduzíveis e confirmadas por meio de digestões de clones representativos de cada uma com enzimas de restrição, correspondam a seqüências alélicas. Iniciadores foram sintetizados com base em polimorfismos encontrados entre os diferentes alelos. No entanto, tentativas de amplificar alelos específicos por meio destes iniciadores se revelaram infrutíferas. Tal insucesso deve-se possivelmente à condição polialélica da cana-de-açúcar, que faz com que polimorfismos entre dois alelos sejam compensados por monomorfismos entre estes e os demais alelos. Assim, a utilização de SNPs como marcadores moleculares baseados em PCR em cana-de- açúcar mostra-se mais complexa quando comparada a plantas diplóides. / The objective of this work was to investigate the existence of single nucleotide polymorphisms (SNPs) in genomic fragments homologous to resistance genes in sugarcane. For this purpose, primers were designed based on the sequence of the extremities of an identified expressed sequence tag (ESTs) similar to the Xa1 gene of rice (EST SCCCCL3080E03.g) and another to the maize Rp1-D gene (EST SCCCCL3080B03.g). These primers were used to amplify genomic fragments of sugarcane varieties in duplicate. The fragments were then cloned and sequenced. In the case of first EST, sequences of 119 inserts from a resistant variety (SP804966) and 156 from a susceptible variety (SP80180) to Xanthomonas albilineans were analyzed. In the case of the second EST, sequences of 167 inserts from a third variety (R570) and 135 of a fourth one (SP811763), resistant and susceptible respectively to Puccinia melanocephala, were analyzed. Sequences were compared using the program DNA Sequencher 3.0 (Gene Codes Corporation, Ann Arbor, MI). In this analysis, only reproducible sequences were considered, that is, sequences that occurred in both replicates. Four to six different sequences were identified within varieties whereas comparisons among varieties revealed the existence of up to two sequences in common. These reproducible sequences, which were further confirmed through digestion of representative clones with appropriate restriction enzymes, could correspond to allelic sequences. Primers were designed based on the SNPs detected among these so-called alleles. However, attempts to amplify specific alleles using these primers were unsuccessful. This could be due to the polyallelic condition of sugarcane in which polymorphisms between two alleles could be compensated by monomorphisms between these and other alleles. Thus the use of SNPs as PCR-based molecular markers is not as straightforward in sugarcane as in diploid species.

cana-de-açúcar

escapaldadura da folha

ferrugem (doença de planta)

genes

leaf scorch

nucleotídeos

nucleotides

plant disease resistance

plant varieties.

polimorfismo

polimorphism

resistência genética vegetal

rust

sugarcane

variedades vegetais.

Avaliação de agentes bióticos e abióticos na indução de resistência e no controle pós-colheita de antracnose (Colletotrichum gloeosporioides) em mamão (Carica papaya) / Evaluation of biotic and abiotic agents on the resistance induction and on the postharvest control of anthracnose (Colletotrichum gloeosporioides) in papaya fruits (Carica papaya)

Cia, Patricia

20 February 2006

Este trabalho teve como principais objetivos avaliar os efeitos dos agentes bióticos (Saccharomyces cerevisiae, Bacillus thuringiensis, Lentinula edodes e Agaricus blazei), e abióticos (UV-C, irradiação gama, acibenzolar-S-metil, quitosana, ácidos acético e salicílico) na proteção de mamões contra C. gloeosporioides, bem como estudar os mecanismos bioquímicos de resistência ativados no tecido vegetal, em resposta ao tratamento com os agentes de maior eficiência, além de investigar os efeitos destes sobre o desenvolvimento in vitro do fungo. Para tanto, mamões cv. Golden foram inoculados com C. gloeosporioides através de injeção subcuticular de 15 µL da suspensão de esporos e, após 10 h, tratados com os diferentes agentes bióticos e abióticos. Para avaliar a possibilidade de indução de resistência pelos agentes, mamões foram também inoculados após 24, 48 e 72 h dos tratamentos. Os frutos foram armazenados a 25 ºC / 80 %UR por 7 dias e, avaliados diariamente quanto a incidência e severidade da podridão. Ao final do período de armazenamento, efetuou-se a avaliação dos parâmetros físico-químicos (cor de casca e de polpa, firmeza, sólidos solúveis, pH e acidez total). Quando de interesse, as atividades de peroxidase, β-1,3-glucanase e quitinase foram também investigadas. In vitro, avaliou-se o crescimento micelial, a germinação de conídios e a esporulação do fungo em resposta aos diferentes tratamentos. Os resultados mostraram que a irradiação gama (0,75 e 1 kGy) reduziu a incidência e a severidade da antracnose. Não houve efeito da UV-C no controle da podridão e todas as doses testadas causaram danos na casca dos frutos. O acibenzolar-S-metil reduziu em mais de 50 % a incidência e a severidade da podridão, além de induzir a maior atividade das enzimas peroxidase, quitinase e β-1,3-glucanase, e não alterar as características físico-químicas dos frutos. O ácido acético, a 2,5 µL L-1, reduziu a severidade e a incidência das lesões nos frutos. A quitosana (1, 2 e 4 %) reduziu significativamente a severidade da antracnose, e a 4 % foi também eficiente em reduzir a incidência da podridão. Concentrações acima de 0,25 % suprimiram a esporulação de C. gloeosporioides nas lesões. No entanto, os frutos tratados com 2 e 4 % de quitosana não amadureceram normalmente, permanecendo com a coloração da casca verde até o final do período de armazenamento. S. cerevisiae (20 mg mL-1) e B. thuringiensis (7,5 mg mL-1), aplicadas 24 h antes da inoculação do patógeno, reduziram a incidência da antracnose nos frutos, mas não o acúmulo de proteínas relacionadas à patogênese. Os cogumelos (A. blazei e L. edodes) e o ácido salicílico não foram eficientes em reduzir a incidência e a severidade da antracnose. In vitro, a irradiação gama, a UV-C, os ácidos acético e salicílico, a quitosana, S. cerevisiae e L. edodes inibiram o crescimento micelial do fungo. A germinação de conídios foi reduzida pelas irradiações gama e UV-C, pelos ácidos acético e salicílico e pela quitosana. Esses resultados demonstram a possibilidade dos agentes estudados serem utilizados no manejo da antracnose, bem como na redução da utilização ou da dosagem de fungicidas empregados no controle da doença. / This work had as main objectives evaluate the effect of biotic and abiotic agents (Saccharomyces cerevisiae, Bacillus thuringiensis, Lentinula edodes and Agaricus blazei), and abiotic (UV-C, gamma irradiation, acibenzolar-S-methyl, chitosan, acetic and salicylic acids) on the protection of papaya fruits against C. gloeosporioides, and study the biochemical mechanisms of resistance activated in the tissues in response to the treatment with the agents exhibiting better efficiency. The effects of the agents on the in vitro development of the fungus were also investigated. For this, papaya fruits cv. Golden were inoculated with C. gloeosporioides through subcuticular injection of 15 µL of the spore suspension and after 10 h treated with the different biotic and abiotic agents. To evaluate the possibility of resistance induction by the different agents, fruits were also inoculated 24, 48 and 72 h after treatments. The fruits were stored at 25 ºC / 80 %RH for 7 days and evaluated daily for the incidence and severity of the anthracnose. At the end of the storage period, the evaluation of the physical-chemical parameters (skin and flesh color, firmness, total soluble solids, pH and tritatable acidity) was carried out. The peroxidase, β- 1,3-glucanase and chitinase activities were also investigated when need. In vitro, mycelial growth, conidium germination and sporulation of the fungus in response to the different treatments were also evaluated. The results showed that the gamma irradiation (0.75 and 1 kGy) reduced the anthracnose incidence and severity. The UV-C did not have effect on the control of the rot and all the doses caused damages in the skin of the fruits. The acibenzolar-S-methyl reduced in more than 50 % anthracnose incidence and severity, and induced the highest activity of peroxidase, chitinase and β-1,3-glucanase, and did not modify the physical-chemical characteristics of the fruits. The acetic acid at 2.5 µL L-1 reduced rot severity and incidence. The chitosan (1, 2 and 4 %) significantly reduced the rot severity, and at 4 % was also efficient in reducing anthracnose incidence. Chitosan concentrations above 0.25 % suppressed the sporulation of C. gloeosporioides in the lesions. However, the fruits treated with chitosan at 2 and 4 % did not ripen normally, remaining with green skin until the end of the storage period. S. cerevisiae (20 mg mL-1) and B. thuringiensis (7.5 mg mL-1), applied 24 h before the pathogen inoculation, reduced anthracnose incidence, but did not change the activities of pathogenesis related proteins. The mushrooms (A. blazei and L. edodes) and the salicylic acid were not efficient in reducing the incidence and the severity of anthracnose. In vitro, gamma irradiation, UV-C, acetic and salicylic acids, chitosan, S. cerevisiae and L. edodes inhibited the mycelial growth. The conidium germination was reduced by gamma and UV-C irradiation, acetic and salicylic acids and chitosan. These results show that these agents can be utilized for anthracnose management, and on the reduction in the use or dosage of fungicides utilized on the anthracnose control.

anthracnose

antracnose

biological control

controle biológico (fitossanidade)

controle físico

doença de planta – resistência

fisiologia pós-colheita

fungo fitopatogênico

mamão

papaya

phytopathogenic fungus

postharvest physiology

Avaliação de agentes bióticos e abióticos na indução de resistência e no controle pós-colheita de antracnose (Colletotrichum gloeosporioides) em mamão (Carica papaya) / Evaluation of biotic and abiotic agents on the resistance induction and on the postharvest control of anthracnose (Colletotrichum gloeosporioides) in papaya fruits (Carica papaya)

Patricia Cia

20 February 2006

Este trabalho teve como principais objetivos avaliar os efeitos dos agentes bióticos (Saccharomyces cerevisiae, Bacillus thuringiensis, Lentinula edodes e Agaricus blazei), e abióticos (UV-C, irradiação gama, acibenzolar-S-metil, quitosana, ácidos acético e salicílico) na proteção de mamões contra C. gloeosporioides, bem como estudar os mecanismos bioquímicos de resistência ativados no tecido vegetal, em resposta ao tratamento com os agentes de maior eficiência, além de investigar os efeitos destes sobre o desenvolvimento in vitro do fungo. Para tanto, mamões cv. Golden foram inoculados com C. gloeosporioides através de injeção subcuticular de 15 µL da suspensão de esporos e, após 10 h, tratados com os diferentes agentes bióticos e abióticos. Para avaliar a possibilidade de indução de resistência pelos agentes, mamões foram também inoculados após 24, 48 e 72 h dos tratamentos. Os frutos foram armazenados a 25 ºC / 80 %UR por 7 dias e, avaliados diariamente quanto a incidência e severidade da podridão. Ao final do período de armazenamento, efetuou-se a avaliação dos parâmetros físico-químicos (cor de casca e de polpa, firmeza, sólidos solúveis, pH e acidez total). Quando de interesse, as atividades de peroxidase, β-1,3-glucanase e quitinase foram também investigadas. In vitro, avaliou-se o crescimento micelial, a germinação de conídios e a esporulação do fungo em resposta aos diferentes tratamentos. Os resultados mostraram que a irradiação gama (0,75 e 1 kGy) reduziu a incidência e a severidade da antracnose. Não houve efeito da UV-C no controle da podridão e todas as doses testadas causaram danos na casca dos frutos. O acibenzolar-S-metil reduziu em mais de 50 % a incidência e a severidade da podridão, além de induzir a maior atividade das enzimas peroxidase, quitinase e β-1,3-glucanase, e não alterar as características físico-químicas dos frutos. O ácido acético, a 2,5 µL L-1, reduziu a severidade e a incidência das lesões nos frutos. A quitosana (1, 2 e 4 %) reduziu significativamente a severidade da antracnose, e a 4 % foi também eficiente em reduzir a incidência da podridão. Concentrações acima de 0,25 % suprimiram a esporulação de C. gloeosporioides nas lesões. No entanto, os frutos tratados com 2 e 4 % de quitosana não amadureceram normalmente, permanecendo com a coloração da casca verde até o final do período de armazenamento. S. cerevisiae (20 mg mL-1) e B. thuringiensis (7,5 mg mL-1), aplicadas 24 h antes da inoculação do patógeno, reduziram a incidência da antracnose nos frutos, mas não o acúmulo de proteínas relacionadas à patogênese. Os cogumelos (A. blazei e L. edodes) e o ácido salicílico não foram eficientes em reduzir a incidência e a severidade da antracnose. In vitro, a irradiação gama, a UV-C, os ácidos acético e salicílico, a quitosana, S. cerevisiae e L. edodes inibiram o crescimento micelial do fungo. A germinação de conídios foi reduzida pelas irradiações gama e UV-C, pelos ácidos acético e salicílico e pela quitosana. Esses resultados demonstram a possibilidade dos agentes estudados serem utilizados no manejo da antracnose, bem como na redução da utilização ou da dosagem de fungicidas empregados no controle da doença. / This work had as main objectives evaluate the effect of biotic and abiotic agents (Saccharomyces cerevisiae, Bacillus thuringiensis, Lentinula edodes and Agaricus blazei), and abiotic (UV-C, gamma irradiation, acibenzolar-S-methyl, chitosan, acetic and salicylic acids) on the protection of papaya fruits against C. gloeosporioides, and study the biochemical mechanisms of resistance activated in the tissues in response to the treatment with the agents exhibiting better efficiency. The effects of the agents on the in vitro development of the fungus were also investigated. For this, papaya fruits cv. Golden were inoculated with C. gloeosporioides through subcuticular injection of 15 µL of the spore suspension and after 10 h treated with the different biotic and abiotic agents. To evaluate the possibility of resistance induction by the different agents, fruits were also inoculated 24, 48 and 72 h after treatments. The fruits were stored at 25 ºC / 80 %RH for 7 days and evaluated daily for the incidence and severity of the anthracnose. At the end of the storage period, the evaluation of the physical-chemical parameters (skin and flesh color, firmness, total soluble solids, pH and tritatable acidity) was carried out. The peroxidase, β- 1,3-glucanase and chitinase activities were also investigated when need. In vitro, mycelial growth, conidium germination and sporulation of the fungus in response to the different treatments were also evaluated. The results showed that the gamma irradiation (0.75 and 1 kGy) reduced the anthracnose incidence and severity. The UV-C did not have effect on the control of the rot and all the doses caused damages in the skin of the fruits. The acibenzolar-S-methyl reduced in more than 50 % anthracnose incidence and severity, and induced the highest activity of peroxidase, chitinase and β-1,3-glucanase, and did not modify the physical-chemical characteristics of the fruits. The acetic acid at 2.5 µL L-1 reduced rot severity and incidence. The chitosan (1, 2 and 4 %) significantly reduced the rot severity, and at 4 % was also efficient in reducing anthracnose incidence. Chitosan concentrations above 0.25 % suppressed the sporulation of C. gloeosporioides in the lesions. However, the fruits treated with chitosan at 2 and 4 % did not ripen normally, remaining with green skin until the end of the storage period. S. cerevisiae (20 mg mL-1) and B. thuringiensis (7.5 mg mL-1), applied 24 h before the pathogen inoculation, reduced anthracnose incidence, but did not change the activities of pathogenesis related proteins. The mushrooms (A. blazei and L. edodes) and the salicylic acid were not efficient in reducing the incidence and the severity of anthracnose. In vitro, gamma irradiation, UV-C, acetic and salicylic acids, chitosan, S. cerevisiae and L. edodes inhibited the mycelial growth. The conidium germination was reduced by gamma and UV-C irradiation, acetic and salicylic acids and chitosan. These results show that these agents can be utilized for anthracnose management, and on the reduction in the use or dosage of fungicides utilized on the anthracnose control.

antracnose

controle biológico (fitossanidade)

controle físico

doença de planta – resistência

fisiologia pós-colheita

fungo fitopatogênico

mamão

anthracnose

biological control

papaya

phytopathogenic fungus

postharvest physiology

Polimorfismos de seqüência nucleotídica em fragmentos genômicos de cana-de-açúcar homólogos a genes de resistência. / Single nucleotide polymorphims in genomic fragments of sugarcane homologous to resistance genes.

Mariana Senna Quirino

06 June 2003

Este trabalho objetivou investigar a existência de polimorfismos de seqüência nucleotídica (SNPs "single nucleotide polymorphisms") em fragmentos genômicos de cana-de-açúcar homólogos a genes de resistência. Para tal, iniciadores sintéticos homólogos às extremidades de uma seqüência expressa identificada (ESTs "expressed sequence tag") como homóloga ao gene Xa1 de arroz (EST SCCCCL3080E03.g) e outra ao gene Rp1-D de milho (EST SCCCCL3080B03.g) foram utilizados para amplificar, em duplicata, fragmentos genômicos de variedades de cana-de-açúcar. Em seguida, os fragmentos foram clonados e seqüenciados. No caso do primeiro EST, foram obtidas seqüências de 119 insertos de uma variedade resistente (SP804966) e 156 de uma variedade suscetível (SP80180) a Xanthomonas albilineans. No segundo caso, foram obtidas seqüências de 167 insertos de uma terceira variedade resistente (R570) e 135 de outra suscetível (SP811763) a Puccinia melanocephala. Para cada EST considerado, as seqüências foram comparadas por meio do programa DNA Sequencher 3.0 (Gene Codes Corporation, Ann Arbor, MI). Nesta análise, somente foram consideradas seqüências reproduzíveis, isto é, que ocorreram nas duas repetições. No caso de ambos ESTs, a comparação de seqüências entre variedades possibilitou a identificação de quatro a seis fragmentos distintos. A comparação entre variedades, por sua vez, revelou a existência de até duas seqüências comuns. Presume-se que estas seqüências reproduzíveis e confirmadas por meio de digestões de clones representativos de cada uma com enzimas de restrição, correspondam a seqüências alélicas. Iniciadores foram sintetizados com base em polimorfismos encontrados entre os diferentes alelos. No entanto, tentativas de amplificar alelos específicos por meio destes iniciadores se revelaram infrutíferas. Tal insucesso deve-se possivelmente à condição polialélica da cana-de-açúcar, que faz com que polimorfismos entre dois alelos sejam compensados por monomorfismos entre estes e os demais alelos. Assim, a utilização de SNPs como marcadores moleculares baseados em PCR em cana-de- açúcar mostra-se mais complexa quando comparada a plantas diplóides. / The objective of this work was to investigate the existence of single nucleotide polymorphisms (SNPs) in genomic fragments homologous to resistance genes in sugarcane. For this purpose, primers were designed based on the sequence of the extremities of an identified expressed sequence tag (ESTs) similar to the Xa1 gene of rice (EST SCCCCL3080E03.g) and another to the maize Rp1-D gene (EST SCCCCL3080B03.g). These primers were used to amplify genomic fragments of sugarcane varieties in duplicate. The fragments were then cloned and sequenced. In the case of first EST, sequences of 119 inserts from a resistant variety (SP804966) and 156 from a susceptible variety (SP80180) to Xanthomonas albilineans were analyzed. In the case of the second EST, sequences of 167 inserts from a third variety (R570) and 135 of a fourth one (SP811763), resistant and susceptible respectively to Puccinia melanocephala, were analyzed. Sequences were compared using the program DNA Sequencher 3.0 (Gene Codes Corporation, Ann Arbor, MI). In this analysis, only reproducible sequences were considered, that is, sequences that occurred in both replicates. Four to six different sequences were identified within varieties whereas comparisons among varieties revealed the existence of up to two sequences in common. These reproducible sequences, which were further confirmed through digestion of representative clones with appropriate restriction enzymes, could correspond to allelic sequences. Primers were designed based on the SNPs detected among these so-called alleles. However, attempts to amplify specific alleles using these primers were unsuccessful. This could be due to the polyallelic condition of sugarcane in which polymorphisms between two alleles could be compensated by monomorphisms between these and other alleles. Thus the use of SNPs as PCR-based molecular markers is not as straightforward in sugarcane as in diploid species.

cana-de-açúcar

escapaldadura da folha

ferrugem (doença de planta)

genes

nucleotídeos

polimorfismo

resistência genética vegetal

variedades vegetais.

leaf scorch

nucleotides

plant disease resistance

plant varieties.

polimorphism

rust

sugarcane

Detection And Characterization Of Plant Genes Involved In Various Biotic And Abiotic Stress Conditions Using Ddrt-pcr And Isolation Of Interacting Proteins

Unver, Turgay

01 August 2008

The main objective of this thesis dissertation is functionally characterizing the genes involved in biotic and abiotic stresses of plants at molecular level. Previously, upon pathogen attack Rad6 gene expression was found to be changed in wheat and barley plants. To functionally characterize the Rad6 gene, VIGS (Virus induced gene silencing) system was used. HR (Hypersensitive response) like symptoms was detected in every silenced barley and wheat plants. To figure out, transcriptomes and proteomes of Rad6 silenced plants were analyzed. 2-D PAGE analysis was also performed on silenced and control wheat plants. No pathogen growth was observed in Rad6 silenced barley lines. Additionally, the susceptible wild type Arabidopsis plants showed resistant phenotype when any of the Rad6 gene copies is mutated. This suggests that Rad6 gene has a negative regulatory role in plant disease resistance which was proved for the first time. Yeast two hybrid protein interaction study suggests that RAD6 carrying out its function by interacting with SGT1 protein and regulating resistance related genes. It has been first time reported in this thesis that E2 (Ubiquitin conjugating enzyme) takes role in plant disease resistance. Boron which is the other consideration in the scope of thesis as an abiotic stress factor at a very limited amount is necessary for the normal development of plants. This study is conducted on highly boron tolerant Gypsophila perfoliata L. collected from a location in the boron mining area. The plant samples were tested in the presence of high boron (35 mg/kg) concentrations. The transcriptomes of the plant samples treated with the excess levels of boron to that of the samples grown under normal concentration were compared using differential display PCR method. Thirty bands showing differential expression levels at varying time points were analyzed. 18 of them were confirmed via qRT-PCR.

QK Plant Physiology 710-899

Investigation of Structure-function and Signal Transduction of Plant Cyclic Nucleotide-gated Ion Channels

Chin, Kimberley

07 January 2014

Cyclic nucleotide-gated channels (CNGCs) are non-selective cation channels that were first identified in vertebrate photosensory and olfactory neurons. Although the physiological roles and biophysical properties of animal CNGCs have been well studied, much less is known about these channels in plants. The Arabidopsis genome encodes twenty putative CNGC subunits that are postulated to form channel complexes that mediate various physiological processes involving abiotic and biotic stress responses, ion homeostasis and development. The identification of Arabidopsis autoimmune CNGC mutants, such as defense no death class (dnd1 and dnd2), and the constitutive expressor of pathogenesis related genes 22 (cpr22) implicate AtCNGC2, 4, 11 and 12 in plant immunity. Here, I present a comprehensive study of the molecular mechanisms involved in CNGC-mediated signaling pathways with emphasis on pathogen defense. Previously, a forward genetics approach aimed to identify suppressor mutants of the rare gain-of-function autoimmune mutant, cpr22, identified key residues that are important for CNGC subunit interactions and channel function. First, I present a structure-function analysis of one of these suppressor mutants (S58) that revealed a key residue in the cyclic nucleotide binding domain involved in the stable regulation of CNGCs. Second, I present a new suppressor screen using AtCNGC2 T-DNA knockout mutants that specifically aimed to identify novel downstream components of CNGC-mediated pathogen defense signaling. In this screen, I successfully isolated and characterized the novel Arabidopsis mutant, repressor of defense no death 1 (rdd1), and expanded this study to demonstrate its involvement in AtCNGC2 and AtCNGC4-mediated signal transduction. Additionally, I demonstrated for the first time, the physical interaction of AtCNGC2 and AtCNGC4 subunits in planta. The findings presented in this thesis broaden our current knowledge of CNGCs in plants, and provide a new foundation for future elucidation of the structure-function relationships and signal transduction mediated by these channels.

Arabidopsis thaliana

cyclic nucleotide gated channels

plant immunity

plant disease resistance

plant pathogen resistance

CNGC

calcium signaling

bimolecular fluorescence complementation

ion channel

signal transduction

calcium

map based cloning

plant autoimmune mutant

plant lesion mimic mutant

calmodulin

floral transition

rdd1

cpr22

dnd1

dnd2

CNGC11

CNGC12

CNGC2

CNGC4

suppressor screen

0309

0817

0307

Investigation of Structure-function and Signal Transduction of Plant Cyclic Nucleotide-gated Ion Channels

Chin, Kimberley

07 January 2014

Cyclic nucleotide-gated channels (CNGCs) are non-selective cation channels that were first identified in vertebrate photosensory and olfactory neurons. Although the physiological roles and biophysical properties of animal CNGCs have been well studied, much less is known about these channels in plants. The Arabidopsis genome encodes twenty putative CNGC subunits that are postulated to form channel complexes that mediate various physiological processes involving abiotic and biotic stress responses, ion homeostasis and development. The identification of Arabidopsis autoimmune CNGC mutants, such as defense no death class (dnd1 and dnd2), and the constitutive expressor of pathogenesis related genes 22 (cpr22) implicate AtCNGC2, 4, 11 and 12 in plant immunity. Here, I present a comprehensive study of the molecular mechanisms involved in CNGC-mediated signaling pathways with emphasis on pathogen defense. Previously, a forward genetics approach aimed to identify suppressor mutants of the rare gain-of-function autoimmune mutant, cpr22, identified key residues that are important for CNGC subunit interactions and channel function. First, I present a structure-function analysis of one of these suppressor mutants (S58) that revealed a key residue in the cyclic nucleotide binding domain involved in the stable regulation of CNGCs. Second, I present a new suppressor screen using AtCNGC2 T-DNA knockout mutants that specifically aimed to identify novel downstream components of CNGC-mediated pathogen defense signaling. In this screen, I successfully isolated and characterized the novel Arabidopsis mutant, repressor of defense no death 1 (rdd1), and expanded this study to demonstrate its involvement in AtCNGC2 and AtCNGC4-mediated signal transduction. Additionally, I demonstrated for the first time, the physical interaction of AtCNGC2 and AtCNGC4 subunits in planta. The findings presented in this thesis broaden our current knowledge of CNGCs in plants, and provide a new foundation for future elucidation of the structure-function relationships and signal transduction mediated by these channels.

Arabidopsis thaliana

cyclic nucleotide gated channels

plant immunity

plant disease resistance

plant pathogen resistance

CNGC

calcium signaling

bimolecular fluorescence complementation

ion channel

signal transduction

calcium

map based cloning

plant autoimmune mutant

plant lesion mimic mutant

calmodulin

floral transition

rdd1

cpr22

dnd1

dnd2

CNGC11

CNGC12

CNGC2

CNGC4

suppressor screen

0309

0817

0307