RESUMO
BACKGROUND: A novel virulent bacteriophage infecting phytobacteria Pseudomonas cichorii (P. cichorii) was isolated from leafy vegetables in Brazil. P. cichorii is a Gram-negative soil phytobacterium, the causal agent of a number of economically important plant diseases worldwide. METHODS AND RESULTS: In this study, a new phage specific for P. cichorii was isolated from solid samples (lettuce, chicory and cabbage), designated vB_Pci_PCMW57. Electron microscopy revealed a small virion (~ 50-nm-diameter icosahedral capsid) with a short, non-contractile tail. The genome of vB_Pci_PCMW57 is 40,117 bp in size, with a GC content of 57.6% and encodes 49 open reading frames. The phage is genetically similar to P. syringae phages Pst_GM1 and Pst_GIL1, and the P. fluorescens phages WRT and KNP. According to electron microscopy and whole-genome sequence analysis, vB_Pci_PCMW57 should be classified as a Caudoviticetes, family Autographiviridae, subfamily Studiervirinae. CONCLUSIONS: The complete phage genome was annotated, and the sequence identity of the virus with other Pseudomonas viruses was higher than 95%. To our knowledge, this is the first report of a bacteriophage infecting Pseudomonas cichorii.
Assuntos
Bacteriófagos , Bacteriófagos/genética , Genoma Viral , Análise de Sequência de DNA , Pseudomonas/genética , Fases de Leitura Aberta/genética , FilogeniaRESUMO
The state of Santa Catarina is the second-largest producer of rice seeds in Brazil. Research on phytopathogenicbacterias in this crop is scarce and the high frequency of panicle diseases leads to the hypothesis that seeds may be infected by bacteria. This research quantified the incidence of bacteria in the seeds, verified the bacteria viability during the storage period and characterized the associated bacteria. Seeds from the 2018/19 and 2019/20 seasons were analyzed. To check the incidence, the seeds were disinfected, plated on a nutrient agar + fungicide culture medium, and incubated for seven days at 27 °C. To assess viability, every 45 days, three cultivars stored in a processing unit were subjected to the same detection methodology. To characterize, prevalent colonies were isolated on semi-selective culture medium Pantoea genus-specific agar (PGSA), where the ones that showed growth were subjected to deoxyribonucleic acid (DNA) extraction and Polymerase Chain Reaction (PCR), DNA sequencing, and sequence comparison on GenBank. The hypersensitivity reaction (HR) in tobacco was performed using a bacterial suspension of each isolate. All seed samples had an average incidence of 83%. During storage, the seeds maintained stable bacterial viability, with an average incidence of 95% at the beginning of storage and 99% at the end of it. All isolates that grew in PGSA culture medium were identified by molecular characterization with 100% identity with two specimens of Pantoeaananatis and one of them induced RH in tobacco.
O estado de Santa Catarina é o segundo maior produtor de sementes de arroz do Brasil. As pesquisas com bactérias fitopatogênicas nesta cultura são escassas e a alta frequência de doenças da panícula leva à hipótese de que sementes podem estar infectadas por bactérias. O objetivo desta pesquisa foi quantificar a incidência de bactérias nas sementes, verificar a viabilidade das bactérias durante o período de armazenamento e caracterizar as bactérias associadas. Foram analisadas sementes das safras 2018/19 e 2019/20. Para verificar a incidência, as sementes foram desinfestadas, plaqueadas em meio de cultura ágar nutriente + fungicida e incubadas por sete dias a 27 °C. Para avaliar a viabilidade, a cada 45 dias, três cultivares armazenadas em uma unidade de beneficiamento foram submetidas à mesma metodologia de detecção. Para caracterizar, colônias prevalentes foram isoladas em meio de cultura semisseletivo Pantoea genus-specific ágar (PGSA), onde as que apresentaram crescimento foram submetidas à extração do ácido desoxirribonucléico (DNA) e Reação em Cadeia da Polimerase (PCR), sequenciamento do DNA e comparação de sequências no GenBank. A reação de hipersensibilidade (HR) em tabaco foi realizada utilizando uma suspensão bacteriana de cada isolado. Todas as amostras de sementes apresentaram incidência média de 83%. Durante o armazenamento, as sementes mantiveram viabilidade bacteriana estável, com incidência média de 95% no início do armazenamento e 99% ao fim. Todos os isolados que cresceram no meio de cultura PGSA, foram identificados por caracterização molecular com 100% de identidade com dois espécimes de Pantoea ananatis e um deles induziu HR em tabaco.
Assuntos
Oryza/parasitologia , Sementes/parasitologia , Pantoea/patogenicidadeRESUMO
ABSTRACT: The state of Santa Catarina is the second-largest producer of rice seeds in Brazil. Research on phytopathogenicbacterias in this crop is scarce and the high frequency of panicle diseases leads to the hypothesis that seeds may be infected by bacteria. This research quantified the incidence of bacteria in the seeds, verified the bacteria viability during the storage period and characterized the associated bacteria. Seeds from the 2018/19 and 2019/20 seasons were analyzed. To check the incidence, the seeds were disinfected, plated on a nutrient agar + fungicide culture medium, and incubated for seven days at 27 °C. To assess viability, every 45 days, three cultivars stored in a processing unit were subjected to the same detection methodology. To characterize, prevalent colonies were isolated on semi-selective culture medium Pantoea genus-specific agar (PGSA), where the ones that showed growth were subjected to deoxyribonucleic acid (DNA) extraction and Polymerase Chain Reaction (PCR), DNA sequencing, and sequence comparison on GenBank. The hypersensitivity reaction (HR) in tobacco was performed using a bacterial suspension of each isolate. All seed samples had an average incidence of 83%. During storage, the seeds maintained stable bacterial viability, with an average incidence of 95% at the beginning of storage and 99% at the end of it. All isolates that grew in PGSA culture medium were identified by molecular characterization with 100% identity with two specimens of Pantoeaananatis and one of them induced RH in tobacco.
RESUMO: O estado de Santa Catarina é o segundo maior produtor de sementes de arroz do Brasil. As pesquisas com bactérias fitopatogênicas nesta cultura são escassas e a alta frequência de doenças da panícula leva à hipótese de que sementes podem estar infectadas por bactérias. O objetivo desta pesquisa foi quantificar a incidência de bactérias nas sementes, verificar a viabilidade das bactérias durante o período de armazenamento e caracterizar as bactérias associadas. Foram analisadas sementes das safras 2018/19 e 2019/20. Para verificar a incidência, as sementes foram desinfestadas, plaqueadas em meio de cultura ágar nutriente + fungicida e incubadas por sete dias a 27 °C. Para avaliar a viabilidade, a cada 45 dias, três cultivares armazenadas em uma unidade de beneficiamento foram submetidas à mesma metodologia de detecção. Para caracterizar, colônias prevalentes foram isoladas em meio de cultura semisseletivo Pantoea genus-specific ágar (PGSA), onde as que apresentaram crescimento foram submetidas à extração do ácido desoxirribonucléico (DNA) e Reação em Cadeia da Polimerase (PCR), sequenciamento do DNA e comparação de sequências no GenBank. A reação de hipersensibilidade (HR) em tabaco foi realizada utilizando uma suspensão bacteriana de cada isolado. Todas as amostras de sementes apresentaram incidência média de 83%. Durante o armazenamento, as sementes mantiveram viabilidade bacteriana estável, com incidência média de 95% no início do armazenamento e 99% ao fim. Todos os isolados que cresceram no meio de cultura PGSA, foram identificados por caracterização molecular com 100% de identidade com dois espécimes de Pantoea ananatis e um deles induziu HR em tabaco.
RESUMO
Pectobacterium is a complex taxon of strains with diverse characteristics. It comprises several genera, including Erwinia, Brenneria, Pectobacterium, Dickeya, and Pantoea. Pectobacterium and Dickeya cause diseases in a wide range of plants, including potatoes, where they are causative agents of soft rot in tubers and blackleg in field-grown plants.Characterizing Pectobacterium species allows for the analysis of the diversity of pectinolytic bacteria, which may support control strategies for plant bacterial diseases. The aim of this study was to perform biochemical, physiological, and molecular characterizations of Pectobacteriumspp. from different sites and host plants. The isolated strains were characterized by the glucose fermentation test, Gram staining, catalase activity, oxidase activity, growth at 37 ºC, reducing substances from sucrose, phosphatase activity, indole production, acid production from different sources (sorbitol, melibiose, citrate, and lactose), pathogenicity in potato, and hypersensitivity reactions. Molecular characterization was performed with species-specific primers ECA1f/ECA2r and EXPCCF/EXPCCR, which identify P.atrosepticum and P.carotovorum subsp. carotovorum (Pcc), respectively, and with primers 1491f/L1RA/L1RG and Br1f/L1RA/L1RG that differentiate Pcc from Dickeya chrysanthemi and from P. carotovorum subsp. brasiliensis. The strains were identified as belonging to the genus Pectobacterium, though they did not fit the biochemical nor the molecular classification standards for subspecies differentiation, indicating significant diversity among the strains.
Pectobacterium é um táxon complexo de isolados bacterianos com características diversas. Compreende vários gêneros como Erwinia, Brenneria, Pectobacterium, Dickeya e Pantoea. Pectobacterium e Dickeya causam doenças em ampla variedade de plantas, incluindo a batateira, na qual são os agentes etiológicos da podridão mole dos tubérculos e da canela-preta de plantas cultivadas em campo.A caracterização de espécies de Pectobacterium permite a análise da diversidade de bactérias pectolíticas, podendo auxiliar estratégias de controle de doenças bacterianas em plantas. O objetivo deste trabalho foi caracterizar bioquímica, fisiológica e molecularmente isolados de Pectobacterium sp. provenientes de diferentes locais e hospedeiros. Os isolados foram caracterizados pelos testes de fermentação de glicose, Gram, catalase, oxidase, crescimento à 37 ºC, redução de substâncias a partir de sacarose, atividade da fosfatase, produção de indol, produção de ácido a partir de sorbitol, melibiose, citrato e lactose, patogenicidade em batata e reação de hipersensibilidade. Para a caracterização molecular, foram utilizados os pares de primersECA1f/ECA2r e EXPCCF/EXPCCR [específicos para P. atrosepticum e P.carotovorum subsp. carotovorum(Pcc), respectivamente] e as tríades de primers 1491f/L1RA/L1RG e Br1f/L1RA/L1RG, para diferenciar Pcc de Dickeya chrysanthemi e de P. carotovorum subsp. brasiliensis. Os isolados foram identificados como pertencentes ao gênero Pectobacterium, no entanto, não se enquadraram na classificação bioquímica e tampouco molecular para diferenciação das subespécies, demonstrando a grande diversidade dos mesmos.
Assuntos
Solanum tuberosum , Reação em Cadeia da Polimerase , PectobacteriumRESUMO
The increased use of pesticides applied to treat diseases caused by bacteria has caused serious environmental problems. There are few fungicides/bactericides for the treatment of plant diseases caused by Xanthomonas campestris pv. campestris (Xcc), and only two natural products with general bactericidal/fungicidal use are available on the market. Thus, this study evaluated the antimicrobial activity of essential oils (EOs), and their combinations, from five distinct genotypes of Cordia curassavica (Jacq.) Roem. & Schult (Syn. Varronia curassavica Jacq.) (CCUR) against Xcc. GC/MS chemical analysis revealed α-pinene, sabinene, (E)-caryophyllene, ar-curcumene, ß-sesquiphellandrene, 7-cyclodecen-1-one, and ar-Turmerone as the major compounds of the five EOs of CCUR. All EOs showed growth inhibition of Xcc with minimum inhibitory concentration between 500 and 1000 µg mL-1. The associations between two EOs from different CCUR genotypes showed that 70% of the total combinations had an additive effect. However, the combinations between CCUR-002 × (-302, -202) and CCUR-302 × (-601) showed a synergistic effect, with mean fractional inhibitory concentration FIC50 values of 0.28, 0.42, and 0.40, respectively. This study demonstrates that combinations of C. curassavica EOs have antimicrobial activity and a potential to be used in the control of black rot. Graphical abstract.
Assuntos
Antibacterianos/farmacologia , Cordia/química , Óleos Voláteis/farmacologia , Óleos de Plantas/farmacologia , Xanthomonas campestris/efeitos dos fármacos , Testes de Sensibilidade Microbiana , Doenças das Plantas/microbiologia , Doenças das Plantas/prevenção & controleRESUMO
ABSTRACT The 16S-23S rDNA spacer region was evaluated as a molecular marker to differentiation of orchids pathogens, Acidovorax avenae subsp. cattleyae and Burkholderia gladioli pv. gladioli. Other species belonging to the two genera such as B. gladioli pv. alliicola, A. avenae subsp. avenae, A. avenae subsp. citrulli, A. anthurii, A. facilis, A. delafieldii and A. konjaci were also analyzed. The PCR amplification of the 16S-23S rDNA spacer region produced a fragment of 1,100 base pairs. The products obtained from all strains were digested with Afa I, Alu I, Hae III and Hpa II and the results showed distinct RFLP patterns for each endonuclease tested. The sequences of 16S-23S rDNA spacer region were aligned and the phylogenetic analysis confirmed the differences between A. avenae subsp. cattleyae e B. gladioli pv. gladioli. The PCR-RFLP technique was very efficient and useful to the identification of these pathogens since they cause very similar symptoms in orchids.
RESUMO A região espaçadora 16S-23S DNAr foi avaliada como marcador molecular para a diferenciação dos patógenos de orquídeas, Acidovorax avenae subsp. cattleyae e Burkholderia gladioli pv. gladioli. Outras espécies pertencentes a esses dois gêneros como B. gladioli pv. alliicola, A. avenae subsp. avenae, A. avenae subsp. citrulli, A. anthurii, A. facilis, A. delafieldii e A. konjaci também foram analisadas. A amplificação por PCR dessa região produziu um fragmento de aproximadamente 1.100 pares de bases para todas as linhagens testadas. Os produtos obtidos foram submetidos a digestões com as enzimas Afa I, Alu I, Hae III e Hpa II e os resultados mostraram perfis distintos de RFLP para A. avenae subsp. cattleyae de B. gladioli pv. gladioli com todas as endonucleases testadas. As seqüências da região espaçadora 16S-23S DNAr foram alinhadas e a análise filogenética confirmou as diferenças entre A. avenae subsp. cattleyae e B. gladioli pv. gladioli. A técnica de PCR-RFLP mostrouse eficiente e muito útil para a identificação desses patógenos, uma vez que eles causam sintomas muito semelhantes em orquídeas.