Caracterização molecular e perfil de sensibilidade de Candida tropicalis isoladas em corrente sanguínea e cateter de pacientes internados em hospitais de ensino / Molecular characterization and susceptibility profile of Candida tropicalis isolated from bloodstream culture and catheter in nosocomial patients from teaching hospitals

Marcello Mihailenko Chaves Magri

28 November 2012

Infecções causadas por Candida tropicalis (C. tropicalis) são associados à elevada morbi-mortalidade, e foram consideradas como importantes causas de infecção de corrente sanguínea no Hospital das Clínicas da Faculdade de Medicina da Universidade de São Paulo (HCFMUSP) de março de 1998 a março de 2001. Adicionalmente, são responsáveis pelo aumento do tempo e dos custos de hospitalização e necessidade de cuidados intensivos. Esse estudo tem como objetivo a caracterização molecular e perfil de sensibilidade de 61 isolados de C. tropicalis a partir de candidemias no HCFMUSP e Universidade Estadual de Campinas (UNICAMP), através das técnicas de amplificação aleatória do DNA polimórfico (RAPD), eletroforese em campo pulsátil (PFGE), tipagem de sequências de múltiplos locus gênicos (MLST) e antifungigrama por microdiluição pelos métodos propostos, Clinical and Laboratory Standards Institute (CLSI) e European Committee on Antibiotic Susceptibility Testing (EUCAST). A análise filogenética por RAPD evidenciou que os iniciadores P1 e P2 mostraram maior capacidade de discriminação que P3. Na análise por PFGE com enzimas de restrição SfiI, SmaI, BssHII e NaeI, a enzima BssHII mostrou maior poder discriminatório. MLST contribuiu com 36 novas diploid sequence type (DSTs) e 23 novos alelos, de acordo com o banco de dados oficial do MLST (http://pubmlst.org/ctropicalis/), representando o primeiro estudo que caracterizaram isolados sequenciais na América do Sul. Entre os isolados sequenciais de um mesmo paciente, as microvariações foram mais frequentes no fragmento de gene XYR1 em 8 pacientes e macrovariações ocorreram em quatro pacientes com mais de um isolado, destacando-se três que apresentaram diferença nos seis alelos estudados. A análise comparativa entre os métodos evidenciou diferenças entre os isolados múltiplos dos pacientes 3, 7 e 11, considerados diferentes pelos três métodos. O poder discriminatório foi de 83,47% para RAPD, 82,18% para PFGE e 97,4 % para MLST. Os resultados do antifungigrana mostraram concordância entre os métodos CLSI e EUCAST de 73,8% para o fluconazol, 67,2% para o itraconazol e 80,3% para o voriconazol. Do total de 61 isolados estudados, 3 isolados de diferentes pacientes foram resistentes ao fluconazol, com MIC de 64 g/mL. O fenômeno de trailing foi observado em 50% das amostras testadas frente ao fluconazol, 23% ao voriconazol e 21,3% ao itraconazol. O uso de pH 5,0 para re-análise do CLSI frente ao fluconazol revelou-se como uma ferramenta útil para esclarecer o perfil de sensibilidade de isolados que apresentaram o fenômeno de trailing. Não houve correlação entre perfil genético gerado pelas técnicas de caracterização molecular estudadas e o perfil fenotípico através do teste de sensibilidade aos antifúngicos / Infections caused by Candida tropicalis (C. tropicalis) have been characterized as important causes of candidemia at the Hospital of the Medical school, University of São Paulo (HCFMUSP) from March 1998 to March 2001 and are associated with high morbidity and mortality. Additionally, they have been related to higher hospitalization costs because of longer hospitalization times and intensive care needs. This study aims to analyze the molecular typing and antifungal susceptibility profile of 61 isolates of C. tropicalis from 41 patients with candidemia in HCFMUSP and University of Campinas (UNICAMP), through Random Amplified Polymorphic DNA (RAPD), Pulsed Field Gel Electrophoresis (PFGE), Multilocus Sequence Typing (MLST) and broth microdilution antifungal susceptibility methodologies proposed by Clinical and Laboratory Standards Institute (CLSI) and European Committee on Antibiotic Susceptibility Testing (EUCAST). Phylogenetic analysis showed higher discriminatory power index of P1 and P2 primers than P3 by RAPD analysis. PFGE was performed with restriction enzymes SfiI, SmaI, NaeI and BssHII) and the enzyme BssHII presented the best performance. MLST analyses revealed 36 new diploid sequence type (DSTs) and 23 new alleles according to the C. tropicalis MLST database (http://pubmlst.org/ctropicalis/), representing the first study to characterize the sequential isolates of C. tropicalis candidemia in South America. Microvariation in a single gene was found in the sequential isolates from 8 patients. The main polymorphisms occurred in the alleles of the XYR1 gene. Macrovariation was detected in isolates from four patients, where 3 patients presented polimorphisms in six gene fragments. The comparative analysis revealed differences among sequential isolates from patients 3, 7 and 11, considered by three different methods. The discriminatory power was 83.47% for RAPD, 82.18% for PFGE and 97.4% for MLST. The agreement between the CLSI and EUCAST methods was 73.8% to fluconazole susceptibility, 67.2% to itraconazole and 80.3% to voriconazole. Of the 61 isolates tested, 3 isolates from different patients were resistant to fluconazole, MIC of 64 mg/mL. The trailing phenomenon was observed in 50% to fluconazole, 23% to voriconazole and 21.3% to itraconazole. Among the isolates studied, the use of pH 5.0 facilitated the determination of minimum inhibitory concentrations (MICs) for the re-analysis of fluconazole by CLSI, proving to be an important tool for the trailing phenomenon. No correlation was observed between genetic profile generated by the techniques of molecular characterization and phenotypic profile determined by susceptibility tests to antifungal drugs

Candida tropicalis

Farmacorresistência fúngica

Fungemia

Tipagem de sequências multilocus

Tipagem molecular

Candida tropicalis

Drug resistance fungal

Fungemia

Molecular typing

Multilocus sequence typing

Avaliação da variabilidade fenotípica e molecular de isolados de \'Candida albicans\' após período de armazenamento das culturas e em duas ocasiões de coleta / Evaluation of phenotypic and molecular variability of Candida albicans isolates after culture storage period and in two collection occasions

Bacelo, Kátia Leston

30 May 2008

O gênero Candida é responsável pela maioria das infecções fúngicas nosocomiais. A identificação do provável foco de origem é de extrema importância para elucidar a epidemiologia desse tipo de infecção e nesse sentido, a utilização de métodos de tipagem, que avaliam características fenotípicas e moleculares dos isolados, é essencial. Assim, o objetivo desse estudo foi tipar isolados de C. albicans, antes e após armazenamento e em diferentes ocasiões de coleta, a fim de verificar a manutenção dos biotipos apresentados, e o poder de discriminação dos métodos utilizados. Foi avaliada a microbiota leveduriforme da saliva de 73 estudantes universitários (tempo 0) sendo que após 180 dias (tempo 180) foi realizada nova coleta de saliva daqueles que apresentaram isolamento de C. albicans na primeira coleta. Os isolados foram analisados por ocasião das duas coletas, quanto à produção de exoenzimas fosfolipase e proteinase, pela morfologia das colônias, pelo perfil de suscetibilidade frente à anfotericina B, fluconazol e itraconazol e pela tipagem molecular por RAPD. As leveduras, após isoladas, foram armazenadas em ágar Sabouraud dextrose (ASD) e água destilada esterilizada. Após 180 dias, foram realizadas, novamente, as provas de tipagem. Todos isolados de C. albicans foram produtores de fosfolipase, nas duas coletas, embora tenha havido oscilação de atividade enzimática entre moderada e alta, no período. O enzimotipo prevalente nos tempos 0 e 180 foi, respectivamente, 22 e 32. Com relação à proteinase, 100% das leveduras apresentaram atividade moderada da enzima no tempo 0. No tempo 180 esse percentual foi de 85%, sendo que os demais não apresentaram atividade dessa enzima. Após armazenamento em ASD e água destilada, foi detectada alteração da atividade de ambas enzimas e conseqüente mudança de enzimotipos, em 40 e 30% dos isolados, respectivamente. Foram identificados 8 morfotipos diferentes de C.albicans no tempo 0 e apenas 50% foi mantido no tempo 180. O morfotipo mais comum foi 000-0. Após armazenamento, a maioria dos isolados apresentou alteração no morfotipo. Todos isolados mostraram-se sensíveis aos antifúngicos analisados nos tempos 0 e 180, denotando apenas um antifungotipo, o 111. Somente um isolado após estocagem em ASD, teve mudança de perfil de sensível para dose dependente ao itraconazol de modo que o antifungotipo foi alterado. A tipagem molecular por RAPD, com os primers OPA-09, OPB-11 e OPE-18, mostrou 19 tipos moleculares distintos entre os isolados obtidos na primeira coleta e permitiu identificar que um isolado de C.albicans obtido no tempo 180, não era relacionado ao obtido, do mesmo indivíduo, no tempo 0. Os demais mostraram perfil de fragmentos de DNA relacionado entre as coletas. Após estocagem, por ambos métodos, todos isolados mostraram correlação genética com o padrão obtido no tempo 0. Os resultados obtidos demonstram que os métodos de conservação aplicados neste estudo não permitem a manutenção da estabilidade das características fenotípicas avaliadas. Por outro lado, além da estabilidade dos biotipos gerados, a tipagem molecular por RAPD mostrou o melhor índice discriminatório, dentre as metodologias utilizadas, ratificando sua capacidade em diferenciar isolados, de uma mesma espécie e, portanto a sua utilidade em inquéritos epidemiológicos. / The Candida genus is responsible for most nosocomial fungal infections. The identification of the probable origin focus is very important to elucidate the epidemiology of this kind of infection and so, the usage of typing methods that evaluate phenotypic and molecular characteristics are essential. Therefore, the objective of this study was to type C. albicans isolates, before and after culture storage and in two different collection occasions to verify the biotype maintenance and the discriminatory power of the utilized methods. The salivary yeast microbiota of 73 university students (time 0) was evaluated and after 180 days (time 180) a new saliva collection of those that had presented C. albicans on the first collection was made. The isolates were analysed, in the two collection occasions on the basis of exoenzymes phospholipase and proteinase production, by colonial morphology, susceptibility profile to amphotericin B, fluconazole and itraconazole and according to molecular typing by RAPD. After isolation, the yeasts were storaged on Sabouraud dextrose agar (SDA) and in sterile distilled water. After 180 days, typing tests were carried out again. All C. albicans isolates were phospholipase productors, in both collections, even though enzyme activity had oscillated between moderate and high at that period. The prevalent enzymotype at time 0 and 180 were, respectively, 22 and 32. In relation to the proteinase, 100% of the yeasts showed moderate enzyme activity at time 0. At time 180, this percentage was 85%, and the others didn`t show enzyme activity. After storage on SDA and in distilled water, it was detected activity alteration of both enzymes and consequent enzymotype change, in 40 and 30% of isolates, respectively. Eight different C. albicans morphotypes were identified at time 0 and just 50% were maintained at time 180. The most common morphotype was 000-0. After storage most isolates presented changes in the morphotype. All isolates showed susceptibility to the analysed antifungals at times 0 and 180, showing just one antifungaltype, the 111. Only one isolate, after storage on SDA had a profile change from susceptible to dose dependent susceptible to itraconazole in a way that the antifungaltype wasn`t changed. The molecular typing by RAPD, with primers OPA-09, OPB-11 and OPE-18, showed 19 distinct molecular types among first collection isolates and allowed to identify that one C. albicans isolate from time 180 wasn`t related with the isolate obtained at time 0, from the same individual. The others showed DNA fragment profiles related between collection occasions. After storage by both methods, every isolate showed genetic relatedness with the profile obtained at time 0. The obtained results showed that the preservation methods used in this study don`t allow stability maintenance of the phenotypical characteristics evaluated. On the other hand, besides biotypes generated stability, the molecular typing by RAPD showed the best discriminatory index, between methodologies used, ratifying its ability in discriminating isolates of the same specie and so, its utility in epidemiological inquiries

antifungal susceptibility testing

antifungigrama

armazenamento

Candida albicans

Candida albicans

fosfolipase

molecular typing

phenotypic typing

phospholipase

proteinase

proteinase

RAPD

RAPD

storage

tipagem fenotípica

tipagem molecular

Molecular Genetic Insights into the Dimorphic Fungal Pathogen Blastomyces dermatitidis

Brown, Elizabeth Michelle Pallette

04 December 2012

The epidemiology of blastomycosis remains poorly understood in part due to the lack of a robust and discriminatory strain typing method for Blastomyces dermatitidis. Here we describe the development of a multilocus sequence (MLST) method to study the genetic variation and population structure of B. dermatitidis. Eighty geographically diverse clinical and environmental isolates were examined. Thirty-six unique sequence types were identified. With a discriminatory index of 91.4%, MLST identifies significant genetic diversity for the characterization of local and global B. dermatitidis isolates. To test whether this fungus represented a single species throughout its geographic range we performed phylogenetic analyses, applying Genealogical Concordance Phylogenetic Species Recognition (GCPSR). Phylogenetic analysis revealed two distinct clades, with five of the eight gene phylogenies studied supporting the separation of these lineages, which were also geographically partitioned. Based on fulfillment of GCPSR, we propose the current species B. dermatitidis harbors two genetically distinct non-interbreeding phylogenetic species.

Blastomyces dermatitidis

blastomycosis

multilocus sequence typing (MLST)

Phylogenetic Species Recognition (PSR)

strain typing

0410

0307

Molecular Genetic Insights into the Dimorphic Fungal Pathogen Blastomyces dermatitidis

Brown, Elizabeth Michelle Pallette

04 December 2012

The epidemiology of blastomycosis remains poorly understood in part due to the lack of a robust and discriminatory strain typing method for Blastomyces dermatitidis. Here we describe the development of a multilocus sequence (MLST) method to study the genetic variation and population structure of B. dermatitidis. Eighty geographically diverse clinical and environmental isolates were examined. Thirty-six unique sequence types were identified. With a discriminatory index of 91.4%, MLST identifies significant genetic diversity for the characterization of local and global B. dermatitidis isolates. To test whether this fungus represented a single species throughout its geographic range we performed phylogenetic analyses, applying Genealogical Concordance Phylogenetic Species Recognition (GCPSR). Phylogenetic analysis revealed two distinct clades, with five of the eight gene phylogenies studied supporting the separation of these lineages, which were also geographically partitioned. Based on fulfillment of GCPSR, we propose the current species B. dermatitidis harbors two genetically distinct non-interbreeding phylogenetic species.

Blastomyces dermatitidis

blastomycosis

multilocus sequence typing (MLST)

Phylogenetic Species Recognition (PSR)

strain typing

0410

0307

High Resolution Genotyping of Chlamydia trachomatis

Christerson, Linus

January 2011

Chlamydia trachomatis is an obligate intracellular bacterium of major human health concern, causing urogential chlamydia infections, lymphogranuloma venereum (LGV) and trachoma. Chlamydia is one of the most common sexually transmitted infections worldwide and can cause infertility. In the first four papers described herein we used a high resolution multilocus sequence typing (MLST) system to investigate the epidemiology of C. trachomatis, and showed that MLST is superior to conventional ompA genotyping with respect to resolution. In the fifth paper we simplified the methodology by developing and validating a multilocus typing (MLT) DNA microarray based on the MLST system. In more detail, MLST analysis of consecutive specimens from 2006 in Örebro County in Sweden, and comparison to specimens from 1999-2000, showed that the new variant C. trachomatis (nvCT) is monoclonal and likely has appeared in recent years. MLST analysis of LGV specimens from men who have sex with men (MSM) showed that the increase of LGV in Europe in the last decade indeed was a clonal outbreak, contrary to the USA where LGV might have been present all along. In the third paper, clinical symptoms could not be correlated with the MLST genotypes, suggesting, together with the combined results of all previous studies, that bacterial factors, if important, need to be understood in the context of host factors. MLST analysis of specimens from a high incidence C. trachomatis area in North Norway revealed interesting epidemiological details concerning unusual genetic variants, the nvCT and MSM, but found no significant difference in genetic diversity compared to two other geographic areas in Norway. Lastly, we developed a MLT array that provides high resolution while being rapid and cost-effective, which makes it an interesting alternative for C. trachomatis genotyping. In conclusion, the MLST system and the MLT array have proven to be useful tools and should now be applied in further investigations to improve our understanding of C. trachomatis epidemiology.

Clinical bacteriology

Klinisk bakteriologi

Caracterização fenotípica de Cepas de Staphylococcus aureus isoladas de queijos ricota

Pinto, Taiz Siqueira

25 March 2011

Made available in DSpace on 2015-04-17T15:03:08Z (GMT). No. of bitstreams: 1 arquivototal.pdf: 760407 bytes, checksum: 36ff52186c6a7e31beb2bd5ddc4a7fa0 (MD5) Previous issue date: 2011-03-25 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior - CAPES / This study aimed to isolate strains of Staphylococcus aureus in ricotta cheeses and to characterize them respecting phenotypic markers of lipolytic activity, and bacteriocin typing and resistance typing. For isolation, were acquired 11 samples of different brands of ricotta cheese sold in supermarkets in João Pessoa - Paraíba. Among the 41 strains, 82.9% proved positive lipase (Lip+) and 17.1%, negative lipase (Lip-). In relation to bacteriocin typing, 9.76% showed bacteriocin producing against a strain of Staphylococcus aureus isolated from surfaces processing food and 55% were susceptible to a strain of Staphylococcus aureus isolated from ricotta cheese. For resistance typing, 87.8% of strains were resistant to streptomycin, 26.59% to penicillin and 19.51% to erythromycin. None of the strains were resistant to tetracycline. Variability was observed between the minimal inhibitory concentrations (MIC), both in resistant strains as sensitive ones, so the variability showed more prevalent with penicillin (ranging from 0.015625 to 16 mg / mL) and the variability between strains of the same cheese. Only erythromycin-resistant strains were subjected to "D-test" to determine the type of resistance, of which all presented inductive resistant. From this results obtained, can conclude that although the phenotypes show an adaptive answer on related to the peculiarities of local environmental pressures, it is clear the importance of these genetic markers to discern new strains of S. aureus for those endemic, as well as to investigate possible epidemiological impacts and on food safety. / Este estudo teve como objetivo isolar cepas de Staphylococcus aureus de queijos ricota e caracterizá-las com relação a marcadores fenotípicos de atividade lipolítica, bacteriocinotipagem e resistotipagem. Para o isolamento, foram adquiridas 11 amostras de queijo ricota de diferentes marcas comercializadas em supermercados da cidade de João Pessoa-PB. Entre as 41 cepas isoladas, 82,9% revelaram-se lipase positiva (Lip+) e 17,1%, lipase negativa (Lip-). Com relação à bacteriocinotipagem, 9,76% mostraram-se produtoras de bacteriocinas frente a uma cepa de Staphylococcus aureus isolada de superfícies de processamento de alimentos e 55% mostraram-se sensíveis a uma cepa de Staphylococcus aureus isolada de queijo ricota. Para resistotipagem, 87,8% das cepas apresentaram-se resistentes a estreptomicina, 26,59% a penicilina e 19,51% a eritromicina. Nenhuma das cepas foi resistente a tetraciclina. Observou-se a variabilidade entre as Concentrações Inibitórias Mínimas, tanto em cepas resistentes como sensíveis, sendo tal variabilidade mais predominante com penicilina (variação de 0,015625 a 16 μg/mL), bem como a variabilidade entre cepas do mesmo queijo. Apenas cepas resistentes a eritromicina foram submetidas ao D-teste a fim de determinar o tipo de resistência, das quais todas as cepas mostraram-se com resistência indutiva. A partir dos resultados obtidos, pode-se concluir que embora os fenótipos revelem uma resposta adaptativa relacionada às peculiaridades das pressões ambientais locais, é evidente a importância destes marcadores genéticos a fim de se distinguir novas linhagens de S. aureus daquelas endêmicas, bem como investigar possíveis impactos epidemiológicos e na segurança alimentar.

Staphylococcus aureus

Fenotipagem

Atividade lipolítica

Bacteriocinotipagem

Resistotipagem

Ricota

Staphylococcus aureus

Phenotyping

Lipase activity

Bacteriocin typing

Resistance typing

Ricotta

CNPQ::CIENCIAS DA SAUDE::NUTRICAO

Avaliação da variabilidade fenotípica e molecular de isolados de \'Candida albicans\' após período de armazenamento das culturas e em duas ocasiões de coleta / Evaluation of phenotypic and molecular variability of Candida albicans isolates after culture storage period and in two collection occasions

Kátia Leston Bacelo

30 May 2008

O gênero Candida é responsável pela maioria das infecções fúngicas nosocomiais. A identificação do provável foco de origem é de extrema importância para elucidar a epidemiologia desse tipo de infecção e nesse sentido, a utilização de métodos de tipagem, que avaliam características fenotípicas e moleculares dos isolados, é essencial. Assim, o objetivo desse estudo foi tipar isolados de C. albicans, antes e após armazenamento e em diferentes ocasiões de coleta, a fim de verificar a manutenção dos biotipos apresentados, e o poder de discriminação dos métodos utilizados. Foi avaliada a microbiota leveduriforme da saliva de 73 estudantes universitários (tempo 0) sendo que após 180 dias (tempo 180) foi realizada nova coleta de saliva daqueles que apresentaram isolamento de C. albicans na primeira coleta. Os isolados foram analisados por ocasião das duas coletas, quanto à produção de exoenzimas fosfolipase e proteinase, pela morfologia das colônias, pelo perfil de suscetibilidade frente à anfotericina B, fluconazol e itraconazol e pela tipagem molecular por RAPD. As leveduras, após isoladas, foram armazenadas em ágar Sabouraud dextrose (ASD) e água destilada esterilizada. Após 180 dias, foram realizadas, novamente, as provas de tipagem. Todos isolados de C. albicans foram produtores de fosfolipase, nas duas coletas, embora tenha havido oscilação de atividade enzimática entre moderada e alta, no período. O enzimotipo prevalente nos tempos 0 e 180 foi, respectivamente, 22 e 32. Com relação à proteinase, 100% das leveduras apresentaram atividade moderada da enzima no tempo 0. No tempo 180 esse percentual foi de 85%, sendo que os demais não apresentaram atividade dessa enzima. Após armazenamento em ASD e água destilada, foi detectada alteração da atividade de ambas enzimas e conseqüente mudança de enzimotipos, em 40 e 30% dos isolados, respectivamente. Foram identificados 8 morfotipos diferentes de C.albicans no tempo 0 e apenas 50% foi mantido no tempo 180. O morfotipo mais comum foi 000-0. Após armazenamento, a maioria dos isolados apresentou alteração no morfotipo. Todos isolados mostraram-se sensíveis aos antifúngicos analisados nos tempos 0 e 180, denotando apenas um antifungotipo, o 111. Somente um isolado após estocagem em ASD, teve mudança de perfil de sensível para dose dependente ao itraconazol de modo que o antifungotipo foi alterado. A tipagem molecular por RAPD, com os primers OPA-09, OPB-11 e OPE-18, mostrou 19 tipos moleculares distintos entre os isolados obtidos na primeira coleta e permitiu identificar que um isolado de C.albicans obtido no tempo 180, não era relacionado ao obtido, do mesmo indivíduo, no tempo 0. Os demais mostraram perfil de fragmentos de DNA relacionado entre as coletas. Após estocagem, por ambos métodos, todos isolados mostraram correlação genética com o padrão obtido no tempo 0. Os resultados obtidos demonstram que os métodos de conservação aplicados neste estudo não permitem a manutenção da estabilidade das características fenotípicas avaliadas. Por outro lado, além da estabilidade dos biotipos gerados, a tipagem molecular por RAPD mostrou o melhor índice discriminatório, dentre as metodologias utilizadas, ratificando sua capacidade em diferenciar isolados, de uma mesma espécie e, portanto a sua utilidade em inquéritos epidemiológicos. / The Candida genus is responsible for most nosocomial fungal infections. The identification of the probable origin focus is very important to elucidate the epidemiology of this kind of infection and so, the usage of typing methods that evaluate phenotypic and molecular characteristics are essential. Therefore, the objective of this study was to type C. albicans isolates, before and after culture storage and in two different collection occasions to verify the biotype maintenance and the discriminatory power of the utilized methods. The salivary yeast microbiota of 73 university students (time 0) was evaluated and after 180 days (time 180) a new saliva collection of those that had presented C. albicans on the first collection was made. The isolates were analysed, in the two collection occasions on the basis of exoenzymes phospholipase and proteinase production, by colonial morphology, susceptibility profile to amphotericin B, fluconazole and itraconazole and according to molecular typing by RAPD. After isolation, the yeasts were storaged on Sabouraud dextrose agar (SDA) and in sterile distilled water. After 180 days, typing tests were carried out again. All C. albicans isolates were phospholipase productors, in both collections, even though enzyme activity had oscillated between moderate and high at that period. The prevalent enzymotype at time 0 and 180 were, respectively, 22 and 32. In relation to the proteinase, 100% of the yeasts showed moderate enzyme activity at time 0. At time 180, this percentage was 85%, and the others didn`t show enzyme activity. After storage on SDA and in distilled water, it was detected activity alteration of both enzymes and consequent enzymotype change, in 40 and 30% of isolates, respectively. Eight different C. albicans morphotypes were identified at time 0 and just 50% were maintained at time 180. The most common morphotype was 000-0. After storage most isolates presented changes in the morphotype. All isolates showed susceptibility to the analysed antifungals at times 0 and 180, showing just one antifungaltype, the 111. Only one isolate, after storage on SDA had a profile change from susceptible to dose dependent susceptible to itraconazole in a way that the antifungaltype wasn`t changed. The molecular typing by RAPD, with primers OPA-09, OPB-11 and OPE-18, showed 19 distinct molecular types among first collection isolates and allowed to identify that one C. albicans isolate from time 180 wasn`t related with the isolate obtained at time 0, from the same individual. The others showed DNA fragment profiles related between collection occasions. After storage by both methods, every isolate showed genetic relatedness with the profile obtained at time 0. The obtained results showed that the preservation methods used in this study don`t allow stability maintenance of the phenotypical characteristics evaluated. On the other hand, besides biotypes generated stability, the molecular typing by RAPD showed the best discriminatory index, between methodologies used, ratifying its ability in discriminating isolates of the same specie and so, its utility in epidemiological inquiries

antifungigrama

armazenamento

Candida albicans

fosfolipase

proteinase

RAPD

tipagem fenotípica

tipagem molecular

antifungal susceptibility testing

Candida albicans

molecular typing

phenotypic typing

phospholipase

proteinase

RAPD

storage

Online databáze sekvenčních a melt typů bakterií / Online Database of Bacterial Sequence and Melt Types

Františová, Zuzana

January 2020

Předmětem této diplomové práce je vytvoření databáze známých sekvenčních a melt typů patogenních bakterií a nástroje pro správu databáze. Metoda popisovaná v této práci je poměrně nová technika typizace patogenních bakterií založena na překladu sekvenčních typů na příslušející melt typ a využívá k tomu převodní klíč, který byl vytvořen ve spolupráci s Centrem molekulární biologie a genové terapie Interní hematologické a onkologické kliniky Fakultní nemocnice Brno. Obsahem práce je vytvoření prostoru na databázovém serveru, načtení potřebných dat, aplikace převodního klíče, vytvoření GUI, vytvoření dalších vhodných ošetření a rozšíření, testování a následná analýza výsledků. V první kapitole jsou diskutovány nejznámější metody bakteriální typizace, další kapitola je pak věnována server-client aplikacím a databázovým nástrojům. Třetí kapitola popisuje implementaci databáze na server a čtvrtá kapitola stručně shrnuje všechny funkce programu. V poslední kapitole je pak popsána analýza vylepšení převodního klíče, které získalo pracovní název půlené alely.

La recombinaison comme moteur de l’évolution des génomes : caractérisation de la conversion génique biaisée chez la souris / Recombination as a driver of genome evolution : characterisation of biased gene conversion in mice

Gautier, Maud

25 September 2019

Au cours de la méiose, les points chauds de recombinaison sont le siège de la formation de cassures double-brin de l’ADN. Ces dernières sont ensuite réparées par un processus qui, chez de nombreuses espèces, favorise la transmission des allèles G et C : la conversion génique biaisée vers GC (gBGC). L’intensité de cet important distorteur de la ségrégation méiotique varie fortement entre espèces mais les facteurs déterminant son évolution sont toujours inconnus. Nous avons donc voulu quantifier directement le biais de transmission chez la souris et comparer les paramètres dont il dépend avec d’autres mammifères. Dans cette étude, en couplant des développements bioinformatiques à une technique de capture ciblée d’ADN suivie de séquençage haut-débit (capture-seq), nous avons réussi à mettre au point une approche qui s’est révélée 100 fois plus performante pour détecter les événements de recombinaison que les méthodes existant actuellement. Ainsi, nous avons pu identifier 18 821 crossing-overs (COs) et non-crossovers (NCOs) à très grande résolution chez des individus uniques, ce qui nous a permis de caractériser minutieusement la recombinaison chez la souris. Chez cette espèce, les points chauds de recombinaison sont ciblés par la protéine PRDM9 et sont donc soumis à une deuxième forme de conversion génique biaisée (BGC) : le biais d’initiation (dBGC). La quantification du dBGC et du gBGC à partir de nos données nous a permis de mettre en lumière le fait que, au moment où des populations structurées s’hybrident, le gBGC des lignées parentales est propagé par un phénomène d’auto-stop génétique (genetic hitchhiking) provenant du dBGC. Nous avons ensuite pu observer que, chez les souris mâles, seuls les NCOs — et plus particulièrement les NCOs contenant un seul marqueur génétique— contribuent à l’intensité du gBGC. En comparaison, chez l’Homme, à la fois les NCOs et au moins une part des COs (ceux qui présentent des tracts de conversion complexes) distordent les fréquences alléliques. Ceci suggère que la machinerie de réparation des cassures double-brin qui induit le biais de conversion génique (BGC) présente des variations au sein des mammifères. Nos résultats sont aussi en accord avec l’hypothèse selon laquelle une pression de sélection limiterait l’intensité de ce processus délétère à l’échelle de la population. Cela se traduirait par une compensation de la taille efficace de population à de multiples niveaux : par le taux de recombinaison, par la longueur des tracts de conversion et par le biais de transmission. Somme toute, notre travail a permis de mieux comprendre la façon dont la recombinaison et la conversion génique biaisée opèrent chez les mammifères. / During meiosis, recombination hotspots host the formation of DNA double-strand breaks (DSBs). DSBs are subsequently repaired through a process which, in a wide range of species, is biased towards the favoured transmission of G and C alleles: GC-biased gene conversion (gBGC). The intensity of this fundamental distorter of meiotic segregation strongly varies between species but the factors dictating its evolution are not known. We thus aimed at directly quantifying the transmission bias in mice and comparing the parameters on which it depends with other mammals. Here, we coupled capture-seq and bioinformatic techniques to implement an approach that proved 100 times more powerful than current methods to detect recombination. With it, we identified 18,821 crossing-over (CO) and non-crossover (NCO) events at very high resolution in single individuals and could thus precisely characterise patterns of recombination in mice. In this species, recombination hotspots are targeted by PRDM9 and are therefore subject to a second type of biased gene conversion (BGC): DSB-induced BGC (dBGC). Quantifying both dBGC and gBGC with our data brought to light the fact that, in cases of structured populations, past gBGC from the parental lineages is hitchhiked by dBGC when the populations cross. We next observed that, in male mice, only NCOs — and more particularly single-marker NCOs — contribute to the intensity of gBGC. In contrast, in humans, both NCOs and at least a portion of COs (those with complex conversion tracts) distort allelic frequencies. This suggests that the DSB repair machinery leading to gBGC varies across mammals. Our findings are also consistent with the hypothesis of a selective pressure restraining the intensity of the deleterious gBGC process at the population-scale: this would materialise through a multi-level compensation of the effective population size by the recombination rate, the length of conversion tracts and the transmission bias. Altogether, our work has allowed to better comprehend how recombination and biased gene conversion proceed in the mammalian clade

Recombinaison

Conversion génique biaisée

PRDM9

Points chauds

Génomique

Évolution moléculaire

Mammifères

Sperm-typing

Recombination

Biased gene conversion

PRDM9

Hotspots

Genomics

Molecular evolution

Mammals

Sperm-typing

570

Relationship of Hand Size and Keyboard Size to Typing Performance Metrics

Gunawardena, Warnaka R.

January 2013

No description available.

Industrial Engineering

Information Technology

Improve Touch Screen Typing

Key size and Hand Size

Touch Screen Typing Speed and Accuracy

Table Top Touch Screen