Phylogenetic Analysis of Subtribe Alopecurinae (Poaceae)

Boudko, Ekaterina

12 March 2014

Subtribe Alopecurinae (Poeae, Poaceae) sensu lato‘s seven genera share interesting morphological similarities (dense spicate panicles and one-flowered spikelets) that were widely thought to have a common origin. However, recent molecular evidence for three of the genera has suggested that the subtribe may be polyphyletic. To test this, five DNA regions were sequenced and analyzed using phylogenetic methods. Results confirm that Alopecurinae s.l. as presently treated is polyphyletic and should be dissolved. Additionally, the genus Cornucopiae may be just another Alopecurus. Limnas and Pseudophleum are not closely allied to Alopecurus or each other, and are even further from Phleum. Phleum is a distinct lineage that is not closely allied to any other included Alopecurinae genus. Evidence for revising infrageneric classifications of Alopecurus and Phleum is presented, as is evidence for separating A. magellanicus into two or more subspecies.

Poaceae

Alopecurinae

Poinae

Poeae

Phleinae

Pooideae

Phylogenetics

Phylogeny

Polyphyly

Molecular

Botany

Taxonomy

Systematics

Alopecurus

Phleum

Beckmannia

Limnas

Cornucopiae

Rhizocephalus

Pseudophleum

Plant

Grass

DNA sequencing

trnT-trnL-trnF

rpoB-trnC

matK

ITS

ETS

Convergent Evolution

Hybridization

Morphology

Evolution

Genetics

Flora

Subtribe

An analysis of the effect of transformation on global– and gene–specific DNA methylation in four cultured cell lines / Jean du Toit

Du Toit, Jean

January 2010

DNA methylation plays a role in several biological functions, such as gene expression regulation, and several endogenous and exogenous factors affect these DNA methylation patterns in the cell. One such alteration of a cell line's DNA methylation pattern is caused by the insertion of a vector into the cell line. Using the cytosine–extension assay and realtime methylation–specific PCR, alterations of DNA methylation levels on both global and gene–specific levels were investigated. In some cell lines the cellular transformation led to an increase in DNA methylation levels, and in others a decrease in DNA methylation amounts was observed. The same phenomenon was seen in the promoter regions of specific genes, showing that vector–insertion into a cell line caused DNA methylation alterations in many regions of the genome. These alterations in DNA methylation are investigated in this reduced representation study using enrichment of the methylated fraction of fragmented DNA and subsequent GS FLX Titanium sequencing of these methylated fragments. The results of sequence data analysis showed that methylated fragments are distributed over the whole genome, but could be related to only a few specific genes. These results have implications for cell culture work, biotechnological applications and uses in gene therapy. / Thesis (M.Sc. (Biochemistry))--North-West University, Potchefstroom Campus, 2011.

Epigenetics

DNA methylation

Cell culture

Transfection

DNA sequencing

Cytosine-extension assay

Real-time methylation-specific PCR

Epigenetika

DNA metilering

Selkulture

Transfeksie

DNS volgorde-bepaling

Sitosien-verlengingstoets

Intydse metilering-spesifieke PKR

Evaluation of molecular methods used for the rapid detection of multi-drug resistant Mycobacterium tuberculosis

Hansen, Tarrant William

January 2008

Tuberculosis remains a major public health issue globally, with an estimated 9.2 million new cases in 2006. A new threat to TB control is the emergence of drug resistant strains. These strains are harder to cure as standard anti-tuberculosis first line treatments are ineffective. Multi Drug Resistant Tuberculosis (MDR-TB) is defined as Mycobacterium tuberculosis that has developed resistance to at least rifampicin and isoniazid, and these strains now account for greater than 5% of worldwide cases. Mutations within the Rifampicin Resistance Determining Region (RRDR) of the rpoB gene are present in greater than 95% of strains that show rifampicin resistance by conventional drug susceptibility testing. As rifampicin mono resistance is extremely rare, and rifampicin resistance is usually associated with isoniaizd resistance, the RRDR region of the rpoB gene is a very useful surrogate marker for MDR-TB. Many molecular assays have been attempted based on this theory and have had varied levels of success. The three methods evaluated in this study are DNA sequencing of the rpoB, katG and inhA genes, the Genotype MTBDRplus line probe assay (Hain Lifesciences) and a novel method incorporating Real-Time PCR with High Resolution Melt analysis targeted at the RRDR using the Rotorgene 6000 (Corbett Lifesciences). The sensitivity for the detection of rifampicin resistance was far better using DNA sequencing or the commercially available line probe assay than detection by the Real-Time PCR method developed in this study.

Genome diversity and evolution in canine transmissible venereal tumour

Strakova, Andrea

January 2018

The canine transmissible venereal tumour (CTVT) is a contagious cancer that is naturally transmitted between dogs by the allogeneic transfer of living cancer cells during coitus. CTVT first arose several thousand years ago and has been reported in dog populations worldwide. The goals of this Thesis were (1) to gain further understanding of CTVT distribution patterns and prevalence around the world, (2) to use genetics to trace the historical spread of CTVT and (3) to map the genetic as well as phenotypic diversity of CTVT tumours around the world. To understand the distribution patterns of CTVT, I obtained information from 645 veterinarians and animal health workers in 109 countries, and generated a snapshot of the locations in which this disease is found. Additionally, as preparation for further genetic analysis, I collected samples from over one thousand CTVT cases from more than 50 countries, optimised methods for high-throughput DNA extraction and quantification and optimised a qPCR-based assay for CTVT diagnosis and host contamination detection. With the goal of tracing the historical spread of CTVT and learning about the genetic diversity of this disease, I sequenced complete mitochondrial genomes of 449 CTVT tumours and their matched hosts. The analysis of the CTVT mitochondrial diversity revealed that CTVT has captured mitochondrial DNA (mtDNA) through horizontal transfer events at least five times during the history of the lineage, delineating five tumour clades. CTVT appears to have spread rapidly around the world within the last 2,000 years, perhaps transported by dogs travelling along historic maritime trade routes. This work indicated that negative selection has operated to prevent accumulation of deleterious mutations in captured mtDNA, and that recombination has caused occasional mtDNA re-assortment. A histology-based screen of CTVT clades did not show any significant phenotypic differences between groups. In order to determine how the five mtDNA clades relate to each other, I analysed data from 539 CTVT exomes. This revealed that a single canine mtDNA haplogroup has recurrently and recently undergone multiple horizontal transfer events. Analysis of this haplotype highlighted a number of candidate genetic variants which may be conferring a selective advantage to this haplotype in CTVT, possibly by influencing mtDNA transcription or replication. Overall, genetic and phenotypic analysis of CTVT tumours from across the globe has broadened our understanding of CTVT diversity, and provided important insights into the biology of a unique transmissible cancer.

Epidemiologia molecular do papilomavírus humano em uma amostra de mulheres do estado de Alagoas / Molecular epidemiology of human papillomavirus in woman of Alagoas

Santos Filho, Moezio de Vasconcellos Costa

16 February 2012

The Human Papillomavirus (HPV) is a virus of the Papillomaviridae family and its genome consists of DNA. It is the main cause of viral sexual transmission. Cervical cancer or uterine colon cancer is the second most common occurrence among women worldwide. Recent studies have proven that some types of HPV are mainly responsible for the development of this type of cancer. In accordance to its oncogenic activity this viral group was divided in low and high risk types. Brazil does not have a representative amount of data related to the prevalence of HPV infection. The incidence data of the virus is obtained through the analysis of carriers of the invasive carcinoma of uterine colon, cervical intraepithelial neoplasias, and others types of infections associated. Molecular assays have been showing throughout the years an excellent sensitivity and specificity in the detection of the HPV s DNA. Nowadays, in situ hybridization techniques are being used as method of choice for the detection of the viral DNA. In many studies, the Polymerase Chain Reaction (PCR) with the application of the primers MY09 and MY11 have shown efficiency in viral tracking, consequently, the development of molecular diagnostics allow monitoring of the disease, decreasing mortality rates caused by cancer of the cervix. The DNA sequencing is an efficient methodology used for the molecular characterization of the viral types, which allows the accomplishment of the alignment for similarity of the sequences obtained through others that were already identified and deposited in the GenBank. The current study s purpose was to identify the different types of HPV and the presence of co-infections through PCR and sequencing of a hyper-variable region of the L1 gene. The studied sample consisted of 515 female volunteers, which 111 (21.55%) presented the incidence of the HPV DNA. Within the acquired specimens, 50% were considered high oncogenic risk (the major incidence was types 16 and 58) and 7.21% had multiple infection. The determination of the base sequencing of the L1 gene is essential to the identification of the viral type. However, the sequencing of the complete gene and both DNA chains become financially unviable for the majority of the specialized laboratories. A practical approach applied in this study was to determine the sequencing of a specific region of the L1 gene with 450pb, where the identification of the HPV became possible by following this methodology. The techniques used showed the necessity of the application of a more sensible and specific viral diagnosis, which contributes to the viral infection control and to the reduction of the mortality rate caused by cervical cancer. / Fundação de Amparo a Pesquisa do Estado de Alagoas / O Papilomavírus Humano (HPV) é um vírus da família Papillomaviridae e possui o seu genoma constituído de DNA. É o causador da transmissão sexual viral de maior frequência. O câncer cervical ou câncer de colo de útero possui a segunda maior ocorrência nas mulheres de todo o mundo. Estudos recentes têm comprovado que alguns tipos de HPV são os principais responsáveis pelo desenvolvimento deste tipo de câncer. De acordo com a sua atividade na carninogênese esse grupo viral foi dividido em tipos de baixo e de alto risco oncogênico. O Brasil ainda não possui uma quantidade representativa de dados relacionados à prevalência de infecção por HPV, os dados de incidência do vírus são obtidos através da análise de portadores de carcinoma invasivo de colo uterino, neoplasias intraepiteliais cervicais e outros tipos de infecções associadas. Ensaios moleculares vêm mostrando ao longo dos anos uma alta sensibilidade e especificidade na detecção do DNA do HPV. Atualmente são utilizadas técnicas de hibridização como método de escolha para a detecção do DNA viral. Em muitos estudos a Reação em Cadeia da Polimerase (PCR) com a aplicação dos primers MY09 e MY11 demonstrou eficiência no rastreamento viral, consequentemente, o desenvolvimento desse diagnóstico molecular possibilitaria o monitoramento da doença, diminuindo as taxas de mortalidade causada pelo câncer de colo do útero. O sequenciamento de DNA é uma metodologia eficiente para a caracterização molecular dos tipos virais, permitindo a realização do alinhamento por similaridade das sequencias obtidas com outras já identificadas e depositadas no GenBank. O presente trabalho teve como propósito identificar os diferentes tipos de HPV e a presença de co-infecções, através de PCR e sequenciamento de uma região hipervariável do gene L1. A amostra estudada foi composta de 515 voluntárias das quais 111 (21,55%) apresentaram a presença do DNA do HPV. Entre os espécimes encontrados 50% são considerados de alto risco oncogênico (maior incidência dos tipos 16 e 58) e 7,21% possuíam infecção múltipla. A determinação das sequencias de base do gene L1 é fundamental para a identificação do tipo viral. Entretanto o sequenciamento do gene completo e em ambos os sentidos da cadeia de DNA se tornam inviáveis financeiramente para a maioria dos laboratórios especializados. Uma abordagem prática aplicada no estudo foi determinar a sequencia de uma região específica do gene L1 contendo 450pb, sendo possível a identificação do HPV seguindo essa metodologia. As técnicas utilizadas mostraram a necessidade da aplicação de um diagnóstico viral mais sensível e específico, contribuindo para o controle da infecção viral e para a diminuição da incidência e da mortalidade causadas pelo câncer cervical.

Human Papillomavirus (HPV)

L1 gene

Polymerase Chain Reaction (PCR)

DNA Sequencing

GenBank

Papilomavírus humano (HPV)

Gene L1

Reação em cadeia da polimerase (PCR)

Sequenciamento de DNA

GenBank

Análise molecular parcial dos genes VP1 e VP2 do vírus da doença infecciosa da bursa isolados no Brasil / Analysis on partial sequence of VP1 and VP2 genes of the Brazilian infectious bursal disease virus isolated in Brazil

Fernandes, Maria Judite Bittencourt

05 April 2010

Orientadores: Clarice Weis Arns, Isabela Cristina Simoni / Tese (doutorado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-16T00:22:52Z (GMT). No. of bitstreams: 1 Fernandes_MariaJuditeBittencourt_D.pdf: 1711625 bytes, checksum: d2876be51222b1ba7526b13ab7a72795 (MD5) Previous issue date: 2010 / Resumo: A doença infecciosa da bursa (IBD), denominada também doença de Gumboro, é uma doença aguda, imunossupressora, altamente contagiosa de aves jovens e de grande importância econômica para a avicultura. O vírus da doença infecciosa da bursa (IBDV), sorotipo 1, pode ser classificado de acordo com sua antigenicidade e patogenicidade em amostras clássicas virulentas (cv), atenuadas, variantes antigênicas ou muito virulentas (vv). Estas diferenças antigênicas são encontradas na região hipervariável do gene VP2, que é responsável pela indução de anticorpos neutralizantes e também dos possíveis marcadores de virulência que ainda não estão bem estabelecidos. O gene VP1 parece também apresentar um papel na virulência do vírus. Primeiramente, o objetivo do presente trabalho foi a identificação e caracterização molecular de 66 amostras brasileiras de IBDV através da RT-PCR de um fragmento do gene VP2 seguida pela digestão por enzimas de restrição (RE) e posterior confirmação pelo sequenciamento. A análise da RT-PCR/RE classificou 25 isolados como cepas vv e 16 como cepas cv além da classificação de 6 grupo moleculares. O sequenciamento também confirmou esta classificação com a presnça dos aminoácidos (aa) típicos das amostras vv (222A, 242I, 256I e 294I). Em 3 destes amostras vv também se observou mutações únicas que mostram pequenas, mas contínuas alterações dos vvIBDV circulantes nas granjas brasileiras. A arvore filogenética confirmou a origem comum das nossas amostras vv com os isolados de outros países assim como a origem monofilética destas amostras. Posteriormente foi feito a RT-PCR de um fragmento representativo do gene VP1 das amostras positivas para IBDV e a análise das sequências e filogenética. Quatorze amostras vv e três cv tiveram êxito nas sequências analisadas. Treze amostras vv apresentaram as substituições de aa comuns para as amostras vv (145T, 146D, 147N e 242E), exceto um que apresentou a sequência das amostras cv e na filogenia agrupou-se com estas amostras. A árvore a partir da VP1 pressupõe um rearranjo genético deste gene. Esta amostra com perfil do segmento A de amostra vv e do segmento B de cv seria o primeiro relato no Brasil de um rearranjo genético natural. Estes rearranjos de segmentos que também foram observados em amostras de outros países ou que podem ser produzidos em laboratório (quimeras) mostram que o segmento B pode estar contribuindo para a patogênese deste vírus. A origem destes rearranjos pode ser de troca genética com o uso de vacinas vivas ou se aceita a hipótese de que o segmento VP1 dos vvIBDV se originaram de um rearranjo genético de fonte desconhecida, estes rearranjos com segmento vvVP2 e cvVP1, seriam descendentes dos ancentrais dos vvVP1. Apenas um seqüenciamento completo das duas sequências e estudos in vivo poderão caracterizar o papel da VP1 na virulência desta amostra. Assim, o monitoramento contínuo das amostras de IBDV através da caracterização molecular pela análise das sequências dos genes e a detecção de alterações genéticas que possam influenciar a patogenicidade do vírus são de extrema importância, pois geram informações fundamentais que possibilitam e subsidiam o controle desta doença no Brasil / Abstract: Infectious bursal disease virus (IBDV) causes a disease among young chickens of great economic importance to the poultry industry worldwide both for the both mortality as the immunosuppression. Two distinct serotypes, 1 and 2, of IBDV are recognized. Only the serotype 1 is pathogenic for chickens and classified according to the antigenicity and/or pathogenicity in classical virulent (cv) strains, very virulent (vv) strains, antigenic variant strains, and attenuated strains. This classification has been based mainly on the VP2 gene sequence, more specifically on the hypervariable region corresponding to the induction of neutralizing antibodies and the serotype specificity. However, the fundamental molecular basis for pathogenicity is not yet clear. Studies with the VP1 gene have also shown its possible role in this virulence and pathogenicity. Firstly, the aim of the present paper was the molecular characterization of sixty-six Brazilian IBDV isolates from broiler and layers flocks during the period from 1997 to 2005 by RT-PCR followed by restriction enzyme analysis of a fragment from VP2 gene variable region. Sequence and phylogenetic analysis of the positive isolates were also carried out. Twenty-five of the isolates were identified as very virulent (vv) and sixteen as classic virulent (cv). All of vv isolates had the typical amino acid (aa) residues and clustered in a phylogenetic tree with the vvIBDV strains. Three vv isolates presented four common aa substitutions and differed from other vv strains indicating that the vvIBDVs circulating on Brazilian farms are undergoing slight but continuous exchanges. Furthermore, the Brazilian IBDV isolates characterized by the VP2 sequence in cv and vv strains were analyzed by the sequence and phylogeny of the VP1 gene fragment. Our vv isolates maintained clustered with the other vvIBDVs in phylogenetic tree obtained from the VP1 gene and presented the common aa too. The same occurred with the cv isolates. However, one isolate vv showed both characters, cv and vv into VP1 sequence and clustered with the ours and other cv isolates in the tree. This isolate has similar type of a reassortment / Doutorado / Microbiologia / Doutor em Genetica e Biologia Molecular

Vírus da doença infecciosa da bursa

Genes VP1

Genes VP2

Sequenciamento de DNA

Filogenia

Infectious bursal disease virus

VP1 gene

VP2 gene

DNA sequencing

Phylogeny

Análise exômica em pacientes portadores de cardiomiopatia hipertrófica / Exomic analysis in patients with cardiomyopathy hypertrophic

Lara Reinel de Castro

23 September 2015

A cardiomiopatia hipertrófica (CMH) é uma doença geneticamente determinada, caracterizada por hipertrofia ventricular primária, com prevalência estimada de 0.2% na população geral. Qualquer portador tem 50% de chance de transmitir esta doença para seus filhos, o que torna cada vez mais relevante a importância do estudo genético dos indivíduos acometidos e de seus familiares. Já foram descritas diversas mutações genéticas causadoras de CMH, a maioria em genes que codificam proteínas do sarcômero, e algumas mutações mais raras em genes não sarcoméricos. O objetivo desse estudo é sequenciar as regiões exônicas de genes candidatos, incluindo os principais envolvidos na hipertrofia miocárdica, utilizando o sequenciamento de nova geração (Generation Sequencing); testar a aplicabilidade e viabilidade deste sistema para identificar mutações já confirmadas e propor as prováveis novas mutações causadoras de CMH. Métodos e resultados: 66 pacientes não aparentados portadores de CMH foram estudados e submetidos à coleta de sangue para obtenção do DNA para analisar as regiões exômicas de 82 genes candidatos, utilizando a plataforma MiSeq (Illumina). Identificou-se 99 mutações provavelmente patogênicas em 54 pacientes incluídos no estudo (81,8%) relacionadas ou não a CMH, e distribuídas em 42 genes diferentes. Destas mutações 27 já haviam sido publicadas, sendo que 17 delas descritas como causadoras de CMH. Em 28 pacientes (42,4%) identificou-se mutação nos três principais genes sarcoméricos relacionados à CMH (MYH7, MYBPC3, TNNT2). Encontrou-se também um grande número de variantes não sonôminas de efeito clínico incerto e algumas mutações relacionadas a outras enfermidades. Conclusão: a análise da sequencia dos exônos de genes candidatos, demonstrou ser uma técnica promissora para o diagnóstico genético de CMH de forma mais rápida e sensível. A quantidade de dados gerados é o um fator limitante até o momento, principalmente em doenças geneticamente complexas com envolvimento de diversos genes e com sistema de bioinformática limitado. / Hypertrophic Cardiomyopathy (HCM) is a genetically determined disease, estimated prevalence of 0.2% in the general population. Any of its carriers has 50% likelihood to pass it on to their children, and that makes the genetic study of these individuals and their relatives even more relevant. There have been several studies describing genetic mutations that cause HCM - the vast majority in genes responsible for sarcomere protein coding - and other rarer mutations in non-sarcomeric genes. The aim of this research is study exonic areas of specific genes, including the most important ones related to myocardial hypertrophy, identifying the genetic mutations that have already been documented, and possible new pathogenic mutations, using the high throughput DNA sequencing (NGS); testing the pplicability and viability to identify HCM-causing mutations. Methods and results: 66 unrelated patients with CM were studied and subject to blood sample in order to extract their genomic DNA to analyze exomic regions of 82 candidates genes, using the high throughput sequencing technology on MiSeg (Illumina) platform. In this study we identified 99 possible damaging mutations in 54 patients (81.8%) that could be related or not to HCM, and distributed in 42 different genes. 27 of this variants have already been published, and 17 of them have been described as HCM causes. 42,4% of the patients (28 individuals) have genetic mutations in the three main sarcomeric genes related to HCM (MYH7, MYBPC3, TNNT2). We also identified a large number of non-synonymous variants of uncertain clinical significance and some mutations related to other diseases. Conclusion: The exome analysis in candidates genes using NGS has demonstrated to be promising for the genetic diagnosis of HCM, in a short time with sensivity. The amount of data obtained in a short period of time is the main limiting factor, especially for genetically complex diseases that involve multiple genes.

Análise de sequência de DNA

Cardiomiopatia hipertrófica

Exoma/genética

Genética médica

Mutação

sequenciamento de nova geração

DNA sequencing analysis

Exome/genetics

Genetic medicine

High throughput nucleotide sequencing

Hypertrophic cardiomyopathy

Mutation

Next generation sequencing

Genetic determinants and evolution of drug resistance in Mycobacterium tuberculosis in Vietnam : toward new diagnostic tools / Déterminants génétiques et évolution de la résistance aux médicaments chez Mycobacterium tuberculosis au Vietnam : vers de nouveaux outils de diagnostic

Nguyen, Quang Huy

20 December 2016

La tuberculose (TB), provoquée par Mycobacterium tuberculosis, est une des trois maladies prioritaires dans le monde. Les TB multi-résistantes (MDR) et ultra-résistantes (XDR-TB) représentent des obstacles majeurs pour la lutte antituberculeuse. Dans les pays à MDR-TB élevée, comme le Vietnam, la détection insuffisante de la résistance aux antibiotiques est un des facteurs principaux qui favorisent la transmission des souches résistantes. De plus, dans ces pays, encore très peu de choses sont connues sur la résistance à la pyrazinamide et aux antibiotiques de seconde ligne et sur les déterminants génétiques liés à ces résistances. Dans ce contexte, ce travail vise donc à acquérir des connaissances sur la résistance aux antibiotiques au Vietnam et à étudier comment M. tuberculosis évolue de l’état sensible à l’état ultra-résistant.260 isolats cliniques collectés au Vietnam entre 2005 et 2009 ont été inclus. Diverses techniques et analyses ont été utilisées: tests de sensibilité aux médicaments (développement d'un test à temps réduit), spoligotypage et MIRU-VNTR (24 loci) et séquençage de gènes. Les données ont été analysées par des analyses statistiques et phylogénétiques. Ce travail s’est d’abord focalisé sur la caractérisation d’isolats hautement résistants et sur la résistance à la pyrazinamide. Une forte proportion d'isolats quadruple résistants aux antibiotiques de première ligne a été identifiée comme pré-XDR et XDR et en majorité appartenant à la famille Beijing. L'analyse moléculaire a également révélé une forte proportion d'isolats, en particulier MDR, quadruple résistants et de la famille Beijing, portant des mutations associées à la résistance à la pyrazinamide.L'analyse génétique et phylogénétique globale a ensuite montré une grande diversité de profils de mutations dans chaque famille et chaque cluster MIRU-VNTR. Ces données suggèrent que M. tuberculosis peut suivre des chemins évolutifs variés pour devenir ultra-résistant. La prédominance de mutations et de combinaisons de mutations associées à un haut niveau de résistance et à un faible coût en termes de fitness suggère un effet cumulatif des mutations et un rôle de l’épistasie dans l'acquisition de la résistance multiple. De plus, une fréquence élevée de mutations compensatoires associées à la résistance à la rifampicine a été détectée chez les isolats très résistants. Ces processus semblent donc influencer fortement l'évolution de la résistance dans notre échantillon. Il est à noter que les mutations liées à des niveaux de résistance élevée et à de faibles coûts en termes de fitness, ainsi que les mutations compensatoires étaient plus particulièrement associées à la famille Beijing.En conclusion, ce travail fournit des connaissances uniques sur la résistance aux antibiotiques chez M. tuberculosis au Vietnam. En particulier, ces données prédisent une évolution de la résistance vers une situation de plus en plus préoccupante. Premièrement, la famille Beijing, en cours d’invasion au Vietnam, apparaît associée à de hauts niveaux de résistance, de faible coût en termes de fitness et aux mutations compensatoires. Deuxièmement, le risque élevé de résistance à la pyrazinamide remet en question son efficacité et son utilisation dans les traitements contre la MDR et la XDR-TB. Troisièmement, les données suggèrent une évolution de M. tuberculosis vers un potentiel de résistance plus élevé par effet cumulatif des mutations associés à la résistance et l’existence de phénomènes d’épistasie. Comme les échantillons étudiés dans ce travail ont été collectés, l’étape suivante est de valider nos hypothèses sur des données actualisées.Enfin, ce travail avec les données déjà publiées a permis d’établir, pour la première fois, un inventaire des mutations associées à la résistance aux antibiotiques chez M. tuberculosis au Vietnam. Cette base de données sera utilisée pour le développement d'une puce à ADN pour la détection rapide de la résistance aux antibiotiques au Vietnam. / Tuberculosis (TB) is one of the deadliest infectious diseases worldwide, mainly caused by Mycobacterium tuberculosis. Multidrug resistant (MDR) and extensively drug resistant (XDR) TB are currently main challenges for TB control. In high MDR-TB burden countries like Vietnam, one of the main factors of drug resistant strain spread is the insufficient capacity of drug resistance detection. Besides, still little is known in these countries about the resistance to second line and pyrazinamide drugs (key drugs in the MDR-TB treatment) and the genetic determinants linked to these resistances. In this context, this work aimed to acquire knowledge on drug resistance in Vietnam and to understand how M. tuberculosis evolved from sensitive to highly drug resistance form by molecular analysis.260 clinical isolates collected in Vietnam between 2005 and 2009 were included. Various techniques and analyses were used: drug susceptibility testing (development of a test with a reduced turn-around time), spoligotyping and 24-MIRU-VNTR typing and gene sequencing. The data were analyzed by statistical and phylogenetic analyses.First, this work was focused on highly drug resistant M. tuberculosis clinical isolates and pyrazinamide resistance. A high proportion of quadruple first-line drug resistant isolates (resistant to isoniazid, rifampicin, streptomycin and ethambutol) have been characterized as pre-XDR and XDR isolates, belonging especially to Beijing family. The molecular analysis revealed also high proportion of drug resistant isolates carrying highly confident pyrazinamide resistance-associated mutations, particularly in MDR and quadruple resistant isolates and in Beijing family.Second, the genetic and phylogenetic analyses showed high diversity of mutation patterns within each family and each MIRU-VNTR cluster suggesting various evolutionary trajectories towards first and second-line drug resistance. The predominance of specific mutations and combinations of mutations associated with high level of resistance and low fitness cost suggests a cumulative effect of mutations and a role for epistasis in multiple-drug resistance acquisition. In addition, high frequency of fitness-compensatory mutations associated with rifampicin resistant mutations was detected in highly drug resistant isolates. These processes may drive the evolution of drug resistance in this sample and lead to a successful spread of highly drug resistant strains. It is worth noting that Beijing family was specifically linked to high-level drug resistance and low fitness cost mutations and to compensatory mutations.In conclusion, this work provides knowledge on the resistance to the first and second-line anti-TB drugs in clinical M. tuberculosis samples collected in Vietnam between 2005 and 2009. These data predict an evolution towards a more problematic situation in terms of drug resistance. First, because the Beijing family, which is currently invading Vietnam, is associated with highly drug resistance, mutations linked to high-level drug resistance and low fitness cost and compensatory mutations. Second, the high risk of pyrazinamide resistance in our sample challenges the efficacy and the use of this drug in MDR-TB treatment. Third, our data suggest an evolution of M. tuberculosis towards a higher potential of drug resistance because of a probable cumulative effect of drug resistant mutations and epistatic interactions. Since the samples under study were collected between 2005-2009, the next step is to test our hypotheses on a recent sampling. Finally, this study together with published data allowed making, for the first time, an inventory of the drug resistance associated mutations in M. tuberculosis isolates from Vietnam.

Mycobacterium tuberculosis

Séquençage d'ADN et mutations

MDR et XDR tuberculose

Phylogénie et génotypage

Mycobacterium tuberculosis

DNA sequencing et mutation

Drug resistance evolution

MDR and XDR tuberculosis

Phylogeny et genotype

Phylogenetic Analysis of Subtribe Alopecurinae (Poaceae)

Boudko, Ekaterina

January 2014

Subtribe Alopecurinae (Poeae, Poaceae) sensu lato‘s seven genera share interesting morphological similarities (dense spicate panicles and one-flowered spikelets) that were widely thought to have a common origin. However, recent molecular evidence for three of the genera has suggested that the subtribe may be polyphyletic. To test this, five DNA regions were sequenced and analyzed using phylogenetic methods. Results confirm that Alopecurinae s.l. as presently treated is polyphyletic and should be dissolved. Additionally, the genus Cornucopiae may be just another Alopecurus. Limnas and Pseudophleum are not closely allied to Alopecurus or each other, and are even further from Phleum. Phleum is a distinct lineage that is not closely allied to any other included Alopecurinae genus. Evidence for revising infrageneric classifications of Alopecurus and Phleum is presented, as is evidence for separating A. magellanicus into two or more subspecies.

Poaceae

Alopecurinae

Poinae

Poeae

Phleinae

Pooideae

Phylogenetics

Phylogeny

Polyphyly

Molecular

Botany

Taxonomy

Systematics

Alopecurus

Phleum

Beckmannia

Limnas

Cornucopiae

Rhizocephalus

Pseudophleum

Plant

Grass

DNA sequencing

trnT-trnL-trnF

rpoB-trnC

matK

ITS

ETS

Convergent Evolution

Hybridization

Morphology

Evolution

Genetics

Flora

Subtribe

Efektivní hledání překryvů u NGS dat / Effective Search for Overlaps in NGS Data

Matocha, Petr

January 2017

The main theme of this work is the detection of overlaps in NGS data. The work contains an overview of NGS sequencing technologies that are the source of NGS data. In the thesis, the problem of overlapping detection is generally defined. Next, an overview of the available algorithms and approaches for detecting overlaps in NGS data is created. Principles of these algorithms are described herein. In the second part of this work a suitable tool for detecting approximate overlaps in NGS data is designed and its implementation is described herein. In conclusion, the experiments performed with this tool and the conclusions that follow are summarized and described.