Nanoparticules métalliques en matrices vitreuses pour l'amplification Raman

Nardou, Éric

20 October 2011

Les fibres optiques utilisées pour le transfert d'information présentent des pertes de signal pendant leur propagation. Ainsi, ces signaux ont besoin d'être régulièrement amplifiés. De nos jours, l'Amplification Raman, basée sur le principe de diffusion Raman stimulée, est une des techniques utilisées pour réaliser ces amplifications. Les nanoparticules de métaux nobles ont des propriétés optiques uniques provenant de l'oscillation collective des électrons lorsqu'elles interagissent avec une onde électromagnétique. Ces particules absorbent fortement le champ électromagnétique à une fréquence appelée fréquence de résonance de plasmon de surface. Ce travail de thèse concerne l'influence des nanoparticules métalliques sur l'amélioration de l'Amplification Raman. Il s'inscrit dans le cadre du projet ANR Fenoptic (2010-2012), réunissant l'entreprise Draka et plusieurs laboratoires français (ICB Dijon, CMCP Paris, LPCML Lyon), qui s'intéressent à l'intégration des nanoparticules de métaux nobles à l'intérieur des fibres optiques afin d'utiliser la résonance de plasmon de surface pour améliorer l'efficacité des amplificateurs optiques. Dans ce travail, différentes sources de nanoparticules métalliques ont été examinées (suspensions, couches, préformes de fibre optique). Les expériences ont porté sur la caractérisation (forme et position du plasmon) de nanoparticules de métaux nobles incluses en matrices vitreuses ainsi que sur des mesures de spectroscopie Raman au travers desquelles le phénomène de Diffusion Raman Exaltée de Surface (SERS) a particulièrement été étudié. Pour la première fois, nous avons mis en évidence l'exaltation du signal Raman d'une matrice vitreuse.

[SPI:OTHER] Engineering Sciences/Other

Diffusion Raman

Fibres optiques

SERS

Amplification Raman

Nanoparticules métalliques

Absorption optique

Résonance de Plasmon de surface

Films minces

Development of Enhanced Molecular Diagnostic Tools for Protein Detection and Analysis

Ebai, Tonge

January 2017

Improved diagnosis, prognosis and disease follow-up is a fundamental procedure and a constant challenge in medicine.  Among the different molecular biomarkers, proteins are the essential regulatory component in blood; hence, by developing enhanced specific and sensitive molecular tools will gives great insight into the different processes in disease treatment.  In this thesis, we build on the proximity ligation assay to develop and apply new adaptable methods to facilitate protein detection. In paper I, I present a variant of the proximity ligation assay (we call PLARCA) using micro titer plate for detection and quantification of protein using optical density as readout in the fluorometer. PLARCA detected femtomolar levels of these proteins in patient samples, which was considerably below the detection threshold for ELISA. In paper II, we developed and adapted a new method into the in situ PLA methods for detection and identification of extracellular vesicles (EVs) using flow cytometry as readout (a method we call ExoPLA).  We identified five target proteins on the surface of the Evs and using three colors, we identified the EV using flow cytometer. In paper III, we aim to improve the efficiency of in situ PLA by creating and developing new designs and versions of the assay we called Unfold probes Through comparison of detection of protein using in situ PLA versus Unfold probes, we observed considerable decrease in non-specific signals, and also a lower detection threshold. In paper IV, we describe the development of a solid phase proximity extension (sp-PEA) assay for protein detection and quantification. We compared detection of IL-8, TNF-alpha, IL-10 and IL-6 using spPEA and PEA; spPEA demonstrations over 2 orders of magnitudes in the lower detection concentrations by decreased in background noise.

protein detection

proximity ligation assays

proximity extension assay

rolling circle amplification

ELISA

flow cytometry

fluorescence microscopy

Medical Biotechnology

Medicinsk bioteknologi

Isotope-based source apportionment of black carbon aerosols in the Eurasian Arctic

Winiger, Patrik

January 2016

Aerosols change the Earth's energy balance. Black carbon (BC) aerosols are a product of incomplete combustion of fossil fuels and biomass burning and cause a net warming through aerosol radiation interactions (ari) and aerosol cloud interactions (aci). BC aerosols have potentially strong implications on the Arctic climate, yet the net global climate effect of BC is very uncertain. Best estimates assume a net warming effect, roughly half to that of CO2. However, the time scales during which CO2 emissions affect the global climate are on the order of hundreds of years, while BC is a short-lived climate pollutant (SLCP) with atmospheric life times of days to weeks. Climate models or atmospheric transport models struggle to emulate the seasonality and amplitude of BC concentrations in the Arctic, which are low in summer and high in winter/spring during the so called Arctic haze season. The high uncertainties regarding BC's climate impact are not only related to ari and aci, but also due to model parameterizations of BC lifetime and transport, and the highly uncertain estimates of global and regional BC emissions. Given the high uncertainties in technology-based emission inventories (EI), there is a need for an observation-based assessment of sources of BC in the atmosphere. We study short-term and long-term observations of elemental carbon (EC), the mass-based analog of optically-defined BC. EC aerosol concentrations and carbon-isotope-based (δ13C and ∆14C) sources were constrained (top-down) for three Arctic receptor sites in Abisko (northern Sweden), Tiksi (East Siberian Russia), and Zeppelin (on Svalbard, Norway). The radiocarbon (∆14C) signature allows to draw conclusion on the EC sources (fossil fuels vs. biomass burning) with high accuracy (&lt;5% variation). Stable carbon isotopic fingerprints (δ13C) give qualitative information of the consumed fuel type, i.e. coal, C3-plants (wood), liquid fossil fuels (diesel) or gas flaring (methane and non-methane hydrocarbons). These fingerprints can be used in conjunction with Bayesian statistics, to estimate quantitative source contributions of the sources. Finally, our observations were compared to predictions from a state of the art atmospheric transport model (coupled to BC emissions), conducted by our collaborators at NILU (Norwegian Institute for Air Research). Observed BC concentrations showed a high seasonality throughout the year, with elevated concentrations in the winter, at all sites. The highest concentrations were measured on Svalbard during a short campaign (Jan-Mar 2009) focusing on BC pollution events. Long-term observations showed that Svalbard (2013) had overall the lowest annual BC concentrations, followed by Abisko (2012) and Tiksi (2013). Isotope constraints on BC combustion sources exhibited a high seasonality and big amplitude all across the Eurasian Arctic. Uniform seasonal trends were observed in all three year-round studies, showing fractions of biomass burning of 60-70% in summer and 10-40% in winter. Europe was the major source region (&gt;80%) for BC emissions arriving at Abisko and the main sources were liquid fossil fuels and biomass burning (wood). The model agreed very well with the Abisko observations, showing good model skill and relatively well constrained sources in the European regions of the EI. However, for the Svalbard and East Siberian Arctic observatories the model-observation agreement was not as good. Here, Russia, Europe and China were the major contributors to the mostly liquid fossil and biomass burning BC emissions. This showed that the EI still needs to be improved, especially in regions where emissions are high but observations are scarce (low ratio of observations to emitted pollutant quantity). Strategies for BC mitigation in the (Eurasian) Arctic are probably most efficient, if fossil fuel (diesel) emissions are tackled during winter and spring periods, all across Eurasia. / <p>At the time of the doctoral defense, the following papers were unpublished and had a status as follows: Paper 2: Manuscript. Paper 3: Manuscript.</p>

Black Carbon

Radiocarbon

Air Pollution

Arctic Amplification

Climate Change

Arctic Haze

Atmospheric Transport Modeling

Emission Inventory

Carbon Isotopes

Effect of haptic guidance and error amplification robotic training interventions on the immediate improvement of timing among individuals that had a stroke / Effet de l’entrainement robotisé par réduction de l’erreur et augmentation de l’erreur sur le timing du mouvement chez la personne ayant eu un accident vasculaire cérébral

Bouchard, Amy

January 2016

Abstract : Many individuals that had a stroke have motor impairments such as timing deficits that hinder their ability to complete daily activities like getting dressed. Robotic rehabilitation is an increasingly popular therapeutic avenue in order to improve motor recovery among this population. Yet, most studies have focused on improving the spatial aspect of movement (e.g. reaching), and not the temporal one (e.g. timing). Hence, the main aim of this study was to compare two types of robotic rehabilitation on the immediate improvement of timing accuracy: haptic guidance (HG), which consists of guiding the person to make the correct movement, and thus decreasing his or her movement errors, and error amplification (EA), which consists of increasing the person’s movement errors. The secondary objective consisted of exploring whether the side of the stroke lesion had an effect on timing accuracy following HG and EA training. Thirty-four persons that had a stroke (average age 67 ± 7 years) participated in a single training session of a timing-based task (simulated pinball-like task), where they had to activate a robot at the correct moment to successfully hit targets that were presented a random on a computer screen. Participants were randomly divided into two groups, receiving either HG or EA. During the same session, a baseline phase and a retention phase were given before and after each training, and these phases were compared in order to evaluate and compare the immediate impact of HG and EA on movement timing accuracy. The results showed that HG helped improve the immediate timing accuracy (p=0.03), but not EA (p=0.45). After comparing both trainings, HG was revealed to be superior to EA at improving timing (p=0.04). Furthermore, a significant correlation was found between the side of stroke lesion and the change in timing accuracy following EA (r[subscript pb]=0.7, p=0.001), but not HG (r[subscript pb]=0.18, p=0.24). In other words, a deterioration in timing accuracy was found for participants with a lesion in the left hemisphere that had trained with EA. On the other hand, for the participants having a right-sided stroke lesion, an improvement in timing accuracy was noted following EA. In sum, it seems that HG helps improve the immediate timing accuracy for individuals that had a stroke. Still, the side of the stroke lesion seems to play a part in the participants’ response to training. This remains to be further explored, in addition to the impact of providing more training sessions in order to assess any long-term benefits of HG or EA. / Résumé : À la suite d’un accident vasculaire cérébral (AVC), plusieurs atteintes, comme un déficit de timing, sont notées, et ce, même à la phase chronique d’un AVC, ce qui nuit à l’accomplissement de tâches quotidiennes comme se vêtir. L’entrainement robotisé est un entrainement qui est de plus en plus préconisé dans le but d’améliorer la récupération motrice à la suite d’un AVC. Par contre, la plupart des études ont étudié les effets de l’entrainement robotisé sur l’amélioration de l’aspect spatial du mouvement (ex : la direction du mouvement), et non l’aspect temporel (ex : timing). L’objectif principal de ce projet était donc d’évaluer et de comparer l’impact de deux entrainements robotisés sur l’amélioration immédiate du timing soit : la réduction de l’erreur (RE), qui consiste à guider la personne à faire le mouvement désiré, et l’augmentation de l’erreur (AE), qui nuit au mouvement de la personne. L’objectif secondaire consistait à explorer s’il y avait une relation entre le côté de la lésion cérébrale et le changement dans les erreurs de timing suivant l’entrainement par RE et AE. Trente-quatre personnes atteintes d’un AVC au stade chronique (âge moyen de 67 ± 7 années) ont participé à cette étude, où ils devaient jouer à un jeu simulé de machine à boules. Les participants devaient activer une main robotisée au bon moment pour atteindre des cibles présentées aléatoirement sur un écran d’ordinateur. Les participants recevaient soit RE ou AE. Une ligne de base et une phase de rétention étaient données avant et après chaque entrainement, et elles étaient utilisées pour évaluer et comparer l’effet immédiat de RE et AE sur le timing. Les résultats ont démontré que RE permet d’améliorer les erreurs de timing (p=0,03), mais pas AE (p=0,45). De plus, la comparaison entre les deux entrainements a démontré que RE était supérieur à AE pour améliorer le timing (p=0,04). Par ailleurs, une corrélation significative a été notée entre le côté de la lésion cérébrale et le changement des erreurs de timing suivant AE (r[indice inférieur pb]=0,70; p=0,001), mais pas RE (r[indice inférieur pb]=0,18; p=0,24). En d’autres mots, une détérioration de l’exécution de la tâche de timing a été notée pour les participants ayant leur lésion cérébrale à gauche. Par contre, ceux ayant leur lésion à droite ont bénéficié de l’entrainement par AE. Bref, l’entrainement par RE peut améliorer les erreurs de timing pour les survivants d’AVC au stade chronique. Toutefois, le côté de la lésion cérébrale semble jouer un rôle important dans la réponse à l’entrainement par AE. Ceci demeure à être exploré, ainsi que l’impact d’un entrainement par RE et AE de plus longue durée pour en déterminer leurs effets à long terme.

Motor learning

Haptic guidance

Error amplification

Timing

Stroke

Apprentissage moteur

Réduction de l’erreur

Augmentation de l’erreur

Accident vasculaire cérébral

Investigation of Strategies for Improving STR Typing of Degraded and Low Copy DNA from Human Skeletal Remains and Bloodstains

Ambers, Angie D.

08 1900

Forensic STR analysis is limited by the quality and quantity of DNA. Significant damage or alteration to the molecular structure of DNA by depurination, crosslinking, base modification, and strand breakage can impact typing success. Two methods that could potentially improve STR typing of challenged samples were explored: an in vitro DNA repair assay (PreCR™ Repair Mix) and whole genome amplification. Results with the repair assay showed trends of improved performance of STR profiling of bleach-damaged DNA. However, the repair assay did not improve DNA profiles from environmentally-damaged bloodstains or bone, and in some cases resulted in lower RFU values for STR alleles. The extensive spectrum of DNA damage and myriad combinations of lesions that can be present in forensic samples appears to pose a challenge for the in vitro PreCR™ assay. The data suggest that the use of PreCR™ in casework should be considered with caution due to the assay’s varied results. As an alternative to repair, whole genome amplification (WGA) was pursued. The DOP-PCR method was selected for WGA because of initial primer design and greater efficacy for amplifying degraded samples. Several modifications of the original DOP-PCR primer were evaluated. These modifications allowed for an overall more robust amplification of damaged DNA from both contemporary and historical skeletal remains compared with that obtained by standard DNA typing and a previously described DOP-PCR method. These new DOP-PCR primers show promise for WGA of degraded DNA.

human skeletal remains

degraded DNA

DNA repair

whole genome amplification

DOP-PCR

DNA fingerprinting.

Forensic genetics.

DNA -- Synthesis.

Caracterização genética de javalis por meio de maracdores microssatélites /

Corrêa da Silva, Paula Vianna.

January 2007

Orientador: Jeffrey Frederico Lui / Banca: Humberto Tonhati / Banca: Selma de Fátima Grossi / Resumo: A ocorrência de híbridos entre javalis e suínos, tanto na natureza como em cativeiro, é bastante comum. Assim, tem-se detectado polimorfismo em javalis, variando o número de cromossomos de 36 a 38. Nesse sentido, objetivou-se, com este trabalho, caracterizar geneticamente javalis (Sus scrofa scrofa) puros e híbridos criados no Brasil, por meio de loci de microssatélites (STRs) do suíno doméstico (Sus scrofa domestica). Para efeito de classificação, os animais foram agrupados, segundo análise de pedigree e número diplóide (2n), em 5 grupos genéticos: grupo I, constituído de 59 suínos domésticos; grupo II, formado por 46 javalis puros de origem; grupo III, constituído de 3 híbridos, com 2n=36, provenientes de acasalamentos entre híbridos e retrocruzamentos; grupo IV, representando 30 híbridos com suíno doméstico de ploidia igual a 37 cromossomos; e grupo V, constituídos de 10 híbridos também com o doméstico, porém com 2n=38, conhecidos popularmente como Javaporcos, devido à similaridade cariotípica e fenotípica com o suíno doméstico. O DNA genômico foi extraído e, posteriormente, amplificou-se, pela técnica de PCR, os fragmentos desses microssatélites - IGF1, ACTG2, TNFB -, os quais foram desenvolvidos para a subespécie Sus scrofa domestica. As condições de amplificação foram padronizadas para as amostras de javali realizadas em um termociclador, com as temperaturas de anelamento variando para cada primer. Ao final das amplificações, os produtos dos microssatélites foram colocados em um seqüenciador capilar modelo ABI 3100 Avant (Applied Biosystems). A partir dos resultados obtidos no presente trabalho, concluiu-se que os microssatélites IGF1, ACTG2 e TNFB, usados em suínos, são eficiente na amplificação heteróloga e podem ser aplicados em javali. Os javalis puros se diferenciam geneticamente dos suínos e dos híbridos...(Resumo completo, clicar acesso eletrônico abaixo) / Abstract: The occurrence of crossbred animals between wild boar and pigs, both in nature and in captivity, is quite common. Thus, polymorphism has been detected among wild boar, varying chromosomes from 36 to 38. Considering this, the objective of the present work was to perform a genetic characterization of wild boar and crossbred boars raised in Brazil, through. the microsatellites loci (STRs) of the domestic pig (Sus scrofa domestica). For classification purposes, the animals were grouped according to pedigree analysis and diploid number (2n) into 5 genetic groups: group I, composed of 59 domestic pigs with 2n = 38; group II, composed of 46 wild boar with 2n = 36 imported from France in 1997; group III, composed of 3 crossbred animals with 2n = 36 from the crossing between crossbred and backcrossing animals; group IV, composed of 30 crossbred animals with domestic pig with ploidy equal to 37 chromosomes and group V, composed of 10 crossbred animals also with domestic pig, but with 2n = 38, popularly known as "Boarpigs" due to their karyotypic and phenotypic similarity with the domestic pig. The genomic DNA was extracted and, after that, the fragments of these microsatellites - IGF1, ACTG2, TNFB - were amplified through the PCR technique, which were developed for the Sus scrofa domestica species. The amplification conditions were standardized for wild boar samples and performed in a thermocycler with the annealing temperatures varying for each primer. At the end of amplifications, the products of microsatellites were placed in a genetic analyzer model ABI 3100 Avant (Applied Biosystems). Considering the results of this research, the microsatellites IGF1, ACTG2 and TNFB used for pigs, were considered to be efficient on the heterologous amplifications and can also be applied on wild boar. The wild boar differs genetically from pigs and crossbreds... (Complete abstract, click electronic access below) / Mestre

Genética animal.

Alleles. eng

Boarpigs. eng

Conservation. eng

Genetic differentiation. eng

Genetic diversity. eng

Heterolugous amplification. eng

Sequenciamento e análise de um banco de cDNA de glândulas salivares de Rhynchosciara americana e caracterização do gene RaDup / Sequencing and analysis of a EST Bank from salivary glands of Rhynchosciara americana and characterization of the gene RaDup

Siviero, Fábio

20 April 2004

Durante o desenvolvimento deste projeto adotou-se como estratégia o sequenciamento de ESTs, com a finalidade de encontrar mensagens relacionadas com desenvolvimento, metabolismo e principalmente amplificação/politenização em glândulas salivares de Rhynchosciara americana, um díptero (Sciarídeo) que apresenta cromossomos politênicos e amplificação gênica rigidamente regulada ao longo do desenvolvimento larval, tanto neste tecido quanto em outros. Um total de 8193 ESTs foi gerado, estas foram anotadas e categorizadas segundo os termos do Gene Ontology Consortium, proporcionando uma visão geral do status metabólico, como em um Northern eletrônico, de um ponto importante no desenvolvimento desta espécie, quando surgem amplificações gênicas específicas e a glândula salivar necessita secretar as proteínas do casulo. Outros frutos deste seqüenciamento foram a determinação de 91 polimorfismos e a criação de uma tabela de códon usage. Diversos ESTs foram identificados com potencial envolvimento com os endociclos observados neste tecido, destes, RaDup e RaMCM5 foram selecionados para estudo. Suas regiões genômicas foram isoladas e suas localizações cromossômicas foram identificadas, em relação a RaDup, toda a porção codificante de seu mensageiro e 12kb de DNA genômico contendo seu gene foram seqüenciados, revelando sua estrutura gênica. Anticorpos foram produzidos para detectar esta proteína, gerando evidências de sua participação tanto na replicação mitótica como nos endociclos presentes nas glândulas salivares. A localização cromossômica de RaDup é um dado muito interessante, pois pela primeira vez um pufe amplificado é relacionado com um gene regulatório. / In this work EST sequencing was used as strategy to find messages related to development, metabolism and polyteny/amplification in salivary glands of Rhynchosciara americana, a dipteran (Sciaridae) that shows in this tissue giant polytene chromosomes and gene amplification tightly regulated throughout development of the larvae. A total of 8193 EST sequences were generated, annotated and categorized using Gene Ontology Consortium terms, providing a general view of the metabolic status, like an electronic Northern, of an important point in development of the larvae, that shows where specific genes are amplified and the salivary gland needs to secrete the proteins to form the cocoon. Other data include determination of 91 SNPs and a statistic of codon usage. Several ESTs were identified with potential connection to endocicles, from these RaDup and RaMCM5 were selected for further studies. Both chromosomal loci were identified and genomic regions isolated, for RaDup the coding region of its mRNA and 12kb of genomic region were completely sequenced, revealing its gene structure, and antibodies were raised against this protein, making evident data about its involvement in replication in mitotic cells and in endocicles in salivary glands. About the chromosomal locus of RaDup, it becomes very interesting, because for the first time one amplified puff can be related to a regulatory gene.

Amplificação de genes

Cell cycles

Ciclo celular

Dipteran

Dipteros

Endociclos

Endocycle

Gene amplification

Politene

Politenia

Puff

Rhynchosciara

Rhynchosciara

Sciaridae

Sciarídeos

Prevalência de Chlamydia trachomatis em mulheres inférteis e gestantes assintomáticas

Gomez, Deborah Beltrami

January 2016

Introdução: A infecção urogenital por Chlamydia trachomatis é a doença sexualmente transmissível bacteriana mais prevalente no mundo e afeta principalmente mulheres jovens sexualmente ativas. Infecções não tratadas podem provocar complicações reprodutivas decorrentes do dano tubáreo. Na gestação, aumenta o risco de parto prematuro, baixo peso ao nascer, morte perinatal, conjuntivite e pneumonia neonatal. Existem poucos dados brasileiros referentes à epidemiologia dessa infecção no nosso meio. O objetivo desse estudo foi determinar a prevalência de C. trachomatis em mulheres inférteis e em gestantes. Método: Foram analisadas transversalmente 77 mulheres inférteis e 60 gestantes assintomáticas. Foram coletadas amostras urinárias para ensaio de PCR e amostras sanguíneas para pesquisa de anticorpos IgG através da técnica de imunofluorescência indireta. Todas as participantes responderam um questionário referente ao seu histórico clínico e ginecológico. Resultados: A prevalência, tanto no ensaio de PCR quanto na imunofluorescência indireta (IgG) para C. trachomatis foi similar entre os grupos. Encontramos anticorpos IgG presentes em 61% das mulheres inférteis e em 56,7% das gestantes. Houve somente 1 PCR positivo no grupo das inférteis (1,3%) e nenhum do grupo das gestantes. Conclusão: Encontramos alta prevalência de anticorpos IgG para C. trachomatis em mulheres inférteis e em gestantes, mas verificamos baixa prevalência de PCR positivo nas participantes. A presença de IgG correlacionou-se com comportamento sexual e tabagismo. / Background: Chlamydia trachomatis (CT) is the most prevalent sexually transmitted bacterial infection and affects mainly young, sexually active, women. Untreated infection may lead to reproductive complications due to tubal damage. Infections during pregnancy may cause preterm labor, low birth weight, perinatal death and neonatal conjunctivitis and pneumonia. There is little data on CT infection in Brazil. The aim of this study was to determine CT prevalence on infertile and pregnant women. Methods: A cross-sectional study included 77 infertile and 60 asymptomatic pregnant women. First void urine was tested to CT using PCR and blood samples were collected for CT IgG antibodies testing using Indirect Immunofluorescence. A questionnaire about medical, gynecological and sexual history was applied to all participants. Results: We found statistically similar prevalence of PCR and IgG antibodies between groups. This study observed a 61% prevalence of CT IgG antibodies in infertile women and 56,7% in pregnant women. PCR was positive in only one (1,3%) infertile woman and in none of the pregnant. Conclusion: A high prevalence of C. trachomatis IgG antibody in Brazilian pregnant and infertile women, but a low prevalence of positive PCR on urine samples were demonstrated. CT antibodies were associated with sexual behavior and smoking.

Chlamydia trachomatis

Infertilidade feminina

Reação em cadeia da polimerase

Chlamydia trachomatis

Prevalence

Nucleic acid amplification techniques

Infertility

Female

Fluorescent antibody technique

Etude de la prévalence des aneuploïdies dans les produits d'avortements spontanés : intéret des techniques FISH et MLFA pour la détection des remaniements chromosomiques. / Study of the prevalence of aneuploidies in spontaneous abortion products : FISH and MLFA techniques for the detection of chromosome changes.

Haoud, Khadidja

22 January 2014

L’avortement spontané (AS) désigne la perte du produit de conception avant sa viabilité, c'est-à-dire avant la 22e semaine d’aménorrhée, ou un poids fœtal inférieur à 500 g. La cause génétique est à l’origine de plus des deux tiers des AS, les aneuploïdies autosomiques, représentant à elles seules jusqu’à 70% des pertes fœtales du 1er trimestre. Le caryotype présente une très bonne sensibilité en ce qui concerne le dépistage des trisomies autosomiques (13, 18 et 21) et des aneuploïdies affectant les chromosomes sexuels, mais il montre d’importantes limites, d’une part en raison des échecs de culture cellulaire et d’autre part en raison de l’existence de remaniements non détectables au caryotype standard. Actuellement plusieurs techniques moléculaires de dépistage rapides des aneuploïdies liées aux échecs de grossesses ont été vérifiées : 1°) la fluorescence in situ par hybridation (FISH) 2°) l’amplification multiplex de sondes nucléiques dépendant des ligatures (MLPA). Ces deux méthodes présentent l’avantage d’être réalisables, sans culture préalable, sur noyaux en interphase ou sur ADN extrait et de permettre la détection d’anomalies cryptiques. Notre étude repose sur l’étude cytogénétique des produits d’AS pour mettre en évidence les anomalies chromosomiques les plus fréquentes à l’origine de ces pertes fœtales et d’en mieux appréhender les mécanismes de survenue. Elle a été réalisée sur 220 patientes âgées de 19 à 45 ans, et était fondée sur l’analyse directe par FISH sur noyaux interphasiques (AneuVysionTM) de prélèvements de villosités choriales et sur l’analyse de l’ADN extrait de tissus fœtaux par MLPA afin de révéler d’éventuelles aneuploïdies et micro-remaniements. L’âge gestationnel au moment des prélèvements était compris entre 7 et 38 semaines d’aménorrhée. Sur un total de 151 échantillons analysés par AneuVysionTM, 10 anomalies chromosomiques ont été observées: 3 trisomies 21, 1 trisomie 18, 1 trisomie 13, 1 mosaïque 46,XX/47,XX+21, 3 triploïdies et 1 monosomie X (Turner). Par ailleurs, sur les 69 autres échantillons analysés par MLPA, 6 étaient ininterprétables. Les anomalies trouvées par cette technique étaient: 2 monosomies X. Pour les échantillons restants, la MLPA a été négative. Nous avons en parallèle réalisé une étude rétrospective fondée sur l’analyse comparative d’un échantillon recruté à Sidi Bel Abbès, de femmes ayant subi un AS et admises à la maternité del’hôpital Hassani Abdelkader de Sidi Bel Abbès et d’un échantillon recruté à Clermont-Ferrand de femmes ayant subi un AS et pour lesquelles un prélèvement pour établir le caryotype du produit de fausse-couche avait été adressé dans le service de cytogénétique du CHU Estaing de Clermont-Ferrand. Cette étude a couvert une période de six années, allant de janvier 2005 à décembre 2010. Les techniques de FISH et de MLPA représentent des outils simples, rapides et sensibles pour la détection des remaniements chromosomiques. Elles représentent une alternative très intéressante à la culture cellulaire, et permettent le diagnostic de désordres génomiques indécelables par les techniques conventionnelles. / Spontaneous abortion (SA) is the loss of the product of fertilization before its viability, that is, before22 weeks of gestation or fetal weight less than 500 g. Genetic causes account for more than two thirds of SA, autosomal aneuploidies alone accounting for up to 70% fetal loss. Chromosomal cytogenetic techniques show significant limitations on the one hand because of the failures of cell culture, and secondly because of the existence of undetectable alterations to the standard karyotype. It was therefore planned to use molecular techniques :- Fluorescent in situ hybridization (FISH)- Multiplex ligation-dependent probe amplification (MLPA). Both techniques have the advantage of being achievable without prior culture of cores interphase or DNA extracted and to enable detection of cryptic abnormalities. The project is based on cytogenetic study of AS products to highlight the most frequent chromosomal abnormalities causing fetal losses, and to better understand their occurrence. Our study was performed on 220 patients from 19 to 45 years, and was based on the direct analysis by FISH on interphase nuclei (AneuVysionTM) of chorionic villus sampling and analysis of DNA extracted fetal tissue by MLPA to reveal any aneuploidy and rearrangements. The gestational age of the samples ranged from the 7th to the 38th week of gestation. In a total of 151 samples analyzed by AneuVysionTM, 10 chromosomal abnormalities were observed: three trisomies 21, one trisomy 18, one trisomy 13, one mosaic 46,XX/47,XX+21, 3 triploidies and one monosomy X (Turner). In addition, among the other 69 samples analyzed by MLPA, 6 were uninterpretable. The abnormalities found by this technique were 2 monosomies X. For the remaining samples, the MLPA was negative. We conducted a retrospective parallel study based on the analysis of a sample recruited in Sidi Bel Abbes, women who have had an AS and were admitted to the maternity hospital Abdelkader Hassani, Sidi Bel Abbes ; and a sample recruited in Clermont-Ferrand : women who underwent AS for which a levy to establish the karyotype product miscarriage had been addressed in the Department of Cytogenetics of CHU Estaing, Clermont-Ferrand. This study covered a period of six years, from January 2005 to December 2010. The techniques of FISH and MLPA are simple, rapid and sensitive tools for the detection of chromosomal rearrangements. They represent a very interesting alternative to cell culture and allow diagnosis for genomic disorders undetectable by conventional techniques.

Avortement spontané

Aneuploïdie

MLPA (génétique)

Technique FISH

Spontaneous abortion

Aneuploidy

Fluorescent in situ hybridization

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Begomovírus de plantas de pimentão e tomate no Estado de São Paulo : ocorrência, variabilidade, identificação de biótipos de bemisia tabaci e de resistência em capsicum spp /

Rocha, Kelly Cristina Gonçales , 1978-

January 2009

Orientador: Renate Krause Sakate / Banca: Carlos Frederico Wilcken / Banca: Arlete Marchi Tavares de Melo / Banca: Marcelo Agenor Pavan / Banca: Antonio Carlos Maringoni / Resumo: Considerando o aumento de begomovírus e mosca-branca no campo o presente trabalho teve como objetivos a detecção, a caracterização molecular e a análise da diversidade genética de begomovírus em pimentão e tomateiro em diferentes municípios do Estado de São Paulo: Piraju, Tejupá, Santa Cruz do Rio Pardo, São Pedro do Turvo, São Miguel Arcanjo, Itapetininga, Lins, Sabino, Timburí, Iacanga, Pirajuí, Avaí, Reginópolis e Salto; a identificação de biótipos de B. tabaci por meio da amplificação do gene mitocondrial (citocromo oxidase I - mtCOI) seguido de seqüenciamento ou RFLP utilizando a enzima Taq I e a avaliação para resistência de acessos de Capsicum spp. a dois isolados de ToSRV. A análise da variabilidade foi realizada por meio de seqüenciamento da região da capa protéica (DNA-A) com oligonucleotídeos universais e, paralelamente, as mesmas amostras foram testadas por amplificação por círculo rolante (RCA) sendo, posteriormente, clivadas com a enzima de restrição HpaII. Um total de 812 amostras foi analisado, sendo 709 de pimentão e 103 de tomate. Por PCR tradicional, foram detectadas positivas para presença de begomovírus 98 amostras provenientes de pimentão e 39 de tomateiro, e por RCA-PCR, foram 332 e 82 respectivamente, evidenciando maior sensibilidade desta técnica. Dessas amostras, foram seqüenciadas 39 de pimentão e 25 de tomateiro, verificando-se ocorrência prevalente da espécie ToSRV no estado de São Paulo. Infecção mista com ToSRV e ToYVSV foi observada tomateiro. Por RCA-RFLP, foram observados quatro padrões de clivagem com a enzima HpaII e todos foram confirmados como sendo da espécie ToSRV indicando variabilidade molecular intraespecífica. Para tomateiro, foram observados 18 padrões de restrição, dois idênticos aos verificados em plantas de pimentão indicando, possivelmente, infecção pelos mesmos isolados de ToSRV, porém... (Resumo completo, clicar acesso eletrônico abaixo) / Abstract: Considering the high incidence of begomoviruses and the whitefly on the field, the objetives of this work were to analyze the genetic diversity of begomoviruses infecting pepper and tomato plants in different counties of São Paulo State: Piraju, Tejupá, Santa Cruz do Rio Pardo, São Pedro do Turvo, São Miguel Arcanjo, Itapetininga, Lins, Sabino, Timburí, Iacanga, Pirajuí, Avaí, Reginópolis and Salto; the identification of biotypes of B. tabaci through the amplification of the mitochondrial gene (cytochrome oxidase I) 4 followed by sequencing the gene or analysis by RFLP using the enzyme TaqI and the evaluation of Capsicum spp. for the resistance source for two isolates of ToSRV. The coat protein from the DNA A of the begomovirus was amplified and sequenced, and the same samples were amplified by rolling circle amplification (RCA) followed by analysis by RCA-RFLP using the HpaII enzyme. A total of 812 samples were analyzed, 709 from pepper and 103 from tomato. By PCR, 98 samples from pepper and 39 from tomato were positives for the presence of begomoviruses, while by RCA-PCR 332 and 82 respectively. Thirty-nine samples from pepper and 25 from tomato were sequenced indicating the prevalence of the ToSRV species in São Paulo State. Mixed infections with ToSRV and ToYVSV were found in tomato plants. By RCA-RFLP four restriction profiles were found for ToSRV in pepper plants. In tomato 18 profiles were observed: two identical as observed for ToSRV in pepper, indicating possible infection with the same ToSRV isolates, a profile for ToSRV and ToYVSV mixed infections and also different profiles for ToSRV isolates didn't found in pepper plants. The sequencing of 17 samples of B. tabaci mitochondrial citochrome oxidase I gene and analysis by Taq I digestion of whiteflies collected in growers areas of pepper and tomato indicated only the presence of the B biotype... (Complete abstract click electronic access below) / Doutor

Pimentão.

Hortaliças.

Mosca branca.

Solanum lycopersicum. eng

Chillies. eng

Vegetables. eng

Tolerence. eng

Rolling circle amplification. eng

Whitefly biotypes. eng