Étude transcriptionnelle d'une souche pathogène aviaire de Escherichia coli (APEC) et son mutant Pst (phosphate specific transport)

Crépin, Sébastien

January 2008

Mémoire numérisé par la Division de la gestion de documents et des archives de l'Université de Montréal.

Escherichia coli pathogène

Régulon Pho

Système Pst

Transcriptomique

Biopuces Affymetrix

Métabolisme bactérien

Réponse au stress

Pathogenic Escherichia coli

Pho regulon

Pst system

Transcriptome

Affymetrix GeneChip

Bacterial metabolism

Stress response

Escala diagramática para avaliação da mancha preta em folhas de citros e efeito da temperatura e da duração do molhamento na pré-penetração de conídios de Guignardia citricarpa Kiely [Phyllosticta citricarpa (McAlp.) Van der Aa]. / Diagrammatic scale for assessment of citrus black spot in leaves and effect of temperature and wetness duration in the pre-penetration conidia of Guignardia citricarpa Kiely [Phyllosticta citricarpa (McAlp.) Van der Aa].

Noronha, Marissônia de Araujo

21 January 2003

A mancha preta dos citros causada pelo fungo Guignardia citricarpa Kiely [Phyllosticta citricarpa (McAlp.) Van der Aa], possui duas formas de infecção, conídios e ascósporos. Informações a respeito da importância dos conídios na epidemiologia da doença são escassas ou controversas. Visando uma maior compreensão sobre o patossistema citros-G. citricarpa (P. citricarpa), os objetivos desta dissertação foram: elaborar e validar uma escala diagramática para avaliação da severidade da mancha preta em folhas de citros; verificar o efeito da temperatura e da duração do período de molhamento na formação de apressórios formados a partir de conídios; observar por meio de microscopia eletrônica de varredura a germinação de conídios e a formação de apressórios sobre folhas destacadas de limão 'Siciliano' submetidas a diferentes temperaturas e períodos de molhamento. A escala diagramática com níveis de severidade de 1; 3; 6; 12; e 24% de área foliar lesionada foi validada por dois grupos de avaliadores, com e sem experiência na quantificação de doenças. Comparada com a avaliação sem escala, o uso da escala proporcionou melhor precisão e acurácia tanto para avaliadores experientes como inexperientes, quando considerada a estimativa média dos mesmos. Na maioria dos casos, os desvios entre estimativas e severidade atual da doença foram mais evidentes para os níveis de severidade entre 5 e 15%. A reprodutibilidade das avaliações resultou em valores de R 2 mais uniformes para a maioria dos avaliadores experientes. Diferenças consideráveis de precisão foram observadas entre avaliadores inexperientes. O efeito da temperatura (10 o C - 40 o C) e da duração do molhamento (4 - 48 h) na formação de apressórios formados a partir de conídios de G. citricarpa (P. citricarpa) foi avaliado sob condições "in vitro" e sobre a superfície de folhas de limão 'Siciliano'. A formação de apressórios ocorreu em todas as temperaturas a partir de 12 horas de molhamento, sendo os extremos de temperatura (10 o C e 40 o C) menos favoráveis à formação de apressórios. A temperatura mínima para formação de apressórios, estimada pela função beta generalizada foi de 3 o C e a máxima de 48,4 o C, ambas para 48 horas de molhamento. A formação de apressórios foi consideravelmente favorecida pela duração do período de molhamento, com o máximo de apressórios formados a 24 horas de molhamento, para a maioria das temperaturas. O período de molhamento constituído de 48 horas foi essencial para que os esporos submetidos a temperaturas de 10 o C e 40 o C, formassem apressórios. A superfície de resposta obtida pela multiplicação das funções beta generalizada e monomolecular apresentou um ajuste satisfatório para os dados observados na estimativa da porcentagem relativa de apressórios formados (R 2 =0,75). As amostras observadas em microscopia eletrônica de varredura possibilitaram a aquisição de imagens de conídios e apressórios sobre a superfície de folhas de limão 'Siciliano' em todas as combinações de temperatura e molhamento avaliadas. / Citrus black spot caused by Guignardia citricarpa Kiely [Phyllosticta citricarpa (McAlp.) van der Aa] presents two infection forms, conidia and ascospores. Information regarding the importance of the conidia in the epidemiology of the disease is scarce and controversial. Seeking a better understanding on the pathosystem citrus-G. citricarpa (P. citricarpa), the objectives of this dissertation were: elaborate and validate a diagrammatic scale for assessments of the citrus black spot; verify the effect of the temperature and of the wetness duration in the appressorium formation; observe through scanning electron microscopy the germination and formation of appressorium on outstanding lemon 'Siciliano' leaves submitted to different temperatures and wetness duration. The diagrammatic scale with severity levels of 1; 3; 6; 12; and 24% of diseased leaf area was validated by two groups of raters, with experience and without experience in the quantification of diseases. The scale provided better precision and accuracy for both experienced and inexperienced raters, considering the estimates average of them. In the majority of cases, the bias between estimated and actual disease severity were more evident for disease severity levels between 5 and 15%. The reproducibility of assessments resulted in R 2 with more uniforms values for the majority of the experienced raters, considerable differences of precision were observed among inexperienced raters. The effect of the temperature (10 o C - 40 o C) and of the wetness duration (4 - 48 h) in the germination of conidia and appressoria formation of G. citricarpa (P. citricarpa), was assessed "in vitro" and on the surface of lemon 'Siciliano' leaves. The appressoria formation occurred in all the temperatures starting from 12 hours of wetness. The extreme temperatures (10 o C and 40 o C) were less favorable to the apressorium formation. The minimum temperature for appressorium formation, estimated by generalized beta function was of 3 o C and the maximum of 48,4 o C, both for 48 hours of wetness. The appressorium formation was favored considerably by the wetness duration period, with the maximum of apressoria formed at 24 hours of wetness, for majority of the temperatures. The wetness duration period constituted of 48 hours was essential so that the spores submitted to temperatures of 10 o C and 40 o C, formed appressorium. The response surface obtained by the multiplication of the generalized beta and monomolecular functions provided a close fit to observed data in the estimate of the relative percentage of formed appressorium (R 2 =0,75). The samples observed in scanning electron microscopy made possible the acquisition of images of conidia and appressoria on the surface of lemon 'Siciliano' leaves in all the temperature combinations and wetness evaluated.

citrus black spot

conidia

conídio

efeito da temperatura

efeito do molhamento

effect of temperature

effect of wetness

fungo fitopatogênico

limão

lime

mancha-preta-dos-citros

microscopia eletrônica de varredura

plant pathogenic fungi

scanning electronic microscopy

Qualidade do mexilhão Perna perna submetido ao processo combinado de cocção, congelamento e armazenamento / The quality of the mussel (Perna perna) processing by cooking, freezing and storage

Cordeiro, Daniela

02 September 2005

Os mexilhões cultivados no litoral Norte de São Paulo, município de Ubatuba, são comercializados in natura, constituindo risco à população. Com o crescimento da atividade é possível sugerir a implantação de uma unidade de processamento de mexilhões que promova um aumento do tempo de armazenamento, facilitando a comercialização e permitindo a exportação, além de fornecer ao consumidor um produto de melhor qualidade. Os mexilhões foram submetidos ao processamento por cocção, congelamento e armazenamento, sendo então determinados o ponto de congelamento, a velocidade de congelamento a as curvas de congelamento do mexilhão semidesconchado. A qualidade microbiológica e físico-química do produto foi avaliada. O beneficiamento do mexilhão iniciou-se com a cocção por imersão em água à ebulição por 10 minutos. Após a retirada das conchas, os mexilhões foram congelados individualmente IQF (Individually Quick Frozen) a -20ºC e armazenados a -18ºC durante 90 dias. A curva de congelamento do mexilhão apresentou forma geral típica, com o ponto de congelamento situando-se na faixa de zero a -1,5ºC; a velocidade de congelamento variou de 2 cm/h a 3,3 cm/h, conforme a disposição dentro da câmara de congelamento. Os resultados físico-químicos mostraram que não houve diferença significativa no valor nutricional dos mexilhões in natura, processados e armazenados, apresentando os teores médios de 7,4mg/100g de proteínas, 5,8 mg/100g de carboidratos e 1,4 mg/100g de lipídeos. Os valores encontrados para BNVT, TMA e pH no mexilhão in natura foram, 4,3 mg/100g; 2,0 mg/100g e 6,2, respectivamente, estando dentro dos limites estipulados pela legislação de 30mg/100g para BNVT e 4 mg/100g de TMA. Após o processo de cocção e congelamento houve um aumento no valor do pH para 6,9, enquanto o BNVT manteve-se na média. Todas as amostras de mexilhão in natura atenderam aos padrões microbiológicos estabelecidos pela legislação (RDC, nº12 de 02 de janeiro de 2001). Salmonella sp e Vibrio parahaemolyticus não foram isoladas em nenhuma das amostras de mexilhões in natura, cozidos, congelados e armazenados. O tratamento térmico foi efetivo no controle dos coliformes fecais, redução de coliformes totais, Staphylococcus coagulase+ e psicrotróficos. O processo de congelamento reduziu a contagem de coliformes totais e Staphyloocccus coagulase+, mantendo-se inalterados durante o armazenamento a -18ºC por 90 dias. Concluiu-se que o beneficiamento do mexilhão pelo processo combinado de cocção, congelamento e armazenamento assegura a qualidade físico-química e microbiológica do produto, podendo ser adotado como padrão para industrialização. / The mussels cultivated in the coast North of São Paulo, city of Ubatuba, are commercialized in natura, constituting risk to the population. With the growth of the activity it is possible to suggest the implantation of a unit of mussel processing that promotes an increase of the storage time, facilitating the commercialization and allowing the exportation, besides supplying to the consumer a product of better quality. The mussels had been submitted to the processing for cooking, freezing and storage, being then determined the freezing point, the speed of freezing to the curves of freezing of the semidesconchado mussel. The microbiological quality and physicochemical of the product were evaluated. The processing of the mussel was started with the immersion in boiling water per 10 minutes. After the withdrawal of the shells, the mussels had been frozen individually IQF (Individually Quick Frozen) at -20ºC and stored at -18ºC during 90 days. The curve of freezing of the mussel presented typical general form, with the freezing point placing from zero to -1,5ºC; the freezing speed varied from 2 cm.h-1 to 3,3 cm.h-1, as the disposal

análise de alimento

bactéria patogênica

conservação de alimento

cooking

cozimento

food analysis

food conservation

food microbiology

food quality

mexilhão

microbiologia de alimento

mussel

pathogenic bacteria

qualidade do alimento

Staphylococcus

Staphylococcus

thermical treatment

tratamento térmico

Reação de acessos de Capsicum spp. a Colletotrichum sp., agente causal da antracnose das Solanáceas. / Reaction of accesses of Capsicum spp. to Colletotrichum sp., causal agent of anthracnose.

Pereira, Mônica Juliani Zavaglia

04 March 2005

A importância do cultivo de espécies do gênero Capsicum vem crescendo nos últimos anos no Brasil, e consequentemente, a ocorrência de doenças torna-se um problema relevante. A antracnose é a mais comum e destrutiva doença de Capsicum no Brasil e em vários países, podendo ocasionar perdas de até 100%. Seu controle usando resistência genética seria altamente desejável. O objetivo deste trabalho foi (i) caracterizar a reação à antracnose de 90 acessos de Capsicum annuum, 30 de C. baccatum, 16 de C. chinense e um de C. frutescens; (ii) estabelecer a correlação da reação à antracnose entre plântulas e frutos de Capsicum e; (iii) avaliar a reação à antracnose das progênies F3RC1 (C.annuum x C. chinense - resistente) x C. annuum e F2RC2 [(C. annuum x C. chinense) x C. annuum] x C. annuum. Para as inoculações, foram utilizados quatro isolados do fungo Colletotrichum sp. provenientes de pimentão e um isolado de pimenta, obtidos de folhas e frutos doentes. As suspensões de inóculo foram preparadas na concentração de 1 x 106 conídios/ml, separadamente para cada isolado. Após ajustada a concentração das suspensões, estas foram misturadas, a fim de reduzir efeitos de possível variabilidade patogênica dos isolados. O delineamento utilizado foi inteiramente casualizado com 20 repetições para plântulas e 15 repetições para frutos verdes destacados. Os ensaios foram conduzidos duas vezes. Nas inoculações das plântulas, foi adicionado 5% de caldo de cana à suspensão, como fonte exógena de energia ao patógeno. A inoculação nas plântulas foi realizada no estádio de primeira folha verdadeira completamente expandida, pela aspersão da suspensão de esporos até o ponto de escorrimento. As plântulas foram mantidas em câmara úmida por 24 horas antes e 72 horas após a inoculação. O ensaio foi instalado em sala climatizada com temperatura de 26 +/- 2°C e fotoperíodo de 12 horas. Foi avaliada a severidade de doença, usando uma escala de notas e também a incidência da doença, com base na percentagem de plântulas doentes. A inoculação nos frutos foi realizada pela deposição de uma gota de 20 µl da suspensão de esporos na parte mediana dos frutos. Posteriormente, com o auxílio de uma agulha entomológica, foi realizado um ferimento abaixo da gota. Os frutos inoculados foram mantidos em câmara úmida durante o período de avaliação. As avaliações foram realizadas pela mensuração do diâmetro médio das lesões, período latente, velocidade de crescimento da lesão e incidência. Baseando-se na avaliação dos frutos para classificação da reação, identificou-se apenas um acesso de C. annuum como resistente (n°233 - Jalapeno), um de C. baccatum (n°222 - BGH 4176) e dois de C. chinense (n°105 - Bode e n°141 - Pimenta n°2). Os demais acessos foram suscetíveis. Não houve correlação entre a reação de plântulas e frutos. As plântulas apresentaram menor quantidade de doença, em relação aos frutos. As progênies F3RC1 (3G, 4A, 4B, 4F, 4H, 5H, 6B, 6F, 8B, 8E, 8F, 9B, 9D, 9E, 9J, 10A, 13D, 13F, 14A, 14C, 16D, 16I, 17B, 19B) e as progênies F2RC2 (33F e 40G) não apresentaram lesões no estádio de frutos. Avançou-se geração nas progênies com reação de resistência em frutos, e suas populações F4RC1 e F3RC2 foram avaliadas no estádio de plântulas. Constatou-se variabilidade para a reação de antracnose nestas populações, com expressão de menor severidade e possibilidade de obter cultivares de pimentas e pimentões resistentes à antracnose. / Capsicum cultivation is an increasing activity in Brasil, and, in conseqüence, disease occurence is becoming more frequent. Anthracnose is the most common and desctructive disease of Capsicum in Brasil and other countries. Losses of 100% due to the disease are very frequent. Control of anthracnose using genetic resistance can be very suitable. The aim of this work was (i) to describe the reaction of 90 accesses of Capsicum annuum, 30 of C. baccatum, 16 of C. chinense and one of C. frutescens to anthracnose (ii) to establish the correlation of the reaction to anthracnose between seedlings and fruits of Capsicum and (iii) to evaluate the reaction to anthracnose of the progenies F3RC1 (C.annuum x C. chinense - resistant) x C. annuum and F2RC2 [(C. annuum x C. chinense - resistant) x C. annuum] x C. annuum. Four isolates of Colletotrichum sp. from pepper and one isolate from hot pepper were used for the inoculations, at a concentration of 1 x 106 spores/ml. After adjustment of the concentration of each suspension, they were mixed, in order to reduce possible effects of pathogenic variability among the isolates. The experimental design used was of completely randomized blocks with 20 and 15 replications for seedlings and green-ripe fruits inoculations, respectively. For the inoculation in seedlings, sugarcane juice at 5% was added to the spore suspensions, which were sprayed on the leaves of the seedlings at one-leaf stage. The seedlings were kept in a moist chamber for 24 hours before and 72 hours after the inoculation, at 26 +/-2°C and 12 hours photoperiod, inside a growth chamber. To evaluate anthracnose on the inoculated plants, disease incidence and disease severity were considered. The last variable was rated based on a 1 to 5 scale, according to the amount of disease on the seedlings. The fruits were inoculated with a 20 µl droplet of the spore suspensions. After depositing the inoculum, the fruits were wounded with a needle at the inoculation point and kept at 24 +/- 2°C, inside covered plastic containers. The evaluation was done based on lesions diameter, latent period, growth rate of lesions and incidence. The fruits evaluations were used for classifying the accesses reactions. Only one access of C. annuum (n°233 - Jalapeno), one of C. baccatum (n°222 - BGH 4176) and two of C. chinense (n°105 - Bode and n°141 - Pimenta n°2) were considered resistant. The remaining accesses varied in degrees of susceptibility. Positive correlation between levels of disease in seedlings and fruits were not significant. The seedlings showed less amount of disease in relation to fruits. The progenies 3G, 4A, 4B, 4F, 4H, 5H, 6B, 6F, 8B, 8E, 8F, 9B, 9D, 9E, 9J, 10A, 13D, 13F, 14A, 14C, 16D, 16I, 17B, 19B (population F3RC1) and 33F and 40G (F2RC2) did not show lesions at the fruit stage. Generations were advanced in this population and populations F4RC2 and F3RC2 were evaluated at seedling stage. These seedlings showed variability for reaction to anthracnose, with lower severity, suggesting possibility of selection for resistance in Capsicum varieties.

anthracnose

antracnose

cruzamento vegetal

fungo fitopatogênico

genótipo

genotype

hot pepper

linhagem vegetal

pathogenic fungus

pepper

pimenta

pimentão

resistência genética vetegal

solanaceae

solanaceae

vegetal crossing

vegetal genetic resistance

vegetal line

Xylella fastidiosa adesão e colonização em vasos do xilema de laranjeira doce, cafeeiro, ameixeira, fumo e espécies de cigarrinhas vetoras e formação de biofilme sobre película de poliestireno. / Xylella fastidiosa - adhesion and colonization in xylem vessels of sweet orange, coffee, plum and tabacco, and insect vectors and formation of biofilme on polystyrene surface.

Alves, Eduardo

06 March 2003

X. fastidiosa é uma bactéria fitopatogênica limitada ao xilema, que tem afetado um grande número de plantas no Brasil e no mundo. Muitos trabalhos já foram realizados sobre esta bactéria, mas pouco se conhece a respeito da adesão, colonização e expressão dos sintomas. Os objetivos deste trabalho foram: a) através do uso da microscopia eletrônica e de luz, determinar e relacionar o número de vasos colonizados de citros, cafeeiro e ameixeira com a sintomatologia em folhas; b) estudar a adesão, migração radial e colonização dos vasos do xilema do pecíolo de folhas de citros pela bactéria; c) estudar algumas variáveis experimentais que afetam a expressão dos sintomas em fumo; d) verificar os sítios de ligação da bactéria em cigarrinhas vetores; e) estudar a adesão e a formação do biofilme por X. fastidiosa em superfície de poliestireno, como uma nova metodologia. Os resultados mostraram em ameixeira e cafeeiro uma relação entre o número de vasos colonizados e a expressão de sintomas necróticos, relação esta que não pode ser observada para citros, o qual apresentava um número de vasos colonizados do pecíolo bem menor que o das outras duas espécies. No estudo da bactéria nos vaso do xilema de citros foi possível verificar as diversas fases do processo de colonização do xilema, bem como a capacidade da bactéria em degradar a parede celular primária da pontuação e migrar para os vasos adjacentes. Neste estudo foi também possível verificar respostas da planta à bactérias caracterizadas pela produção de cristais no lúmen dos vasos do xilema e o acúmulo de goma e hiperplasia de células nas folhas. No estudo com variedades de fumo verificou-se que a cultivar Havana apresentou expressão de sintomas mais intensa que as variedades TNN e RP1 e que o aparecimento dos mesmos não foi influenciado pelo volume de inóculo e pelo local de inoculação, mas sim pela adubação com sulfato de amônio, a qual retardou o aparecimento dos sintomas e reverteu os sintomas inicias em folhas após a aplicação. Em cigarrinhas, células bacterianas com morfologia similar as de X. fastidiosa, foram visualizadas aderidas pela parte lateral na câmara do cibário (sulco longitudinal, parede lateral e membrana do diafragma) de Acrogonia citrina, e Oncometopia facialis, no canal do apodeme de Dilobopterus costalimai e pela parte polar no precibário de O. facialis. Finalmente, no estudo da adesão de X. fastidiosa a película de poliestireno, os resultados revelaram as várias fases da formação do biofilme, aspectos da sua arquitetura, e indicaram que a técnica é uma ferramenta adequada para o estudo da formação do biofilme e também da morfologia das bactérias. Os resultados são discutidos em termos de modelos de adesão e colonização, da bactéria e importância para o conhecimento dos mecanismos de patogenicidade da bactéria em plantas e transmissão pelos vetores. / X. fastidiosa is a xylem-limited bacterium that has been affecting a high number of plants in Brazil and in the world. A lot of researches were already accomplished on this bacterium, but little is known regarding the adhesion, colonization and expression of the symptoms in plants. The objectives of this work were: a) through the use of electron microscopy and of light microscopy determine and to correlate the number of xylem colonized vessels of petiole of sweet orange, coffee and plum with chlorosis and leaf scorching in leaves; b) study the adhesion, radial migration and colonization of the vessels of the petiole xylem of sweet orange by the bacterium; c) study some experimental variables that affect the expression of symptoms in tobacco; d) verify the retention sites of the bacterium in sharpshooters; d) study the adhesion and biofilm formation by X. fastidiosa on polystyrene surface. The results showed a relationship between the number of colonized vessels in plum and coffee and the expression of necrotic symptoms. However, that relationship was not observed for sweet orange, which presented a number of colonized vessels smaller than the other two species. In the study of the bacterium in the xylem vessels of sweet orange it was possible to verify the several phases of the colonization process of the xylem as well as the ability of the bacterium to degrade the primary cell wall of the pit and migrate to adjacent vessels. It was also possible to verify responses of the plant to the bacterium characterized by the production of crystals in the lumen of the xylem vessels and gum accumulation and hyperplasia in the leaf cells. Regarding the tobacco varieties it was verified that the expression of symptoms is more intense in the cultivar Havana than in the cultivars TNN and RP1. It was also seen that symptoms expression was not influenced by the inoculum volume or the inoculation place, but it was altered by fertilization with ammonium sulfate, which delayed the beginning of the symptoms and reverted the symptoms in leaves after the application. In sharpshooters, bacterial cells exhibiting morphology similar to X. fastidiosa were visualized attached to the lateral side in the cibarium camera (longitudinal, lateral wall and membrane of the diaphragm) of Acrogonia citrina, and Oncometopia facialis, in the apodemal channel of Dilobopterus costalimai, and in the polar part in the pre-cibarium of O. facialis. Finally, in the study of the adhesion of X. fastidiosa on polystyrene surface, the results revealed the several phases of biofilm formation; aspects of its architecture, and it also indicated that the technique is an appropriate tool to study of the formation of biofilms and also of the bacterial morphology. The results are discussed regarding adhesion models, colonization, and distribution of the bacterium in the plant and the importance of knowing the pathogenicity mechanisms of X. fastidiosa and its transmission by the insect vectors.

bactérias fitopatogênicas

cigarrinhas

citrus variegated chlorosis

clorose-variegada-dos-citros

light microscopy

microscopia

microscopia eletrônica de transmissão

microscopia eletrônica de varredura

plant pathogenic bactéria

scanning electron microscopy

sharpshooters

transmission electron microscopy

xilema

xylella

Avaliação da cinética populacional de Leifsonia xyli subsp. xyli em resposta a fatores do hospedeiro e do ambiente / The analysis of population kinetics of leifsonia xyli subsp. xyli in response to factors of host and environment

Ramos, Adalgisa Thayne Munhoz

29 January 2013

O raquitismo das soqueiras (RSD), causado pela bactéria Leifsonia xyli subsp. xyli (Lxx) é uma das principais doenças na cana-de-açúcar, contudo, as informações sobre a biologia do patógeno, bem como sobre sua interação com cana são limitadas. Desta forma, três estudos foram conduzidos com o objetivo de verificar a interferência de fatores do hospedeiro e do ambiente na cinética populacional da Leifsonia xyli subsp. xyli (Lxx) in planta e in vitro. Num primeiro, foi quantificada, através de PCR em tempo real (qPCR), a colonização da bactéria de plantas de duas variedades submetidas a estresse por restrição hídrica e por injúria mecânica infligida através de corte da planta. Num segundo, o desenvolvimento in vitro da bactéria foi avaliado, por 10 dias, em resposta à adição ao meio de cultivo de fluido vascular de plantas de cana. Já o terceiro estudo avaliou o efeito do hormônio ácido abscísico (ABA) na cinética populacional de Lxx em cana. No primeiro estudo, os resultados apontaram efeito positivo tanto do estresse hídrico como da injúria no título bacteriano em plantas da variedade CB 49-260. Já na variedade RB83 5486, não houve efeito significativo destes agentes de estresse no título bacteriano. No segundo estudo, o maior desenvolvimento da população de Lxx ocorreu em meio de cultivo sem adição de fluido vascular, ao passo que o desenvolvimento da população em presença de fluido da variedade resistente não inoculada com Lxx foi maior, quando em presença de fluido de plantas da mesma variedade inoculadas com a bactéria. A adição de fluido vascular da variedade suscetível, por outro lado, inibiu substancialmente o desenvolvimento das culturas bacterianas. A análise cromatográfica do fluido vascular indicou diferenças na concentração de compostos do fluido das duas variedades, bem como entre plantas da mesma variedade inoculadas ou não com a bactéria. No terceiro estudo, apesar das variações nos títulos da Lxx detectados ao longo do tempo, tanto nas plantas testemunhas como nas plantas tratadas com ABA, não houve diferenças significativas (p>0,05) entre os tratamentos dentro de um período de avaliação de 4 meses. Em seu conjunto, os resultados, além de fornecerem informações inéditas sobre a interação entre Lxx e cana, ainda permitiram direcionar futuros estudos a fim de aprimorar o conhecimento sobre os mecanismos de colonização do hospedeiro desta bactéria. / Ratoon Stunting Disease (RSD) caused by the bacterium Leifsonia xyli subsp. xyli (Lxx) is a major disease in sugarcane; however, information on the biology of this pathogen and on its interaction with sugarcane is limited. Three studies were conducted to analyze effects of the host and environment on the population kinetics of Leifsonia xyli subsp. xyli (Lxx) in plant and in vitro. In the first treatment, we used real time PCR (qPCR) to quantify bacterial colonization in two sugarcane varieties subjected to water stress and mechanical injury. In the second treatment, we evaluated the in vitro growth of the bacteria for 10 days after the addition of 15% of sugarcane vascular fluid to the culture medium. The third treatment evaluated the effect of the application of abscisic acid (ABA) on Lxx colonization in sugarcane. In the first treatment, the results showed an increase in Lxx colonization in the variety CB 49-260 exposed to water stress and mechanical injury. For the variety RB83 5486, there was no significant effect of these stresses on the bacterial colonization. In the second treatment, the greatest development of Lxx population occurred in the culture medium without the addition of vascular fluid (control), while bacterial population in the presence of fluid from resistant variety non-inoculated with Lxx was greater, compared to the growth in the presence of plant fluids of the same variety inoculated with the bacteria. The addition of vascular fluid of the susceptible variety, on the other hand, significantly inhibited bacterial growth. The chromatographic analysis of the vascular fluid indicated differences in the compounds concentration in the fluid of the two varieties, as well as in plants of the same variety inoculated or not with the bacteria. In the third study, despite variations in Lxx colonization detected over time, the control plants and plants treated with ABA showed no significant differences (p> 0.05) among treatments during the trial period of four months. The results, in addition to providing new information about the interaction between Lxx and sugarcane, allowed to direct further studies on mechanisms of host colonization of this bacterium.

Bactérias fitopatogênicas

Cana-de-açúcar

Cinética de populações

Danos mecânicos

Estresse hídrico

Fluido vascular

mechanical injury

Plant pathogenic bacteria

polymerase chain reaction

population kinetics

Raquitismo das soqueiras

ratoon stunting disease

Reação em Cadeia por Polimerase

sugarcane

vascular fluid

water stress

Illumination of the Golgi apparatus of Pathogenic and Nonpathogenic Naegleria species

Poe, Tyler M, Marciano-Cabral, Francine

01 January 2019

In this study, Naegleria fowleri, a pathogenic amoeba and the causative agent of Primary Amebic Meningoencephalitis (PAM), was utilized to determine the presence or absence of classically conserved Golgi molecules featured in the expression of a Golgi apparatus. Previous studies concluded no Golgi expression via light microscopy and transmission electron microscopy, but a recent report on Naegleria gruberi indicated the presence of dispersed Golgi tubules. Non-pathogenic species of the Naegleria genus such as Naegleria gruberi 30540 and Naegleria lovaniensis 30569 were utilized in Western immunoblot analysis compared to reduced whole-cell lysate proteins of two strains of N. fowleri and Vero CCL-81, Chlorocebus sp. kidney epithelial cells, which were utilized as a positive control for Golgi expression. N. fowleri and N. lovaniensis whole-cell lysates had indications of a 110 kDa reduced protein, associated with the predicted molecular weights of the beta-COPI subunit of the COPI cis-Golgi vesicular transport complex with further Western immunoblot indication of a weak band around 25 kDa corresponding to rabbit polyclonal antibodies specific for ARF1. Serial Dilutions of Wheat Germ Agglutinin Alexa Fluor 488TM were performed on Vero cells, Naegleria fowleri 30894, and N. gruberi 30540 with 1:100 dilution of recommended stock dilution of WGA 488 determined for utilization in sequential immunofluorescence. Sequential immunofluorescence with Wheat Germ Agglutinin Alexa Fluor 488TM and then blocked with 3% BSA:PBS [wt/vol] dilution with subsequent incubation in rabbit anti-beta-COPI primary 1:250, and 1:1000 of Alexa Fluor 594 goat anti-rabbit secondary antibody exposure showed strong indications of organized cis- and trans-punctate Golgi body markers in close association in individual and dividing cells of Naegleria fowleri and conserved Golgi expression in the positive control Vero cells, but further experiments are necessary to verify this finding with N. fowleri.

Naegleria fowleri

immunofluorescence

wheat germ agglutinin

golgi apparatus

Vero cells

Western immunoblots

Animals

Cell Biology

Cells

Diagnosis

Investigative Techniques

Microbial Physiology

Organismal Biological Physiology

Other Microbiology

Other Neuroscience and Neurobiology

Pathogenic Microbiology

Public Health Education and Promotion

Preconditioning of the tumor microenvironment by means of low dose chemotherapies for an effective immunotherapy of breast cancer

AQBI, HUSSEIN F

01 January 2019

Breast cancer mortality is mainly due to distant recurrence of the disease arising from dormant tumor cells established by cancer therapies. Patients who initially respond to cancer therapies often succumb to distant recurrence of the disease. It is not clear why people with the same type of breast cancer respond to treatments differently; some escape from dormancy and relapse earlier than others. In addition, some tumor clones respond to immunotherapy while others do not. We investigated how autophagy plays a role in accelerating or delaying recurrence of neu overexpressing mouse mammary carcinoma (MMC) following adriamycin (ADR) treatment, and in affecting response to immunotherapy. We explored two strategies: 1) transient blockade of autophagy with chloroquine (CQ), which blocks fusion of autophagosomes and lysosomes during ADR treatment, and 2) permanent inhibition of autophagy by a stable knockdown of ATG5 (ATG5KD), which inhibits the formation of autophagosomes in MMC during and after ADR treatment. We found that while CQ prolonged tumor dormancy, but that stable knockdown of autophagy resulted in early escape from dormancy and recurrence. Interestingly, ATG5KD MMC contained an increased frequency of ADR-induced polyploid-like cells and rendered MMC resistant to immunotherapy. On the other hand, a transient blockade of autophagy did not affect the sensitivity of MMC to immunotherapy. Our observations suggest that while chemotherapy-induced autophagy may facilitate tumor relapse, cell-intrinsic autophagy delays tumor relapse, in part, by inhibiting the formation of polyploid-like tumor dormancy. Although immunotherapy of breast cancer by means of anti-HER2 antibodies prolongs survival of breast cancer patients, disease recurrence remains a major challenge. On the other hand administration of human vaccines against infectious disease in a preventive setting or during latency/dormancy has been successful in offering a cure. Here, we sought to use adoptive immunotherapy (AIT) at the time of tumor dormancy in order to prevent progression of breast cancer. We used a low dose immunogenic chemotherapy by means of 5-FU, Adriamycin, and Cyclophosphamide (FAC) in order to stabilize tumor progression prior to AIT using autologous tumor-reactive lymphocytes. Low dose FAC established local tumor dormancy, inhibited distant tumor dormancy occurring long before distant metastasis, and induced predominate a Ki67- quiescent type of tumor dormancy, which is less susceptible to tumor immunoediting. Dormant tumor cells expressed the cell survival pathways, including the endothelin receptor/ligand (ETRA, ETRB and ET-1) and PD-L1, thereby protecting them from elimination by AIT. In addition, tumor-reactive CD8+ T cells also produced ET-1 as a survival ligand for ETRA positive tumor cells. A combination of AIT with the blockade of tumor cell survival pathways resulted in a significant improvement of AIT against tumor dormancy. We also showed that the inhibition Bcl-xL downstream of the tumor cell survival pathways is specifically effective against dormant tumor cells, suggesting a combination of AIT with small molecules inhibitors of Bcl-xL. Altogether, we showed that distant tumor dormancy is established long before distant recurrence of breast cancer, and that the expression of several tumor cell survival pathways in dormant cells protects them from immunotherapy. Our results suggest that immunotherapeutic targeting of tumor dormancy combined with the blockade of a common downstream cell survival pathway could prevent tumor progression and recurrence of the disease.

Tumor dormancy

Breast cancer

AIT

Tumor relapse

Alternative and Complementary Medicine

Bacteriology

Biotechnology

Immunology and Infectious Disease

Integrative Biology

Life Sciences

Molecular Biology

Other Microbiology

Pathogenic Microbiology

Application des nouvelles approches de cristallisation et de cristallographie sérielle à l’étude structurale de complexes enzymes : ARNt / Application of new crystallization approaches and serial crystallography to the structural study of enzyme/tRNA complexes

De Wijn, Raphaël

14 December 2018

Cette thèse porte sur deux aspects complémentaires, le développement et l’implémentation de nouvelles approches de cristallisation et de cristallographie sérielle ainsi que leur mise en œuvre dans l’étude structurale de complexes enzymes : ARNt. La cristallographie est la méthode la plus employée en biologie structurale, mais elle présente encore des points délicats. Plusieurs méthodes avancées ont été déployées dans ce travail pour y pallier qui ont conduit à la résolution de la structure de l’ARNt nucléotidyltransférase du psychrophile Planococcus halocryophilus et à l’étude de son adaptation structurale au froid ; des puces microfluidiques de cristallisation qui ont servi à la résolution de plusieurs structures à température ambiante par cristallographie sérielle ; enfin le Xtal Controller utilisé pour l’étude d’évènements de nucléation et de croissance cristalline dans un but de préparation d’échantillons pour analyse sous rayonnement XFEL. Entre autres systèmes biologiques, cette thèse présente la caractérisation de deux familles d’inhibiteurs visant les aspartyl-ARNt synthétases, notamment du pathogène Pseudomonas aeruginosa. / This thesis focuses on two complementary aspects, the development and implementation of new approaches of crystallization and of serial crystallography as well as their use in the structural study of enzymes/tRNA complexes. Crystallography is the most used method in structural biology, but it presents delicate points. Different methods were implemented in this work to overcome these points, which led to the resolution of the structure of the CCA-adding enzyme of the psychrophilic organism Planococcus halocryophilus and to the study of its structural adaptation to the cold; novel microfluidic crystallization chips that have been used for the resolution of several structures by serial crystallography at room-temperature; finally the Xtal Controller used for the study of nucleation and crystal growth events with the purpose of preparing samples for analysis under XFEL radiation. Among other biological systems, this thesis presents the study and characterization of two families of inhibitors targeting aspartyl-tRNA synthetases, including the one of the pathogenic organism Pseudomonas aeruginosa.

Biologie structurale

Cristallographie sérielle

Cristallogénèse

Puces microfluidiques

Xtal Controller

Organisme psychrophile

Organisme pathogène

Structural biology

Serial crystallography

Crystallogenesis

Microfluidic chips

Xtal Controller

Psychrophilic organism

Pathogenic organism

571.4

572.5

548

Delineation Of Signal Transduction Events During The Induction Of SOCS3 By Mycobacterium Bovis BCG : Possible Implications For Immune Subversion Mechanisms

Yeddula, Narayana

07 1900

Pathogenic Mycobacteria are among the most unrelenting pathogens known to mankind as one-third of the world population is latently infected with Mycobacterium tuberculosis, the causative agent of pulmonary tuberculosis. Despite many species of mycobacteria elicits robust host T cell responses as well as production of cytokines like interferon-γ (IFN- γ) that are essential for the control of infection, the mounted immune response contain, but does not eliminate the infection. One potential mechanism by which mycobacteria may achieve a state of long-term persistence amid a robust host immune response is by modulating the signaling cascades leading to macrophage activation. Activation of proinflammatory responses by the host macrophages upon infection with mycobacteria requires the involvement of a variety of signaling events. Studies have indicated that macrophages infected with pathogenic mycobacteria produce significantly less tumor necrosis factor (TNF)-α and other proinflammatory molecules compared with infection with nonpathogenic mycobacteria, which likely play a role in enhancing mycobacterial survival in vivo. Furthermore, macrophages infected with mycobacteria become refractory to many cytokines including IFN-γ and modulation of host cell signaling responses is critical for the suppression of a generalized inflammatory response which might influence the persistence of mycobacteria within the host. In this context, Suppressor of cytokine signaling (SOCS) 3, a member of SOCS family function as negative regulators of multiple cytokine and toll like receptor induced signaling. The SOCS3 has been shown to specifically inhibit signaling by IFN-γ, IL-6 family of cytokines and can act as a negative regulator of inflammatory responses. In this regard, many species of mycobacteria including M. bovis BCG triggers the inducible expression of SOCS3. Further, it has been suggested that M. bovis BCG triggered SOCS3 and SOCS1 proteins leads to the inhibition of IFN- γ stimulated JAK/STAT signaling in macrophages. Albeit JAK/STAT signaling pathway is generally believed to be involved, STAT-independent signals are suggested to take part in the induction of SOCS proteins in many systems signifying the involvement of multiple signal pathways in regulation of SOCS expression. Further little is known about the early, receptor proximal signaling mechanisms underlying mycobacteria-mediated induction of SOCS3. Albeit mycobacteria reside within phagolysosomes of the infected macrophages, many cell wall antigens like LAM, PIM, TDM, PE family antigens etc are released and traffic out of the mycobacterial phagosome into endocytic compartments as well as can gain access to the extra cellular environment in the form of exocytosed vesicles. In this context, PIM represent a variety of phosphatidyl-myo-inositol mannosides (PIM) 1-6 containing molecules and are integral component of the mycobacterial envelope. PIM are suggested to be the common anchor of LM and LAM as PIM, LM, and LAM originate from identical biosynthetic pathway. PIM are present in virulent M. tuberculosis H37Rv as well as in M. bovis BCG and a number of biological functions have been recently credited to PIM2. PIM2 is suggested to trigger the activation of cells via Toll like receptor (TLR)-2 and stimulation resulted in activation of NF-κB, AP-1, and mitogen-activated protein (MAP) kinases. PIM2 induces proinflammatory stimuli such as TNF-α and IL-12 in murine and human macrophages in a TLR2 dependent manner. PIM exhibited pulmonary granuloma-forming activities as well as was shown to be responsible for the recruitment of NKT cells to granulomas. Accordingly, mycobacterial envelope antigen PIM2 could initiate or affect the inflammatory responses similar to mycobacteria bacilli. In this perspective, we explored whether M. bovis BCG or novel cell surface antigens like PIM2 or Rv0978c, a PE-PGRS protein with unknown function can contribute to M. bovis BCG triggered molecular signaling events leading to SOCS3 expression in macrophages. Our studies clearly demonstrated that M. bovis BCG can trigger SOCS3 expression in macrophages. The inception of signaling by M. bovis BCG is TLR2-MyD88 dependent, but not TLR4 dependent. The perturbation of TLR2 signaling and the downregulation of MyD88 resulted in significant decrease in SOCS3 expression implicating the role of TLR2-MyD88 axis in M. bovis BCG triggered signaling. Experiments with cycloheximide and neutralizing antibodies to IL-10 evinced that M. bovis BCG triggered SOCS3 expression is a primary response and requires direct activation of signaling cascades. In the current study, we show for the first time that infection of macrophages with M. bovis BCG activates NOTCH1 signaling events, which leads to expression of SOCS3. The perturbation of NOTCH signaling in infected macrophages either by siRNA mediated down regulation of NOTCH1 or RBP-Jk or by inhibition with pharmacological inhibitor gamma secretase-I, resulted in the marked reduction in the expression of SOCS3. Further, the enforced expression of the NOTCH1 intracellular domain (NICD) in RAW264.7 macrophages induces the expression of SOCS3, which can be further potentiated by M. bovis BCG. Furthermore, the inhibition of TLR2 signaling by a TLR2 dominant-negative construct resulted in inhibition of NOTCH1 activation. Additionally, our results demonstrates for the first time that physical association of TLR2 with both Phosphoinositide-3 Kinase (PI3K) and NOTCH1, which suggest the significant role of TLR2 triggering by of M. bovis BCG in the activation of PI3K and NOTCH1. More importantly, signaling perturbations data suggest the involvement of cross-talk among the members of PI3K and MAPK cascades with NOTCH1 signaling in SOCS3 expression. In addition, SOCS3 expression requires the NOTCH1 mediated recruitment of CSL/RBP-Jk and Nuclear Factor-B (NF-B) to the SOCS3 promoter. A number of biological functions triggered by mycobacteria are often attributed to many of the cell wall antigens. As part of our current investigation, we explored whether two novel cell wall associated antigens namely PIM2 and a PE-PGRS antigen, Rv0978c could play as significant or crucial cell wall ingredients which imparts ability to M. bovis BCG to trigger activation of NOTCH signaling leading to SOCS3 expression. Akin to M. bovis BCG, PIM2 activates NOTCH1 signaling resulting NICD formation which leads to the expression of SOCS3 in a TLR2-MyD88 dependent manner. PIM2 mediated NOTCH1 activation, both directly influences the SOCS3 expression by serving as coactivator in RBP-Jk complex and indirectly triggers SOCS3 expression by activating PI3K-MAPK-NF-κB cascade. One important outcome of the genome sequencing project of M. tuberculosis was the discovery of two new multigene families designated PE and PPE, named for the Pro-Glu (PE) and Pro-Pro-Glu (PPE) motifs near the N-terminus of their gene products. Many PE and PPE proteins are composed only of PE or PPE homologous domains. However, in other proteins, the PE domain is often linked to a unique domain of various lengths that is rich in alanine and glycine amino acids, termed the PGRS domain (PE-PGRS subfamily). PE family genes were suggested to play roles in the virulence of the pathogen and many members of PE family proteins are reported be localized on the surface of M. tuberculosis bacilli. Some of the PE proteins may play a role in immune evasion and antigenic variation or may be linked to virulence. Additionally, it has been suggested that the PE-PGRS subfamily of PE genes is enriched in genes with a high probability of being essential for M. tuberculosis. The uniqueness of the PE genes is further illustrated by the fact that these genes are restricted to mycobacteria. However, despite their abundance in mycobacteria, very little is known regarding the expression or the functions of PE family genes. In this context, we have chosen to study Rv0978c as a typical member of PE-PGRS family based on the following observations. Rv0978c was upregulated in TB bacilli upon infection of macrophages. Rv0978c was demonstrated to be a member of a group of genes called in vivo-expressed genomic island, which were shown to be upregulated in M. tuberculosis bacilli during infection of mice. Rv0978c was also shown to be upregulated, at least eightfold, in human brain microvascular endothelial cell-associated M. tuberculosis infection, suggesting a role for endothelial cell invasion and intracellular survival. In the current investigation, we have demonstrated that Rv0978c is hypoxia responsive gene based on promoter analysis and upregulated in M. tuberculosis during the infection of macrophages. Further, Rv0978c is associated with cell wall and is exposed outside the surface of the bacterium suggesting the possible access to intracellular compartments of the infected macrophages. In this perspective, our results clearly demonstrate that Rv0978c triggers SOCS3 expression by activating PI3K-ERK1/2-NF-B cascade in mouse macrophages. Additionally, Rv0978c elicited humoral antibody reactivities in a panel of human sera or in cerebrospinal fluid samples obtained from different clinical categories of tuberculosis patients. DNA immunizations experiments in mice clearly suggested that Rv0978c is an immunodominant antigen demonstrating significant T cell and humoral reactivites. These observations clearly advocate that Rv0978c protein is expressed in vivo during active infection with M. tuberculosis and that the Rv0978c is immunogenic. These results clearly describe the cross-talk of NOTCH1 signaling with signaling pathways like PI3K and MAPK pathways during infection of macrophages with M. bovis BCG eventually resulting in regulation of specific gene expressions, such as SOCS3. These observations lead to a possibility of differential effects of NOTCH1 signaling activated upon infection by an intracellular bacillus, which could be involved in modulation of macrophage functions depending on a local immunological milieu. Taken together, our findings suggest that, induction of Suppressors of Cytokine Signaling 3 molecule by M. bovis BCG or by its cell wall antigens represents a crucial immune subversion mechanism in order to suppress or attenuate host responses to cytokines to generate the conditions that favor survival of the mycobacteria.

Signal Transduction

BCG

Macrophages

Mycobacterium Tuberculosis

Supressor Of Cytokine Signaling

Mycobacteria

Pathogenic Mycobacteria

Mycobacterium bovis BCG

SOCS3

PIM2

Rv0978c

Novel Cellwall Antigens

PE-PGRS Antigen

PE Antigens

M. tuberculosis

Bacteriology