Ecologie microbienne de produits végétaux : Adaptation de traitements assainissants pour la valorisation de ces produits / Microbial ecology of vegetable matter : Adaptation of cleaning treatments for the valuation of these products

Metivier, Romain

16 December 2015

L’utilisation de coproduits en tant que matière première provenant d’une autre voie industrielle, fait qu’il n’est plus considéré comme « déchet ». Leur valorisation est donc un axe de développement pour les entreprises agronomiques et agroalimentaires. Cependant, leur nouveau statut de « matière première » entraîne des contraintes pour les industriels.Celles-ci sont diverses selon les voies de destination : sanitaires, toxicologiques …Ce travail s’intéresse à deux coproduits issus de filières différentes de transformation végétale :(1) l’épiderme de pomme, comme source d’antioxydants. Leur valorisation passe par l’emploi de matières premières peu traitées d’un point de vue phytosanitaire qui pourront être a priori plus contaminées par des flores diverses.(2) Les broyats de végétaux issus de la culture céréalière comme matière première de produits biosourcés. Ils présentent naturellement de fortes contaminations en microorganismes sporulés.La valorisation de ces deux coproduits nécessite donc des traitements assainissants adaptés.Ainsi, il était indispensable de déterminer la nature, la variabilité et l’évolution des écologies microbiennes présentes sur ces coproduits par des techniques rapides de dénombrement ainsi que d’identification par biologie moléculaire. L’étude de différents procédés assainissants a également été réalisé pour combiner l’efficacité de désinfection à la préservation des qualités nutritionnelles (pomme) ou des propriétés physiques (broyats). / The use of byproduct as raw material from another industrial sector, facts that it is not considered any more as "waste". Their valuation is thus an axis of development for the agronomic and food-processing industry. However, their new consideration of "raw material" entails constraints for the industrialists. These constraints are diverse according to the destination ways of the byproduct: sanitary, toxicological… This work focus on two byproducts resulting from different vegetable process: (1) apple peels, as antioxidant source. Their valuation needs to use raw materials with low phytosanitary treatment, so these materials may be more contaminated by different floras. (2) Crushed vegetable matter stemming from cereal crop as raw material of biosourced products. They occur naturally a strong microbial spore contamination. The valuation of these two byproducts requires adapted cleaning treatments. So, it was the main thing to determine nature, variability and evolution of the present microbial ecologies of these byproducts by fast techniques of enumeration and identification by molecular biology. The study of different cleaning process was also realized to combine efficiency of disinfection with the preservation of nutritional qualities (apple) or physical properties (crushed vegetable matter).

Coproduits

Traitement vapeur

Ozone

Traitements assainissants

Tempo®

PCR-DGGE

PCRq

Écologie microbienne

Byproducts

Steam treatment

Ozone

Cleaning treatments

Tempo®

PCR-DGGE

QPCR

Microbial ecology

Expressão de genes homeobox em células de carcinoma epidermóide de boca estimuladas com EGF e TGF-beta / Expression of homeobox genes in oral squamous cell carcinoma cell lines, stimulated with EGF and TGF-beta

Marcia Sampaio Campos

21 January 2008

Genes homeobox, vitais para muitos aspectos relacionados com crescimento e diferenciação celular, têm sido descritos desregulados em alguns cânceres. Seu papel na carcinogênese, principalmente de carcinomas epidermóides de boca, permanence pouco claro e pobremente caracterizado. Desse modo, esse estudo objetivou avaliar, em cultura de células, o perfil de expressão de seis genes homeobox (ASH2L, HOXA7, HHEX, PKNOX1, PITX1, TGIF) selecionados dentre aqueles previamente identificados no Projeto Genoma Câncer de Cabeça e Pescoço (2001) sob estímulo de EGF e TGF-beta1. Para tal, linhagens celulares de carcinoma epidermóide de cabeça e pescoço primário (HN6) e metastático (HN31) e uma linhagem não-tumoral (HaCat) foram cultivadas sob condições-padrão. Após a confecção dos cDNAs de cada linhagem, por meio de RT-PCR, os transcritos foram amplificados e quantificados pela técnica de PCR em tempo real. Os dados foram normalizados com o gene HPRT e a quantificação relativa foi realizada seguindo o método do delta Ct. De acordo com os resultados foi possível verificar que o EGF produziu uma modulação variável da expressão dos genes avaliados em todas as linhagens celulares, enquanto que, em geral, o TGF-beta1 foi capaz de aumentar significantemente (ANOVA, p<0,05) a expressão dos transcritos de 5 genes homeobox (HOXA7, HHEX, PKNOX1, PITX1, TGIF). Particularmente transcritos dos genes PITX1 e TGIF foram signicantemente mais expressos nas linhagens tumorais (HN6 e HN31) frente à linhagem não-tumoral quando tratados com TGF-beta1. Desse modo, sugere-se que os genes homeobox estudados desempenhem diferentes funções na carcinoma epidermóide de boca, e que, especialmente PITX1 e TGIF atuem como oncogenes inibindo a resposta anti-proliferativa dependente de TGF-beta e levando a progressão tumoral. / Homeobox genes, vital to many aspects related with cellular growth and differentiation, had been described as deregulated in some cancers. Their role in carcinogenesis, mainly oral squamous cell carcinomas, remains unclear and poorly characterized. Thus, this study had the purpose to evaluate, in cell cultures, the expression profile of six homeobox genes (ASH2L, HOXA7, HHEX, PKNOX1, PITX1, TGIF) selected among genes previously identified in the Head and Neck Cancer Genoma Project (2001), under stimulation with EGF and TGF-beta1. Oral squamous cell carcinoma cell lines from primary tumour (HN6) and from methastasis (HN31), and a non-tumoral cell line (HaCat) were cultured under standard procedures. CDNAs were obtained by RT-PCR and the transcripts were amplified and quantified by real-time PCR. Data were normalized by HPRT gene and the relative quantification was made by the delta Ct method. According to the results, it was possible to observe that EGF produced a variable modulation of the analyzed genes, in all cell lines. Generally, TGF-beta1 was able to significantly increase (ANOVA, p<0,05) the expression of the transcripts of 5 homeobox genes (HOXA7, HHEX, PKNOX1, PITX1, TGIF). Transcripts of PITX1 and TGIF genes were particularly more expressed in the tumoral cell lines (HN6 e HN31), when compared to the non-tumoral cell line, when treated with TGF-beta1. It is suggested that the studied homeobox genes play different roles in oral squamous cell carcinoma and that, especially the PITX1 and TGIF act as oncogenes, inhibitting the TGF-dependent anti-proliferative response, leading to tumour progression.

Carcinoma epidermóide de boca

EGF

Genes Homeobox

Linhagens celulares

PCR quantitativo

TGF-beta

Cell lines

EGF

Homeobox genes

Oral squamous cell carcinoma

qPCR

TGF-beta

Biogeografia de comunidades fúngicas em áreas cultivadas com cana-de-açúcar / Biogeography of fungal communities in sugarcane fields

Thiago Gumiere

28 January 2013

A cana-de-açúcar é atualmente a cultura de maior importância agrícola do Estado de São Paulo, a partir da qual são gerados açúcar e etanol, além de vários outros subprodutos. No entanto, com a expansão das fronteiras agrícolas e alterações nas práticas de manejo, ocorre atualmente um momento de adequação de tal cultivo, que visa uma maior produtividade e sustentabilidade de produção. Para isto, dentre outros fatores, o papel da comunidade microbiana presente nos solos pode ter fundamental importância, auxiliando no melhor desenvolvimento da planta. No entanto, pouco se sabe sobre a comunidade microbiana existente nos solos cultivados com cana-de-açúcar. Dessa forma, este trabalho teve como objetivo avaliar a diversidade e a abundância de fungos em solos de cultivo de cana-deaçúcar no estado de São Paulo, em áreas sob diferentes atributos químicos, físicos e de manejo. Objetivou-se também, verificar a ocorrência de padrões biogeográficos na estruturação de tais comunidades. Para isso, foi realizada a análise da estrutura das comunidades fúngicas por polimorfismo de comprimento de fragmentos de restrição terminal (T-RFLP), juntamente com a quantificação destas comunidades por meio da PCR em tempo real (qPCR) em 476 amostras de solo, obtidas de 11 áreas de cultivo (usinas). Dentro deste conjunto de dados, temos que os atributos químicos, físicos e manejo explicam maiores valores de variância dentro de cada área amostra, mas pouco explicam da variância geral dos dados, sugerindo a ocorrência de padrões biogeográficos das comunidades de fungos neste ambiente. Tal ocorrência foi confirmada pela significância estatística da correlação entre distância e dissimilaridade das comunidades de fungos, dando suporte a geração dos primeiros mapas biogeográficos de fungos em tais solos. Adicionalmente, a abundância de fungos mostrou-se relacionada com a produtividade da cultura, indicando este ser um dos fatores que modulam a produtividade de cana-de-açúcar nas áreas avaliadas. / The sugarcane is nowadays, the most important crop in the State of São Paulo, serving as the raw material for the production of sugar and ethanol, besides many others by-products. Considering the expansion of agricultural barriers, and shifts in fields management, such cultivation is under a re-arrangement process, aiming to a higher productivity and sustainability. In order to achieve that, among other factors, the role of microbial communities present in soils can be essential to support plant development. However, a few is known about the microbial community under sugarcane crop production soils. Hence, this work intended to evaluate the fungi diversity and abundance in soils cultivated with sugarcane in the State of São Paulo, exploring areas under distinct chemical and physical attributes and also distinct management practices. It was also aimed to determine the occurrence of biogeographically patterns in the structure of such communities. Indeed, it was made the analysis of the fungal community structure by terminal restriction fragment length polymorphism (T-RFLP), together with the quantification of these communities by real time PCR (qPCR) in 476 soils samples, collected in 11 areas cultivated with sugarcane (mills). Within this dataset, it was found that chemical, physical and management attributes explain higher values of variance within each sampled area, but explain little about the total variance of data, suggesting the occurrence of biogeographically patterns in fungal communities in this environment. It was confirmed by the statistical significance of the correlation between distance and dissimilarity of fungal communities, supporting the generation of very first biogeographically maps in such soils. Additionally, the abundance of fungi revealed to be related with sugarcane productivity, indicating this issue as one of the factors modulating the sugarcane productivity in the evaluated areas.

Biogeografia

Cana-de-açúcar

Fungos

Interação planta-microrganismo

Microbiologia do solo

Polimorfismo

Reação em Cadeia por Polimerase

Fungal biogeography

qPCR

Soil microbiology

T-RFLP

Detec??o de Anaplasma platys em c?es e em carrapatos: padroniza??ode qPCR e an?lise epidemiol?gica no Estado do Rio de Janeiro, Brasil e na regi?o ocidental de Cuba / Detection of Anaplasma platys in dogs and ticks: standardization of qPCR and epidemiological analysis in the State of Rio de Janeiro, Brazil and in western Cuba

Silva, Claudia Bezerra da

11 March 2016

Submitted by Celso Magalhaes (celsomagalhaes@ufrrj.br) on 2017-10-19T13:49:16Z No. of bitstreams: 1 2016 - Claudia Bezerra da Silva.pdf: 8032175 bytes, checksum: ef71dd2a0e7801e9000e116c822a3a00 (MD5) / Made available in DSpace on 2017-10-19T13:49:16Z (GMT). No. of bitstreams: 1 2016 - Claudia Bezerra da Silva.pdf: 8032175 bytes, checksum: ef71dd2a0e7801e9000e116c822a3a00 (MD5) Previous issue date: 2016-03-11 / Coordena??o de Aperfei?oamento de Pessoal de N?vel Superior - CAPES / and investigate the circulation of this agent in dogs in the Itaguai microregion, Rio de Janeiro, Brazil, and dogs and ticks in two provinces of the island of Cuba, analyzing epidemiological aspects associated with infections caused by this bacterium in dogs. A new real-time polymerase chain reaction method (qPCR) was patterned to target the citrate synthase gene (gltA) for the identification of A. platys in naturally infected dogs. The primers and probe were designed to amplify a fragment of 84 base pairs based on gltA gene sequences of A. platys available in GenBank. 186 blood samples of dogs from Itaguai microregion, Rio de Janeiro, Brazil, were tested by qPCR. The same samples were tested by cytology and nested polymerase chain reaction (nPCR, 16S rDNA) to determine the performance of qPCR front of these techniques. 17.20% of the samples tested positive by qPCR were significantly more than that detected by nPCR (13.98%). The qPCR technique was more specific than cytology, due to false-positive results obtained by optical microscopy. The prevalence of A. platys in dogs from Itaguai microregion was 14.4%. Dogs less than six months, infested by ticks, that spend the most of the time restrict to domestic environment and without shelter are factors associated with infection by this hemoparasite in dogs in the study area. During research, A. platys held in Cuba, 100 blood samples were collected from residents dogs in four cities located in the provinces of Havana and Mayabeque. When inspecting the animals, found ticks were collected, identified and carefully grouped, forming a total of 49 pools. DNA extracted from blood samples from dogs and ticks were subjected nPCR (16S rDNA). Positive samples in nPCR were also subjected to conventional PCR (gltA gene), and the products were sequenced. Only the species Rhipicephalus sanguineus sensu lato was found in Cuban dogs and 10.2% (n=5/49) of these ticks added to 16.0% (n=16/100) dogs were considered positive for A. platys. All sequences analyzed of the gltA and 16S rDNA genes, respectively, showed a 99-100% identity with sequences from A. platys reported in other countries. Phylogenetic analysis showed two clusters defined for the 16S rDNA gene and three clusters defined for the gltA gene. Based on the gltA gene, the deduced amino acid sequence showed two points of non-synonymous mutations at positions 88 and 168 compared to the reference sequence DQ525687. A preliminary study on the epidemiological aspects associated with infection with A. platys showed no statistical association with the variables studied (p> 0.05). This study also to report the first evidence of A. platys in both dogs and ticks in Cuba also presents for the first time the development of a new qPCR method that contributes to the advancement of research involving A. platys. The epidemiological study in Brazil allowed us to identify significant factors in the occurrence of canine anaplasmosis, while in Cuba, it can be concluded that more research is needed to assess what the deciding factors in the transmission and spread of A. platys in that country. / platys, e investigar a circula??o deste agente em c?es na microrregi?o de Itagua?, Rio de Janeiro, Brasil, e c?es e carrapatos em duas prov?ncias da ilha de Cuba, analisando aspectos epidemiol?gicos associados ? infec??o causada por esta bact?ria em c?es. Um novo m?todo de rea??o em cadeia da polimerase em tempo real (qPCR) foi padronizado com alvo no gene citrato sintase (gltA) para a identifica??o de A. platys em c?es naturalmente infectados. Os oligoiniciadores e a sonda foram desenhados para amplificar um fragmento de 84 pares de base baseado em sequ?ncias do gene gltA de A. platys dispon?veis no GenBank. 186 amostras de sangue de c?es da microrregi?o de Itagua?, Rio de Janeiro, Brasil, foram testados pela qPCR. As mesmas amostras foram testadas pela citologia e rea??o em cadeia da polimerase nested (nPCR, 16S rDNA) para determinar o desempenho da qPCR frente ? essas t?cnicas. 17,20% das amostras testadas pela qPCR foram positivas, significativamente mais do que detectado pela nPCR (13,98%). A t?cnica de qPCR foi mais espec?fica que a citologia, em virtude dos resultados falsopositivos obtidos pela microscopia ?ptica. A preval?ncia de A. platys em c?es da microrregi?o de Itagua? foi de 14,4%. C?es com menos de seis meses, infestados por carrapatos, que possam maior tempo restrito ao ambiente dom?stico e sem abrigo s?o fatores associados a infec??o por este hemoparasito em c?es na regi?o do estudo. Durante investiga??o de A. platys realizada em Cuba, 100 amostras de sangue foram coletadas de c?es residentes em quatro cidades localizadas nas prov?ncias de Habana e Mayabeque. Ao inspecionar os animais, carrapatos encontrados foram coletados, identificados e criteriosamente agrupados, formando um total de 49 pools. Amostras de DNA extra?das do sangue dos c?es e de carrapatos foram submetidas a nPCR (16S rDNA). Amostras positivas na nPCR foram tamb?m submetidas a PCR convencional (gene gltA), e os produtos foram sequenciados. Somente a esp?cie Rhipicephalus sanguineus sensu lato foi encontrada em c?es cubanos, e 10,2% (n=5/49) desses carrapatos somado aos 16,0% (n=16/100) de c?es foram considerados positivos para A. platys. Todas as sequ?ncias analisadas dos genes gltA e 16S rDNA, respectivamente, mostraram uma identidade de 99-100% com sequ?ncias de A. platys reportadas em outros pa?ses. A an?lise filogen?tica mostrou dois clusters definidos para o gene 16S rDNA e tr?s clusters definidos para o gene gltA. Com base no gene gltA, a sequ?ncia de amino?cidos deduzidos demonstrou dois pontos de muta??es n?o-sin?nimas nas posi??es 88 e 168 comparados com sequ?ncia de refer?ncia DQ525687. Um estudo preliminar sobre os aspectos epidemiol?gicos associados com a infec??o por A. platys demonstrou nenhuma associa??o estat?stica com as vari?veis avaliadas (p > 0,05). O presente estudo al?m de relatar a primeira evid?ncia de A. platys em ambos c?es e carrapatos em Cuba, tamb?m apresenta pela primeira vez o desenvolvimento de um novo m?todo de qPCR que contribui para o avan?o da pesquisa envolvendo A. platys. O estudo epidemiol?gico realizado no Brasil permitiu identificar fatores importantes na ocorr?ncia da anaplasmose canina, enquanto em Cuba, pode-se concluir que mais investiga??es s?o necess?rias para avaliar quais os fatores decisivos na transmiss?o e dispers?o de A. platys nesse pa?s.

dogs

molecular diagnostic

phylogeny

Anaplasma platys

c?es

diagn?stico molecular

qPCR

nested PCR

filogenia

Rhipicephalus sanguineus sensu lato

Ci?ncias Biol?gicas

Biogeografia de comunidades fúngicas em áreas cultivadas com cana-de-açúcar / Biogeography of fungal communities in sugarcane fields

Gumiere, Thiago

28 January 2013

A cana-de-açúcar é atualmente a cultura de maior importância agrícola do Estado de São Paulo, a partir da qual são gerados açúcar e etanol, além de vários outros subprodutos. No entanto, com a expansão das fronteiras agrícolas e alterações nas práticas de manejo, ocorre atualmente um momento de adequação de tal cultivo, que visa uma maior produtividade e sustentabilidade de produção. Para isto, dentre outros fatores, o papel da comunidade microbiana presente nos solos pode ter fundamental importância, auxiliando no melhor desenvolvimento da planta. No entanto, pouco se sabe sobre a comunidade microbiana existente nos solos cultivados com cana-de-açúcar. Dessa forma, este trabalho teve como objetivo avaliar a diversidade e a abundância de fungos em solos de cultivo de cana-deaçúcar no estado de São Paulo, em áreas sob diferentes atributos químicos, físicos e de manejo. Objetivou-se também, verificar a ocorrência de padrões biogeográficos na estruturação de tais comunidades. Para isso, foi realizada a análise da estrutura das comunidades fúngicas por polimorfismo de comprimento de fragmentos de restrição terminal (T-RFLP), juntamente com a quantificação destas comunidades por meio da PCR em tempo real (qPCR) em 476 amostras de solo, obtidas de 11 áreas de cultivo (usinas). Dentro deste conjunto de dados, temos que os atributos químicos, físicos e manejo explicam maiores valores de variância dentro de cada área amostra, mas pouco explicam da variância geral dos dados, sugerindo a ocorrência de padrões biogeográficos das comunidades de fungos neste ambiente. Tal ocorrência foi confirmada pela significância estatística da correlação entre distância e dissimilaridade das comunidades de fungos, dando suporte a geração dos primeiros mapas biogeográficos de fungos em tais solos. Adicionalmente, a abundância de fungos mostrou-se relacionada com a produtividade da cultura, indicando este ser um dos fatores que modulam a produtividade de cana-de-açúcar nas áreas avaliadas. / The sugarcane is nowadays, the most important crop in the State of São Paulo, serving as the raw material for the production of sugar and ethanol, besides many others by-products. Considering the expansion of agricultural barriers, and shifts in fields management, such cultivation is under a re-arrangement process, aiming to a higher productivity and sustainability. In order to achieve that, among other factors, the role of microbial communities present in soils can be essential to support plant development. However, a few is known about the microbial community under sugarcane crop production soils. Hence, this work intended to evaluate the fungi diversity and abundance in soils cultivated with sugarcane in the State of São Paulo, exploring areas under distinct chemical and physical attributes and also distinct management practices. It was also aimed to determine the occurrence of biogeographically patterns in the structure of such communities. Indeed, it was made the analysis of the fungal community structure by terminal restriction fragment length polymorphism (T-RFLP), together with the quantification of these communities by real time PCR (qPCR) in 476 soils samples, collected in 11 areas cultivated with sugarcane (mills). Within this dataset, it was found that chemical, physical and management attributes explain higher values of variance within each sampled area, but explain little about the total variance of data, suggesting the occurrence of biogeographically patterns in fungal communities in this environment. It was confirmed by the statistical significance of the correlation between distance and dissimilarity of fungal communities, supporting the generation of very first biogeographically maps in such soils. Additionally, the abundance of fungi revealed to be related with sugarcane productivity, indicating this issue as one of the factors modulating the sugarcane productivity in the evaluated areas.

Biogeografia

Cana-de-açúcar

Fungal biogeography

Fungos

Interação planta-microrganismo

Microbiologia do solo

Polimorfismo

qPCR

Reação em Cadeia por Polimerase

Soil microbiology

T-RFLP

The Study of Tissue-Specific DNA Methylation as a Method for the Epigenetic Discrimination of Forensic Samples

Antunes, Joana AP

21 November 2017

In forensic sciences, the serological methods used to determine which body fluid was collected from the crime scene are merely presumptive or labor intensive since they rely on protein detection or on microscopic identification of cells. Given that certain forensic cases may need the precise identification of a body fluid to determine criminal contact, such is the example of a suspected sexual assault of a minor; certainty in the body fluid of origin may depict a precise picture of the events. The identification of loci that show differences in methylation according to the tissue of origin can aid forensic analysts in determining the origin of a DNA sample. The process of DNA methylation occurs naturally in the genome of living organisms and consists in the presence of a methyl group on the carbon 5 of a cytosine, which is typically followed by a guanine (CpG). Analyzing patterns of DNA methylation in body fluids collected from a crime scene is preferential to the analysis of proteins or mRNA since the same extracted DNA used for STR typing can be used for DNA methylation analysis. We have validated and identified loci able to discriminate blood, saliva, semen and vaginal epithelia. In the current study, we have also established the minimum amount of DNA able to provide reliable results using methodologies such as pyrosequencing and high-resolution melt (HRM) analysis for the different markers identified. Lastly, we performed an alternative bioinformatic analysis of data collected using an array that studied methylation in over 450,000 individual cytosines on the human genome. We were able to sort the locations that showed potentially higher methylation differences between body fluids and investigated over 100 of them using HRM analysis. The results of that study, allowed the identification of three new loci able to distinguish blood and two new loci able to distinguish saliva and vaginal epithelia, respectively. The use of DNA methylation patterns to aid forensic investigations started with a publication in 2010, therefore each small contribution such as this work may, similarly to what occured in the biochemistry field, result in the discovery of a method able to put the technology in the hands of forensic analysts.

epigenetics

forensic sciences

DNA

DNA methylation

pyrosequencing

high-resolution melt analysis

PCR

qPCR

body fluids

Life Sciences

Biodégradation des herbicides en sols tempérés - Contrôle des communautés bactériennes dégradantes par la bioturbation du sol

Monard, Cécile

30 April 2008

L'intensification de l'agriculture s'est accompagnée d'une utilisation importante de pesticides qui a généré une pollution généralisée des sols et des eaux, problème environnemental majeur et actuel. Sous la pression de sélection liée à l'usage régulier de pesticides (molécules xénobiotiques) des bactéries du sol se sont adaptées à ces molécules et ont acquis la capacité de les utiliser comme source nutritive et donc de les dégrader. La biodégradation constitue un service écologique majeur fournit par le sol, puisqu'elle est à la base des capacités épuratrices du sol et au-delà, de la résilience des écosystèmes. Le sol étant également un grand réservoir de biodiversité, ces bactéries dégradantes sont sous contrôle de différentes interactions biotiques et notamment celles impliquant les lombriciens, qualifiés d'organismes ingénieurs des sols de par leur action de bioturbation. Grâce à un développement méthodologique important et novateur (RT-qPCR, SIP-ARN), nous avons étudié l'impact de la bioturbation du sol par la macrofaune lombricienne sur les communautés bactériennes du sol intervenant dans la biodégradation de molécules xénobiotiques. L'atrazine a été utilisée comme molécule modèle à double titre : d'un point de vu fondamental, son utilisation pendant plus de 50 ans en France a permis aux bactéries du sol de s'adapter et au titre de l'actualité, bien qu'elle soit interdite en France depuis 2003, il s'agit toujours du principal polluant retrouvé dans les eaux souterraines et de surface. Nous avons analysé par une double approche quantitative et qualitative l'impact de la bioturbation du sol par les lombriciens sur l'abondance, l'activité et la diversité des bactéries indigènes du sol et sur celles dégradant l'atrazine. Nous avons mis en évidence que : (i) la digestion du sol par les lombriciens stimule l'activité d'une partie des bactéries du sol mais qu'une autre fraction ne résiste pas au passage dans le tube digestif des vers, (ii) la bioturbation du sol par les lombriciens génère des ‘hot spot' pour l'activité de dégradation de l'atrazine. Ainsi dans les parois de galeries les bactéries dégradantes sont sélectionnées, la dissipation de l'atrazine est rapide et les premiers acteurs du processus de dégradation ont été identifiés, (iii) la dégradation accélérée de l'atrazine dépend d'espèces bactériennes clés interagissant au sein de consortia dégradants, ainsi la diversité des bactéries dégradantes n'est pas corrélée à la fonction de dégradation. L'ensemble des résultats obtenus nous montre également que l'impact de la bioturbation par la macrofaune lombricienne sur l'activité de dégradation dépend des propriétés physico-chimiques et biologiques initiales du sol. L'ensemble de ces connaissances présente un intérêt dans un contexte de bioremédiation in situ des sols pollués puisque les lombriciens constituent une grande part de la macrofaune dans nos sols tempérés et qu'ils modifient significativement les bactéries dégradant l'atrazine au sein des microsites de sols qu'ils génèrent.

[SDV] Life Sciences

pesticides

lombriciens

biodégradation

bioturbation

atrazine

SIP-ARN

RT-qPCR

consortium bactérien

gènes atz

services écosytemiques

sols tempérés

La symbiose à Wolbachia ( -protéobactérie) : impacts sur le système immunitaire et l'immunocompétence de son hôte Armadillidium vulgare (crustacé isopode)

Chevalier, Frédéric

15 June 2011

La symbiose constitue une force évolutive majeure permettant de nombreuses adaptations des partenaires, en particulier dans la réponse des hôtes aux agents pathogènes. La bactérie endosymbiotique Wolbachia ( -protéobactérie) confère ainsi à certains insectes une résistance aux agents pathogènes humains dont ils sont les vecteurs. Chez le crustacé isopode Armadillidium vulgare, la présence de Wolbachia altère l'immunocompétence de son hôte en diminuant le taux d'hémocytes circulants (THC) et en augmentant la septicémie naturelle. La présence de Wolbachia dans les hémocytes et les organes hématopoïétiques a soulevé de nombreuses questions quant aux conséquences que cela entraîne sur le fonctionnement du système immunitaire et sur l'immunocompétence d'A. vulgare. Nous avons donc étudié l'impact de cette symbiose sur les hémocytes, l'immunocompétence et l'expression de gènes de l'immunité. Ainsi Wolbachia est présente dans plus d'un tiers des hémocytes (hybridation in situ fluorescente) et sa présence diminue la proportion d'hémocytes granulaires circulants (cytométrie en flux) chez les animaux âgés d'un an, sans affecter le THC à cet âge. L'activité phénoloxydase diminue avec l'âge et le statut symbiotique. En revanche, la présence de Wolbachia semble protéger les hémocytes de l'apoptose et augmenter l'immunocompétence d'A. vulgare lors d'une infection par Listeria ivanovii. Enfin, la quantification de l'expression des gènes de l'immunité, identifié après l'établissement du premier transcriptome de référence d'isopode (projet ANR EndoSymbArt), a révélé une tendance à la sous-expression au niveau de l'animal entier et des ovaires mais à la sur-expression dans les tissus immunitaires. La présence deWolbachia modifie donc les caractéristiques du système immunitaire aux niveaux cellulaire et humoral ainsi que l'immunocompétence d'A. vulgare. L'étude de nouveaux paramètres permettra d'établir si la présence de Wolbachia constitue réellement un avantage pour son hôte ou si au contraire la bactérie présente un coût parasitaire important.

Armadillidium vulgare

Wolbachia

immunité

hémocytes

organes hématopoïétiques

activité PO

taux d'hémocytes circulants

cytométrie en flux

RT-qPCR

Étude des mécanismes physiologiques et moléculaires de la filamentation de Sphaerotilus natans, bactérie modèle du foisonnement invasif en boues activées

Lacroix, Sébastien

03 April 2008

Le foisonnement filamenteux est un problème récurant dans de nombreuses stations d'épuration à boues activées. L'objectif de ces travaux est d'améliorer la compréhension des mécanismes physiologiques et moléculaires impliqués dans la filamentation des microorganismes, afin de pouvoir orienter de futures stratégies de lutte contre le phénomène de bulking. Sphaerotilus natans, qui peut croître réversiblement sous forme monocellulaire ou filamenteuse, a été utilisée comme bactérie modèle pour cette étude. Différents types de cultures, ainsi que des suivis par cytométrie en flux et marquage au cFDA/SE, ont montré que les diverses souches de S. natans adoptent des morphologies différentes et que les filaments croissent par divisions cellulaires successives et non par un chaînage des bactéries. Une analyse par RT-QPCR a mis en évidence que l'expression du gène sthA augmente fortement après induction de la filamentation et reste ensuite à un niveau élevé. Une comparaison de l'expression protéique des formes monocellulaire et filamenteuse, par LC-MS-MS, a permis d'identifier des protéines impliquées dans la filamentation, et notamment dans la synthèse de la gaine. La concentration intracellulaire en ARNr, mesurée par RT-QPCR, varie durant la croissance de S. natans et d'autres microorganismes, entraînant une diminution importante de l'intensité du marquage FISH, mesurée par cytométrie en flux. L'utilisation de la technique FISH pour quantifier des microorganismes est donc remise en question, d'autant plus dans des matrices aussi complexes que les boues activées. Ces observations mettent également en doute l'hypothèse, émise en utilisant ce mode de quantification, d'une déstructuration des filaments consécutive à un retour à des conditions de culture plus favorables.

Bactérie filamenteuse

Sphaerotilus natans

boues activées

bulking

mécanismes de filamentation

protéomique

ARNr

FISH

RT-QPCR

LC-MS-MS

cytométrie en flux

Distribution and activity of nitrogen-fixing bacteria in marine and estuarine waters

Farnelid, Hanna

January 2013

In aquatic environments the availability of nitrogen (N) generally limits primary production. N2-fixing prokaryotes (diazotrophs) can convert N2 gas into ammonium and provide significant input of N into the oceans. Cyanobacteria are thought to be the main N2-fixers but diazotrophs also include a wide range of heterotrophic bacteria. However, their activity and regulation in the water column is largely unknown. In this thesis the distribution, diversity, abundance, and activity of marine and estuarine heterotrophic diazotrophs was investigated. With molecular methods targeting the nifH gene, encoding the nitrogenase enzyme for N2 fixation, it was shown that diverse nifH genes affiliating with heterotrophic bacteria were ubiquitous in surface waters from ten marine locations world-wide and the estuarine Baltic Sea. Through enrichment cultures of Baltic Sea surface water in anaerobic N-free medium, heterotrophic N2 fixation was induced showing that there was a functional N2-fixing community present and isolates of heterotrophic diazotrophs were obtained. In Sargasso Sea surface waters, transcripts of nifH related to heterotrophic bacteria were detected indicating heterotrophic N2-fixing activity. Nitrogenase expression is thought to be highly regulated by the availability of inorganic N and the presence of oxygen. Low oxygen zones within the water column can be found in association with plankton. The presence of diazotrophs as symbionts of heterotrophic dinoflagellates was investigated and nifH genes related to heterotrophic diazotrophs rather than the cyanobacterial symbionts were found, suggesting that a symbiotic co-existence prevailed. Oxic-anoxic interfaces could also be potential sites for heterotrophic N2 fixation. The Baltic Sea contains large areas of anoxic bottom water. At the chemocline and in anoxic deep water heterotrophic diazotrophs were diverse, abundant and active. These findings extend the currently known regime of N2 fixation to also include ammonium-rich anaerobic waters. The results of this thesis suggest that heterotrophic diazotrophs are diverse and widely distributed in marine and estuarine waters and that they can also be active. However, limits in the knowledge on their physiology and factors which regulate their N2 fixation activity currently prevent an evaluation of their importance in the global marine N budget.

454-pyrosequencing

diazotrophs

heterotrophic bacteria

marine bacteria

marine microbial ecology

microbiology

nifH

nitrogenase

nitrogen fixation

PCR

qPCR

SWEDARP 2007/08

OSO 2007/08