Biologia reprodutiva de fêmeas de Astyanax fasciatus com números de cromossomos diferentes vivendo em ambiente natural e no cativeiro / Reproductive biology of Astyanax fasciatus females with different chromosome numbers living in natural environment and in captivity

Gabriela Brambila de Souza

02 February 2015

Ações antrópicas, como a construção de reservatórios, alteraram a migração de peixes que afeta a função normal do eixo hipotalamo-hipófise-gônadas. Para atenuar o impacto ambiental sobre a biota, existem programas de repovoamento com objetivo de reproduzir as espécies de peixes atingidas pelas barragens. Na piscicultura de Ponte Nova, na Bacia do Alto Tietê, o peixe migratório Astyanax fasciatus é rotineiramente produzido para o repovoamento com protocolos de reprodução artificial convencionais, mas o seu sucesso varia entre as fêmeas. Um estudo de citogenética detectou que o número de cromossomos foi diferente entre os reprodutores, uma característica comum em A. fasciatus. O objetivo do presente estudo foi estudar a fisiologia reprodutiva de Astyanax fasciatus com diferentes números de cromossomos, em ambiente natural (AN) e em cativeiro (Cat) e as possíveis alterações que possam explicar diferentes resultados de resposta à reprodução induzida em cativeiro. Fêmeas adultas de cada grupo experimental (G1-46 cromossomos; com baixa resposta à reprodução induzida; e G2 - 48 cromossomos; com boa resposta à reprodução induzida) foram coletadas em Cat e em AN ao longo de um ano. Amostras de sangue foram retiradas para análise plasmática de estradiol (E2), e os ovários para o cálculo da fecundidade relativa (FR), diâmetro oocitários, Índice Gonadossomático (IGS) e análises histológicas para identificação do estágio de maturação. As fêmeas do G1 nos dois ambientes iniciaram a fase vitelogênica do ciclo reprodutivo no inverno com o aumento da concentração de E2 plasmático. Nas fêmeas de AN, neste mesmo grupo, a maior porcentagem de oócitos vitelogênicos foi mantida nos ovários desde a primavera até o verão, período no qual a concentração de E2 continuou elevada no plasma. Por outro lado, no Cat, as concentrações de E2 não se mantiveram elevadas nas demais estações do ano, limitando-se apenas ao pico do inverno. Mesmo assim, as fêmeas confinadas mantiveram a FR significativamente mais elevada quando comparadas àquelas de AN, assim como maiores porcentagens de oócitos vitelogênicos, evidenciando a ausência de desova e lentidão no processo de reabsorção do vitelo. Já as fêmeas do G2, em AN iniciaram a fase vitelogênica do seu ciclo reprodutivo no outono, com o aumento progressivo dos níveis de E2 que atingiram seu pico na primavera, com a desova ocorrendo no verão. Por outro lado, a permanência no Cat, de alguma forma, alterou a sensibilidade às dicas ambientais do ciclo sazonal, e os níveis de E2 e a FR se mantiveram altos praticamente o ano todo. Estes dados sugerem que A. fasciatus com números diferentes de cromossomos têm padrões reprodutivos diferentes tanto em Cat como em AN e que em cativeiro fêmeas do G1 terão maior sucesso na indução quando manipuladas logo após o inverno, já fêmeas do G2 em Cat parecem ter sucesso na indução praticamente o ano todo / Anthropic actions, such as the construction of reservoirs, alter fish migration affecting the normal function of the brain-pituitary-gonads axis. To mitigate the environmental impact on the biota, fish restocking programs aim to reproduce fish species affected by dams. In the Ponte Nova Fish Farm, in the Upper Tietê River Basin, the migratory fish Astyanax fasciatus is routinely produced for restocking with a conventional artificial breeding protocol, but its success varies among the females. A cytogenetic study detected that the number of chromosomes was different among the broodstocks, a common feature in A. fasciatus. The purpose of this study was to study the reproductive physiology of Astyanax fasciatus with different numbers of chromosomes in a natural environment (AN) and captivity (Cat) and the possible changes that might explain different results in the success of induced reproduction in captivity. Adult females of each experimental group (G1-46 chromosomes; with low response to induced reproduction, and G2 - 48 chromosomes, with good response to induced reproduction) were collected in Cat and AN over one year. Blood samples were taken to analyze plasma estradiol (E2), and samples of ovaries to calculate the relative fecundity (FR), oocyte diameter, gonadosomatic index (GSI) and histological analyzes to identify the maturation stage. Females of G1, in both environments, started the vitellogenic phase of the reproductive cycle in the winter, with an increase in E2 levels. In the wild animals, the highest percentage of vitellogenic oocytes was maintained in the ovaries from spring to summer, a period in which E2 levels remained high. On the other hand, in captivity, a higher level of E2 was observed only in winter. Even so, the females in captivity maintained the fecundity significantly higher when compared with the wild ones, and also a higher percentage of vitellogenic oocytes, evidencing the absence of spawning and a delay in the yolk absorption. In G2, the vitellogenic stage of oocytes in wild females started in the fall, with a progressive increase in E2 levels, reaching its peak in spring, with the spawning in summer. On the other hand, remaining in the captivity, somehow altered the availability to the environmental tips of the seasonal cycle, and E2 levels as well as the FR virtually remained high throughout the year. These data suggest that A. fasciatus with different numbers of chromosomes have different reproductive patterns, both in a Cat and AN. G1 females could succeed in induced reproduction when handled immediately after winter, while G2 females seem to succeed the artificial reproductive induction throughout the year

Astyanax

Cativeiro

Estradiol

Fecundidade

Número de cromossomos

Reprodução

Astyanax

Captivity

Chromosome numbers

Estradiol

Fecundity

Reproduction

Caracterização fenotípica em indivíduos com microarranjos na região cromossômica 22q11 / Phenotypic characterization in individuals with microarrays in the 22q11 chromosomal region

Stéfany Lopes Lucas Empke

20 July 2015

Objetivo: Descrever as manifestações clínicas de indivíduos com hipótese diagnostica da Sindrome de deleção 22q11 (SD22q11) confirmados por testes genéticos, na primeira avaliação e durante o acompanhamento dos mesmos em avaliações subsequentes para uma melhor definição do curso natural da doença. Local: Laboratório de Genética e Citogenética Humana do HRAC-USP Bauru/SP. Casuística e metodologia: O presente trabalho é retrospectivo e analisou os dados de prontuários de 72 indivíduos cadastrados no HRAC-USP, os quais receberam hipótese diagnóstica da SD22q11 e foram confirmadas por teste genético (MLPA ou FISH). A avaliação envolveu a analise dos dados relatados por todos os setores do HRAC-USP. Resultados e discussão: Foramanalisados 72prontuários deindivíduos com a SD22q11. Constatamos que a idade media dos indivíduos quando do cadastro no HRAC-USP foi de seis anos. Também constatamos que houve um longo período de tempo entre os retornos ao hospital e que, nesses retornos, nem todas as especialidades foram contempladas. Esses fatos prejudicaram a analise da historia natural da anomalia em questão. Com relação às características fenotipicas, observamos a presença de sinais clínicos típicos, como por exemplo: face alongada, lábios finos, hipoplasia alar, anormalidades menores na orelha, dígitos longos e fendas palpebrais, fissuras labiopalatinas, cardiopatias congenitas, dificuldade de aprendizagem, atraso de linguagem e distúrbios comportamentais. A fissura oral foi à manifestação otorrinolaringológica mais frequente, presente em 75% dos pacientes, onde as fissuras submucosas foram as mais frequentes (43%). As características cognitivas como, atraso de fala (87%), dificuldades de aprendizagem (95%) e distúrbios comportamentais (81%), tiveram um resultado significativo, descritas em quase todos os indivíduos. As cardiopatias congênitas estavam presentes em 47,2% dos prontuários analisados. De um modo geral, comparando a frequência dos sinais clínicos encontrados neste trabalho com dados da literatura, constatamos que as frequências encontram-se dentro do esperado. Conclusão: A maioria dos indivíduos cadastrados no HRAC-USP, pertencentes ao grupo de estudo, apresentou idade superior a 06 anos. Portanto, a observação do curso natural da historia da SD22q11 para avaliar características fenotípicas que surgissem ao longo da evolução clinica do indivíduo e que pudessem ajudar no diagnóstico, ficou prejudicada. Mesmo nos casos onde o indivíduo foi cadastrado no HRAC-USP com idade inferior a dois anos, o diagnóstico foi tardio devido a falta de uma ação multidisciplinar e interdisciplinar no hospital. Mesmo não sendo possível avaliar as características fenotípicas surgidas durante a historia natural da doença, constatamos que as manifestações clínicas relatadas nos prontuários cursam com as características da SD22q11 e em frequências que corroboram com as da literatura / To describe clinical manifestations observed in medical records of individuals registered in the hospital with a diagnostic hypothesis of 22q11.2DS confirmed by genetic tests (MLPA OR FISH), since the first assessment in the HRAC-USP and during the follow up of these individuals in subsequent assessments, in order to achieve a better definition to the natural courses of the disease. Local: Laboratory of Human Genetics and Cytogenetics (HRAC-USP Bauru/SP). Methods: This retrospective study analyzed 72 medical records of individuals registered at the HRAC-USP, who were diagnosed with 22q11DS and who had this diagnosis confirmed by a genetic test (MLPA OR FISH). The assessment concerned the analysis of reported data in all sectors of the HRAC-USP. Results and Discussion: 72 medical records of individuals with 22q11DS were analyzed. It was verified that the average age of individuals when registering at the HRAC-USP was six years old. It was also verified that it took a long period of time for these individuals to return to the hospital and, when they did, not all specialties were contemplated. These facts harmed the analysis of the natural history of the anomaly. About the phenotypic characteristics, some typical clinical signs were observed, such as: long face, thin lips, hypoplasia nasal alar, minor abnormalities in the ear, long digits and narrow palpebral fissures, palatal abnormalities, congenital heart defects, learning disabilities, delay speech and behavioral disorders. An oral cleft was the most frequent otorhinolaryngology manifestation, present in 75% of the patients; among which submucous cleft palate were the most frequent (43%). Cognitive features such as, delay speech (87%), learning disabilities (95%) and behavioral disorders (81%) had a significant result, described in almost all individuals. Congenital heart defects were observed at 4% to 48% of individuals with 22q11.2DS, in this study it was observed in 47.2%. In general, comparing the frequency of some clinical signs observed in this study with the literature data, it was verified that the frequencies were within expectations. Conclusion: Most of the individuals registered at the HRAC belonging to the study group were over 6 years old. Therefore, the observation of natural course of the history of 22q11DS to evaluate the phenotypic characteristics that would arise during the clinical evolution of the individual and that could help in the diagnosis was harmed. Even in cases when the individual was registered at the HRAC-USPunder the age of two, the diagnosis was delayed due to lack of a multidisciplinary and interdisciplinary action in the hospital. Even not being possible to measure the phenotypic characteristics that emerged during the natural history of the disease, it was verified that the clinical manifestations reported in the records occur with the 22q11DS characteristics and in frequencies that corroborate with the literature

22q11

aberrações cromossômicas

deleção

síndrome Velocardiofacial

chromosome aberrations

deletion

velocardiofacial Syndrome

Início e manutenção da inativação do cromossomo X em células humanas / Establishment and maintenance of X-chromosome inactivation in human cells

Ana Maria Fraga

16 April 2012

Em fêmeas de mamíferos, um dos cromossomos X é inativado proporcionando compensação de dose entre os produtos gênicos de machos e fêmeas. A inativação do cromossomo X (ICX) ocorre no embrião em desenvolvimento, e se caracteriza pela aquisição de marcas heterocromáticas no cromossomo X inativado (Xi), que são mantidas nas células somáticas ao longo das divisões celulares. O melhor modelo para estudo do início da ICX são as células-tronco embrionárias femininas. Provenientes da massa celular interna de blastocistos, elas representam um embrião em desenvolvimento e possuem os dois X ativos; a diferenciação das células promove a ICX in vitro, o que permite a identificação dos fatores e mecanismos moleculares envolvidos. A derivação de linhagens de célulastronco embrionárias humanas (human embryonic stem cells - hESCs) em 1998 permitiu novas possibilidades de estudo da ICX, pois a maioria dos trabalhos procurou esclarecer o mecanismo da ICX no modelo murino. Tradicionalmente, a manutenção da ICX em humanos tem sido investigada em células somáticas híbridas ou transformadas; porém, sabe-se que estas não representam um contexto celular natural. Assim, o presente trabalho teve como objetivos principais explorar a potencialidade de hESCs no estudo do início da ICX, e ainda investigar a função de três fatores na manutenção da ICX em células humanas imortalizadas: DNMT1 (enzima responsável pela manutenção da metilação do DNA), SMCHD1 (proteína da família de coesinas/condensinas), e XIST (um RNA não-codificador que inicia o processo de heterocromatinização do futuro Xi) foram selecionados para este estudo, uma vez que todos participam da manutenção da ICX em camundongos. Até o momento foram derivadas em nosso laboratório quatro linhagens de hESCs, as primeiras da América Latina. A caracterização das linhagens mostrou que, apesar de se manterem indiferenciadas, as hESCs femininas encontram-se em estágio pós-ICX, pois mesmo indiferenciadas já apresentam um dos X inativado. Nossos dados indicam que, submetidas às atuais condições de cultivo, as hESCs não são bons modelos para o estudo do início da ICX, e é possível que a inativação de um cromossomo X durante o cultivo confira alguma vantagem seletiva às células. A estratégia utilizada no estudo da manutenção da ICX foi o silenciamento dos três genes por interferência de RNA (RNAi). Não foi possível diminuir significativamente a expressão dos genes XIST e SMCHD1. Porém, o silenciamento de DNMT1 foi expressivo, e em resposta foi observada reativação do gene MAOA, localizado no cromossomo X e submetido à inativação. Apesar de nossas análises mostrarem que os efeitos da diminuição de DNMT1 foram restritos ao gene MAOA, estes resultados sugerem a existência de diferentes hierarquias de controle epigenético dos genes submetidos à ICX em células humanas / In female mammals, one of the X chromosomes is inactivated to achieve dosage compensation between males and females. The X chromosome inactivation (XCI) occurs early during embryogenesis and is characterized by the acquisition of heterochromatic features on the inactive X (Xi), which are maintained during all the subsequent cell divisions. Embryonic stem cells are the most suitable cells to study the establishment of XCI. They are obtained from the inner cell mass (ICM) of blastocysts, and can represent a developing female embryo, possessing two active X-chromosomes; when differentiated, these cells recapitulate XCI in vitro, and thus one can identify XCI regulators and factors involved. The derivation of human embryonic stem cells (hESCs) in 1998 offered new possibilities to study XCI, since most of the mechanistic studies of XCI have so far been investigated in the mouse model system. Traditionally, maintenance of XCI in humans has been addressed in somatic cell hybrids or transformed cells; however, they do not represent a natural cellular context. The main goals of the present work were to verify the potential of hESCs as models of XCI, and also to study the function of three important factors in XCI maintenance in immortalized human cells. DNMT1 (DNA-methyltransferase 1), SMCHD1 (a cohesin/condensin protein family member) and the XIST gene (a non-coding RNA which triggers XCI and promotes X heterochromatin formation on the future Xi) were selected, as they are key factors in XCI maintenance in the mouse. Until now four hESCs lines were derived in our lab. Their characterization showed that, in spite of been undifferentiated, the female hESCs have already undergone XCI. Our data suggest that, under the actual culture conditions, hESCs are not good models to study XCI, and it is also possible that X inactivation confers selective advantage to hESCs. Knockdown by RNA interference was used to study the roles of three genes in XCI maintenance. We could not efficiently knockdown XIST or SMCHD1. However, the DNMT1 silencing was substantial, and led to the reactivation of MAOA, an X-linked gene subjected to XCI. Although the effect of DNMT1 silencing was restricted to MAOA, our data suggest that there are different epigenetic hierarchies to control the expression of the genes subjected to XCI in human cells.

Células-tronco embrionária humana

Epigenética

Inativação do cromossomo X

Epigenetic

Human embryonic stem cell

X-chromosome inactivation

Pesquisa de mutações no gene CDKN2A em pacientes com critérios clínicos de melanoma hereditário. / Search for mutations in the CDKN2A gene in patients with clinical pattern of hereditary melanoma.

Jair Huber

28 January 2004

A incidência do melanoma, tumor maligno que se origina dos melanócitos, vem crescendo em todo o mundo. História familial positiva da doença tem sido relatada em 8 a 14% dos pacientes afetados. Muitos estudos sugeriram o envolvimento da região 9p21, onde se encontra o gene CDKN2A, no surgimento dessa neoplasia. Este é um gene supressor tumoral clássico e a inativação dos dois alelos tem sido detectadas em linhagens celulares tumorais de famílias com melanoma hereditário e esporádico. Mutações em linhagens germinativas do gene CDKN2A têm sido identificadas em aproximadamente 20% das famílias com melanoma familial. Utilizando técnicas de biologia molecular como Reação em Cadeia da Polimerase (PCR), Conformação Estrutural de Fita Simples (SSCP) e seqüenciamento, este projeto estudou 22 pacientes com critérios clínicos de melanoma hereditário e encontrou uma mutação (P48T) em um paciente numa família de três afetados. Em 13 casos foi identificado pelo menos um dos três polimorfismos: 500 C>G (31,9%), 540 C>T (27,3%) e A148T (4,5%). Os resultados demonstram a importância da pesquisa de mutações no gene CDKN2A principalmente em famílias com dois ou mais membros afetados pela doença. / The incidence of melanoma, malign tumor that originates from melanocytes, is increasing all over the world. Positive familial history of disease has been related in 8 to 14% of affected patients. Several studies have suggest the 9p21 region evolvement, where is located the CDKN2A gene, in the arising of this neoplasia. It is a classic tumor suppressor gene and the inactivation of two alleles has been detected in tumor cells lines of families with hereditary and sporadic melanoma. Nowadays germeline mutations in CDKN2A gene have been identified in almost 20% of families with familial melanoma. Using molecular biology techniques like Polymerase Chain Reaction (PCR), Single Strand Conformational Polymorphism (SSCP) and sequencing, this project studied 22 patients with clinical pattern of hereditary melanoma and it found one mutation (P48T) in one patient belonged to a three affected family. Thirteen cases had at least one of the three polymorphisms: 500 C>G (31,9%), 540 C>T (27,3%) e A148T (4,5%). The results show the importance of the search for mutations in the CDKN2A gene mainly in families with two or more affected by disease.

CDKN2A

Cromossomo 9.

Melanoma hereditário

Neoplasia

PCR

SSCP

CDKN2A

Chromosome.

Hereditary melanoma

Neoplasia

PCR

SSCP

Estudo de freqüência alélica de cinco loci STR do cromossomo X na população do Estado de São Paulo e sua contribuição na identificação humana / Study of allelic frequency of five X-Chromosome?s loci STR on Sao Paulo State people and its role in human identification

Ricardo Henrique Alves da Silva

11 June 2007

A identificação forense através da análise de ácidos nucléicos é realizada, freqüentemente, pelo estudo de regiões polimórficas do DNA, tais como os STRs, regiões que apresentam repetições consecutivas curtas. Para a utilização destes marcadores na identificação humana é necessário conhecer a distribuição de seus alelos na população a qual o indivíduo pertence, visto que essa varia entre diferentes populações. Desta forma, o presente trabalho teve como objetivo determinar a freqüência alélica de cinco STRs do cromossomo X (DXS6854, DXS7424, DXS101, DXS6808 e DXS7132), a fim de avaliar a contribuição destes marcadores, através de cálculos estatísticos, na prática forense e em testes de paternidade. Foram coletadas amostras de esfregaço bucal, através de swab bucal, sendo depositado em cartão de coleta, e/ou sangue, através de punção digital depositada em cartão de coleta, em 243 sujeitos da pesquisa, sendo estes indivíduos não aparentados, residentes no Estado de São Paulo. A extração do DNA foi realizada a partir do Kit DNA IQ® (Promega), de acordo com as normas do fabricante e, na reação de PCR, utilizou-se um multiplex desenvolvido pela empresa BIOCOD (Belo Horizonte, MG), sendo a tipagem dos loci obtida através de corrida eletroforética, em gel de poliacrilamida desnaturante, no seqüenciador automático AlfExpress® (Amersham Biosciences). Os resultados foram analisados através dos programas PowerStats ver. 12 (Promega®) e Arlequin ver. 3.1. Como resultados principais foram observados: a grande variabilidade de alelos presentes na população estudada para os STRs selecionados; que o Poder de Discriminação em mulheres variou de 0,658 (DXS6808) a 0,975 (DXS101), assim como em homens entre 0,451 (DXS6808) e 0,881 (DXS101); as chances de exclusão foram calculadas em duas situações, par pai/filha (MECD) e trio pai/mãe/filha (MECT), sendo os melhores resultados apresentados pelo DXS101; além de verificar que a diversidade haplotípica (nas amostras masculinas) foi de 0,9993, indicando uma Probabilidade de Coincidência menor que 0,0007. Sendo assim, é possível concluir que, com exceção do DXS6808, os demais loci STR permitem uma boa aplicação na prática forense, permitindo sua utilização para cálculo estatístico em análises de identificação humana e testes de parentesco. / The forensic identification through DNA analysis is, frequently, done by the study of DNA?s polymorphic regions, such as STR, short tandem repeats. In order to use these markers in human identification, it?s necessary to know the allelic distribution in the population in wich the person belongs. This research aimed to settle the allelic frequencies of five X-chromosome?s STR (DXS6854, DXS7424, DXS101, DXS6808 e DXS7132) and analysis the contribution of these markers, through statistical parameters, in forensic activities and paternity tests. For this, samples of oral rub were collected by oral swab, being deposited on collect card, and/or blood by digital punction, deposited on collect card, with 243 research subject, being not related, living at Sao Paulo State, Brazil. The DNA extraction was performed using Kit DNA IQ® (Promega), according to manufacturer rules and, at PCR, was used a multiplex developed by BIOCOD (Belo Horizonte, Minas Gerais State), being the loci typifying obtained by eletrophoretical procedure, on polyacrilamid gel, using AlfExpress® (Amersham Biosciences). The results were statistically analyzed by PowerStats ver. 12 (Promega®) and Arlequin ver. 3.1 programs. The principal results showed: the great allele variability in this population sample to the selected STRs; that Power of Discrimination in women varied from 0.658 (DXS6808) to 0.975 (DXS101), as well as in men between 0.451 (DXS6808) and 0.881 (DXS101); the mean exclusion chance were calculated at two conditions, pair father/daughter (MECD) and trios involving daughters (MECT), being the best results performed by DXS101; and verify that haplotipical diversity (in men samples) was 0.9993, showing a Chance of Coincidence under 0.0007. In this way, it?s possible to conclude that, with exception of DXS6808, the other STRs loci studied can be used at forensic practice, using for statistical math in human identification and kinship testing.

Cromossomo X

DNA

Identificação humana

Odontologia Legal

DNA

Forensic Dentistry

Human identification

X-Chromosome

Estudo cromossômico da tribo Dalbergieae sensu Klitgaard & Lavin (2005) com ênfase no clado Dalbergia s. str. (Leguminosae, Papilionoideae) = Chromosome studies of the tribe Dalbergieae sensuKlitgaard & Lavin (2005) with emphasis on Dalbergia sensu strictoclade (Leguminosae, Papilionoideae) / Chromosome studies of the tribe Dalbergieae sensuKlitgaard & Lavin (2005) with emphasis on Dalbergia sensu strictoclade (Leguminosae, Papilionoideae)

Polido, Caroline do Amaral, 1983-

23 August 2018

Orientadores: Eliana Regina Forni Martins, Ana Paula de Moraes / Tese (doutorado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-23T11:58:38Z (GMT). No. of bitstreams: 1 Polido_CarolinedoAmaral_D.pdf: 4429006 bytes, checksum: a6c32402c33fb0d67c72b757af07b400 (MD5) Previous issue date: 2013 / Resumo: O resumo poderá ser visualizado no texto completo da tese digital quando for liberada / Abstract: The abstract is available with the full electronic document when available / Doutorado / Biologia Vegetal / Doutora em Biologia Vegetal

Citogenética

Fabaceae

Cromossomos - Classificação

Coloração cromossômica

Hibridização in situ

Cytogenetics

Fabaceae

Chromosomes - Classification

Chromosome painting

In situ hybridization

Genetically modelled Artificial Neural Networks for Optical Character Recognition : An evaluation of chromosome encodings

Lindqvist, Emil Gedda & Kalle

January 2011

Context. Custom solutions to optical character recognition problems are able to reach higher recognition rates then a generic solution by their ability to exploiting the limitations in the problem domain. Such solutions can be generated with genetic algorithms. This thesis evaluates two different chromosome encodings on an optical character recognition problem with a limited problem domain. Objectives. The main objective for this study is to compare two different chromosome encodings used in a genetic algorithm generating neural networks for an optical character recognition problem to evaluate both the impact on the evolution of the network as well as the networks produced. Methods. A systematic literature review was conducted to find genetic chromosome encodings previously used on similar problem. One well documented chromosome encoding was found. We implemented the found hromosome ncoding called binary, as well as a modified version called weighted binary, which intended to reduce the risk of bad mutations. Both chromosome encodings were evaluated on an optical character recognition problem with a limited problem domain. The experiment was run with two different population sizes, ten and fifty. A baseline for what to consider a good solution on the problem was acquired by implementing a template matching classifier on the same dataset. Template matching was chosen since it is used in existing solutions on the same problem. Results. Both encodings were able to reach good results compared to the baseline. The weighted binary encoding was able to reduce the problem with bad mutations which occurred in the binary encoding. However it also had a negative impact on the ability of finding the best networks. The weighted binary encoding was more prone to enbreeding with a small population than the binary encoding. The best network generated using the binary encoding had a 99.65% recognition rate while the best network generated by the weighted binary encoding had a 99.55% recognition rate. Conclusions. We conclude that it is possible to generate many good solutions for an optical character problem with a limited problem domain. Even though it is possible to reduce the risk of bad mutations in a genetic lgorithm generating neural networks used for optical character recognition by designing the chromosome encoding, it may be more harmful than not doing it.

chromosome encodings

genetic algorithms

optical character recognition

resilient propagation

Computer Sciences

Datavetenskap (datalogi)

Pathologies des hélicases et vieillissement précoce : modèle d'étude par dérivation de cellules souches pluripotentes induites (iPS) / Pathologies of helicases and premature aging : study by derivation of induced pluripotent stem cells

Gatinois, Vincent

27 November 2017

Les hélicases sont des enzymes ubiquitaires catalysant la séparation de l’ADN double-brin et impliquées dans la réplication, la réparation de l’ADN et dans le maintien des télomères. Chez l’Homme, 3 hélicases présentent des mutations responsables de syndromes cliniques : WRN pour le syndrome de Werner, BLM pour le syndrome de Bloom et RECQL4 pour le syndrome de Rothmund-Thomson. Tous ces syndromes associent un vieillissement pathologique accéléré à un risque accru de développement de cancer notamment par une augmentation de l’instabilité génomique. Les connaissances sur les mécanismes moléculaires et cellulaires impliqués dans ces maladies du vieillissement sont encore très partielles, notamment en ce qui concerne le lien entre l’instabilité génomique et le vieillissement. Au cours de ce projet, l'utilisation de prélèvements sanguins et cutanés de patients atteints de ces pathologies rares a permis de générer des modèles de cellules souches pluripotentes induites (iPS). Ces cellules présentent l’avantage de s’auto-renouveler et de pouvoir théoriquement se différencier dans tous les types cellulaires d’un organisme. Parallèlement, un témoin de sénescence a été généré de la même manière avec des cellules d’un patient souffrant du syndrome de la progéria de Hutchinson-Gilford. Après caractérisation de ces cellules, nous avons identifié des ensembles de phénotypes cellulaires et moléculaires dans le but de récapituler in vitro les pathologies. Nous avons également engagé les cellules iPS dans des voies de différenciation proches des tissus atteints dans les pathologies in vivo. Enfin, nous avons étudié la stabilité génomique de ces lignées dans les différents types cellulaires cultivés. Ainsi nous avons observé que la lignée Bloom est le siège de recombinaisons particulièrement fréquentes et est caractérisée par une instabilité du génome dans tous les types cellulaires étudiés. Egalement, la lignée Werner semblerait se distinguer par une instabilité de ses télomères. Enfin, l’ensemble des lignées des pathologies du vieillissement prématuré présenterait un défaut mitochondrial. / Helicases process the double-stranded DNA dissociation. They are involved in replication, DNA repair and maintenance of telomeres. In human, 3 helicases display mutations responsible for clinical syndromes: WRN for the Werner syndrome, BLM for the Bloom syndrome and RECQL4 for the Rothmund-Thomson syndrome. All these diseases cause premature ageing and high risk of cancer. Molecular and cellular mechanisms involved in these diseases are not well defined. Particularly, little is known concerning the link between genomic instability and ageing. During this project, we used blood samples and skin biopsies of affected patients to generate models by reprogramming cells to induced pluripotent stem cells (iPSCs). These cells have the advantage of self-renewing and theoretically could be differentiated in all cell types. At the same time, an iPSC senescence control was performed from cells of a Hutchinson-Gilford Progeria syndrome patient. iPSCs were characterized for pluripotency. In the aim of recapitulate these pathologies in vitro, we identified sets of cellular and molecular phenotypes. We also engaged differentiation of iPSCs in cell pathways closed to the affected tissues in vivo. Finally, we studied the genomic stability of iPSCs and derived cells. We observed that Bloom cells are susceptible to frequent recombinations and are characterized by a genome instability through all studied cell types. Werner cells showed an instability of telomeres length. Finally, all premature ageing diseases displayed mitochondrial defects.

Ips

Cellules souches

Hélicase

Instabilité chromosomique

Télomère

Ipsc

Stem Cells

Helicase

Chromosome instability

Telomere

Investigating Tissue factor gene regulation using the Chromosome Conformation Capture (3C) technique

Palisetty, Hari vanaja

January 2011

No description available.

Tissue factor

blood coagulation

gene regulation

Chromosome Conformation Capture

3C

Cell and Molecular Biology

Cell- och molekylärbiologi

Rôles et régulations de Polo et BubR1 sur les cassures double-­‐brin de l'ADN en mitose / Roles and regulations of Polo and BubR1 on DNA-­‐ double-­‐strand breaks during mitosis

Landmann, Cedric

15 December 2017

La présence de cassures double-brin de l'ADN en mitose est problématique pour les cellules, car cette situation produit des fragments de chromosome ne possédant pas de centromères. En l'absence d'un mécanisme permettant leur prise en charge, ces fragments acentriques n'étant pas attachés au fuseau mitotique, pourraient être ségrégés aléatoirement dans les cellules filles, causant de l'instabilité génomique. Nous avons découvert un mécanisme permettant la transmission correcte des fragments acentriques dans les cellules filles via une structure faisant le lien entre les deux fragments cassés. Plusieurs protéines sont recrutées sur les cassures, comme les kinases mitotiques BubR1 et Polo, et favorisent la ségrégation correcte de ces chromosomes cassés. Cependant, les mécanismes permettant le recrutement de BubR1 et Polo sur les cassures d'ADN en mitose sont inconnus. De plus, les mécanismes moléculaires par lesquels BubR1 et Polo favorisent la ségrégation correcte des fragments acentriques restent à être identifiés. La première partie de mon projet a été d'étudier le rôle et la régulation de BubR1 sur les cassures d'ADN pendant la mitose. Nous avons montré que BubR1 requiert Bub3 pour se localiser sur les chromosomes cassés afin de favoriser leur ségrégation correcte. Nous avons également détecté l'accumulation de FizzyCDC20, un cofacteur de l'E3 ubiquitine ligase APC/C (Anaphase-Promoting- Complex/Cyclosome), sur les cassures d'ADN, et son recrutement dépend de son interaction avec la KEN Box de BubR1. De plus, l'utilisation d'un substrat synthétique de l'APC/C nous a permis de démontrer que la dégradation par l'APC/C est inhibée localement autour du chromosome cassé, de manière dépendante de BubR1. Ces résultats suggèrent fortement que le complexe BubR1/Bub3 recrut é sur les cassures d'ADN inhibe localement l'APC/C en séquestrant FizzyCDC20 et empêche ainsi la dégradation de substrats clefs impliqués dans la ségrégation correcte des chromosomes cassés. La seconde partie de mon projet a été d'étudier les relations d'interdépendance entre Polo et BubR1/Bub3/Fizzy sur les cassures d'ADN en mitose. Nous avons utilisé un laser UV pulsé pour induire des cassures dans un chromosome à un instant précis pendant la mitose, puis nous avons suivi le recrutement de protéines tagguées GFP sur les cassures de chromosome. Cette étude révèle que Polo est rapidement recrutée sur les cassures d'ADN et précède BubR1, Bub3 et Fizzy. De plus, la disparition de BubR1, Bub3 et Fizzy des cassures d'ADN coïncide avec la télophase alors que Polo disparait des cassures pendant l'interphase. Nous avons également montré que le recrutement de BubR1, Bub3 et Fizzy sur les cassures d'ADN est retardé dans les mutants polo, indiquant que Polo est requis pour un recrutement efficace de BubR1, Bub3 et Fizzy sur les cassures d'ADN. Pour finir, nous avons montré que l'accumulation de Polo et BubR1/Bub3/Fizzy sur les cassures d'ADN dépend de deux composants de la réponse aux dommages à l'ADN, le complexe MRN (Mre11-Rad50-Nbs1) et ATM (ataxia-telangiectasia mutated). Ce travail a permis d'avoir une meilleure compréhension sur la dynamique de recrutement de Polo et BubR1/Bub3/Fizzy sur les cassures d'ADN en mitose. De plus, le mécanisme moléculaire par lequel le complexe BubR1/Bub3 agit pour faciliter la ségrégation des chromosomes cassés a pu être en partie élucidé. / The presence of DNA double strand breaks (DSB) during mitosis is challenging for the cell, as it produces fragments of chromosome lacking a centromere. If not processed, this situation can cause genomic instability resulting in improper segregation of the broken fragments into daughter cells. We uncovered a mechanism by which broken chromosomes are faithfully transmitted to daughter cells via the tethering of the two broken chromosome ends. Several proteins including the mitotic kinase BubR1 and Polo are recruited to the breaks and mediate the proper segregation of the broken fragments. However, the mechanism underlying Polo and BubR1 recruitment to DNA breaks is unknown. Moreover, the molecular mechanisms by which Polo and BubR1 mediate the proper segregation of the broken fragments remain to be elucidated. We first investigated the role and regulation of BubR1 on DNA breaks during mitosis. We show that BubR1 requires Bub3 to localize on the broken chromosome fragment and to mediate its proper segregation. We also find that FizzyCdc20, a co--‐factor of the E3 ubiquitin ligase Anaphase--‐Promoting--‐Complex/Cyclosome (APC/C), accumulates on DNA breaks in a BubR1 KEN box--‐dependent manner. A biosensor for APC/C activity demonstrates a BubR1--‐dependent local inhibition of APC/C around the segregating broken chromosome. These results are consistent with a model where Bub3/BubR1 complex on DNA breaks functions to inhibit the APC/C locally via the sequestration of FizzyCdc20, thus preserving key substrates from degradation, which promotes proper transmission of broken chromosomes. In a second study, we investigated the dependency relationship between Polo and BubR1/Bub3/Fizzy on DNA breaks in mitosis. We used a pulsed UV laser to break one chromosome at a define time during mitosis. We immediately follow the recruitment of GFP--‐tagged proteins to laser--‐induced DNA breaks. My study reveals that Polo is promptly recruited to DNA breaks and precedes BubR1, Bub3 and Fizzy. In addition, while BubR1, Bub3 and Fizzy dissociation from the breaks coincide with telophase and the nuclear envelope reformation, Polo remains on the breaks well into interphase. We further show that the appearance of BubR1, Bub3 and Fizzy on DNA breaks is delayed in polo mutant, indicating that Polo is required for the robust and efficient recruitment of BubR1, Bub3 and Fizzy to DNA breaks. Finally, the timely accumulation of Polo, BubR1 and Bub3 to DNA breaks depends on two components of the DNA Damage Response, the MRN complex (Mre11--‐Rad50--‐Nbs1) and ATM (ataxia--‐telangiectasia mutated). This work gives us a better understanding on how Polo and BubR1, Bub3 and FizzyCdc20 are recruited to DNA breaks in mitosis and how they promote broken chromosomes segregation.

BubR1

Chromosomes cassés

Drosophile

Mitose

Ségrégation des chromosomes

Polo

BubR1

Broken chromosomes

Drosophila

Mitosis

Chromosome seggregation

Polo