Generation of a human gene index and its application to disease candidacy.

Christoffels, Alan

January 2001

<p>With easy access to technology to generate expressed sequence tags (ESTs), several groups have sequenced from thousands to several thousands of ESTs. These ESTs benefit from consolidation and organization to deliver significant biological value. A number of EST projects are underway to extract maximum value from fragmented EST resources by constructing gene indices, where all transcripts are partitioned into index classes such that transcripts are put into the same index class if they represent the same gene. Therefore a gene index should ideally represent a non-redundant set of transcripts. Indeed, most gene indices aim to reconstruct the gene complement of a genome and their technological developments are directed at achieving this goal. The South African National Bioinformatics Institute (SANBI), on the other hand, embarked on the development of the sequence alignment and consensus knowledgebase (STACK) database that focused on the detection and visualisation of transcript variation in the context of developmental and pathological states, using all publicly available ESTs. Preliminary work on the STACK project employed an approach of partitioning the EST data into arbitrarily chosen tissue categories as a means of reducing the EST sequences to manageable sizes for subsequent processing. The tissue partitioning provided the template material for developing error-checking tools to analyse the information embedded in the error-laden EST sequences. However, tissue partitioning increases redundancy in the sequence data because one gene can be expressed in multiple tissues, with the result that multiple tissue partitioned transcripts will correspond to the same gene.</p> <p><br /> Therefore, the sequence data represented by each tissue category had to be merged in order to obtain a comprehensive view of expressed transcript variation across all available tissues. The need to consolidate all EST information provided the impetus for developing a STACK human gene index, also referred to as a whole-body index. In this dissertation, I report on the development of a STACK human gene index represented by consensus transcripts where all constituent ESTs sample single or multiple tissues in order to provide the correct development and pathological context for investigating sequence variation. Furthermore, the availability of a human gene index is assessed as a diseasecandidate gene discovery resource. A feasible approach to construction of a whole-body index required the ability to process error-prone EST data in excess of one million sequences (1,198,607 ESTs as of December 1998). In the absence of new clustering algorithms, at that time, we successfully ported D2_CLUSTER, an EST clustering algorithm, to the high performance shared multiprocessor machine, Origin2000. Improvements to the parallelised version of D2_CLUSTER included: (i) ability to cluster sequences on as many as 126 processors. For example, 462000 ESTs were clustered in 31 hours on 126 R10000 MHz processors, Origin2000. (ii) enhanced memory management that allowed for clustering of mRNA sequences as long as 83000 base pairs. (iii) ability to have the input sequence data accessible to all processors, allowing rapid access to the sequences. (iv) a restart module that allowed a job to be restarted if it was interrupted. The successful enhancements to the parallelised version of D2_CLUSTER, as listed above, allowed for the processing of EST datasets in excess of 1 million sequences. An hierarchical approach was adopted where 1,198,607 million ESTs from GenBank release 110 (October 1998) were partitioned into &quot / tissue bins&quot / and each tissue bin was processed through a pipeline that included masking for contaminants, clustering, assembly, assembly analysis and consensus generation. A total of 478,707 consensus transcripts were generated for all the tissue categories and these sequences served as the input data for the generation of the wholebody index sequences. The clustering of all tissue-derived consensus transcripts was followed by the collapse of each consensus sequence to its individual ESTs prior to assembly and whole-body index consensus sequence generation. The hierarchical approach demonstrated a consolidation of the input EST data from 1,198607 ESTs to 69,158 multi-sequence clusters and 162,439 singletons (or individual ESTs). Chromosomal locations were added to 25,793 whole-body index sequences through assignment of genetic markers such as radiation hybrid markers and g&eacute / n&eacute / thon markers. The whole-body index sequences were made available to the research community through a sequence-based search engine (http://ziggy.sanbi.ac.za/~alan/researchINDEX.html).</p>

Human genetics

Human genome

Human gene mapping

DNA

Human chromosomes

Human gene libraries

Gene libraries.

Understanding the mechanisms underlying DSB repair-induced mutagenesis at distant loci in yeast

Saini, Natalie

22 May 2014

Increased mutagenesis is a hallmark of cancers. On the other hand, this can trigger the generation of polymorphisms and lead to evolution. Lately, it has become clear that one of the major sources of increased mutation rates in the genome is chromosomal break formation and repair. A variety of factors can contribute to the generation of breaks in the genome. A paradoxical source of breaks is the sequence composition of the genomic DNA itself. Eukaryotic and prokaryotic genomes contain sequence motifs capable of adopting secondary structures often found to be potent inducers of double strand breaks culminating into rearrangements. These regions are therefore termed fragile sequence motifs. Here, we demonstrate that in addition to being responsible for triggering chromosomal rearrangements, inverted repeats and GAA/TTC repeats are also potent sources of mutagenesis. Repeat-induced mutagenesis extends up to 8 kb on either side of the break point. Remarkably, error-prone repair of the break by Polζ reconstitutes the repeats making them a long term source of mutagenesis. Despite its negative connotations for genome stability, the mechanisms underlying the unstable nature of double strand break repair pathways are not known. Previous studies have demonstrated that break induced replication (BIR), a mechanism employed to repair broken chromosomes with only one repairable end, is highly mutagenic, undergoes frequent template switching and often yields half-crossovers. In the work presented here, we show that the instabilities inherent to BIR can be attributed to its unusual mode of synthesis. We determined that BIR proceeds via a migrating bubble with long stretches of single-stranded DNA and culminates with conservative inheritance of the newly synthesized DNA. We propose that the mechanisms described here might be important for generation of repair-associated mutagenesis in higher organisms. Secondary structure forming repeats like inverted repeats have been found to be enriched in cancer cells. These motifs often constitute chromosomal rearrangement hot-spots and demonstrate the phenomenon of kataegis. This study provides a mechanistic insight into how such breakage-prone motifs contribute to hypermutability of cancer genomes.

Mutagenesis

Yeast

Chromosomes

Régulation dynamique de l’association des cohésines aux chromosomes, établissement et maintien de la cohésion des chromatides sœurs / Dynamic regulation of cohesin association with chromosomes, sister chromatid cohesion establishment and maintenance

Feytout, Amélie

09 December 2010

Le complexe cohésine maintient associées les chromatides sœurs depuis la réplication jusqu’à leur ségrégation en mitose. Une question majeure est de comprendre comment la cohésion est établie lors de la phase S. Chez les mammifères et S. pombe, les cohésines sont associées de manière labile aux chromosomes pré-réplicatifs et l’établissement de la cohésion en phase S s’accompagne de la stabilisation de l’association des cohésines aux chromosomes. L’objectif de ce travail est de comprendre comment la dynamique des cohésines est régulée et comment son inhibition créée la cohésion.En G1 les cohésines associées aux chromosomes s’échangent avec le pool soluble et leur dissociation dépend de Pds5 et Wapl. La première partie de ce travail présente les résultats d’un crible génétique visant à identifier de nouveaux régulateurs de la dynamique des cohésines.L’établissement de la cohésion nécessite l’acétyltransférase Eso1 mais pas en contexte Δwpl1, indiquant que la seule mais essentielle fonction d’Eso1 est de s’opposer à celle de Wapl. L’acétylation de Smc3 par Eso1 contribue mais n’est pas suffisante pour contrecarrer Wapl, suggérant l’existence d’un autre événement dépendant d’Eso1. En G1, Pds5 agit avec Wapl pour dissocier les cohésines des chromosomes mais après la phase S, Pds5 est requise pour leur maintien sur les chromosomes et pour la cohésion à long terme. Pds5 co-localise avec la fraction stable de cohésines mais pas Wapl. Nous suggérons un modèle dans lequel la cohésion est créée par deux événements d’acétylation couplés à la progression de la fourche de réplication conduisant à l’éviction de Wapl des cohésines destinées à produire la cohésion. / Following DNA replication, sister chromatids are connected by cohesin to ensure their correct segregation during mitosis. How cohesion is created is still enigmatic. The cohesin subunit Smc3 becomes acetylated by ECO1, a conserved acetyl-transferase, and this change is required for cohesion. As in mammals, fission yeast cohesin is not stably bound to G1 chromosomes but a fraction becomes stable when cohesion is made. The aim of this work was to understand how cohesin dynamics is regulated and how the change in cohesin dynamics creates cohesion.In G1 chromatin bound cohesin exchange with the soluble pool and the unloading reaction relies in part on Wapl. The first part of this study reports on the identification of G1/S factors as new candidate regulators of cohesin dynamics.Following S phase a stable cohesin fraction is made. The acetyl-transferase Eso1 is not required for this reaction when the wpl1 gene is deleted. Yet, it is in wild-type cells, showing that the sole but essential Eso1 function is counteracting Wapl. Eso1 acetylates the cohesin sub-unit Smc3. This renders cohesin less sensitive to Wapl but does not confer the stable binding mode, suggesting the existence of a second Eso1-dependent event. The cohesin sub-unit Pds5 act together with Wapl to promote cohesin removal from G1 chromosomes but after S phase Pds5 is essential for cohesin retention on chromosomes and long term cohesion. Pds5 co-localizes with the stable cohesin fraction whereas Wapl does not. We suggest a model in which cohesion establishment is made by two acetylation events coupled to fork progression leading to Wapl eviction while keeping Pds5 on cohesin complexes intended to make cohesion.

Ségrégation des chromosomes

Cohésion des chromatides sœurs

Cohésines

Schizosaccharomyces pombe

Chromosome segregation

Sister chromatid cohesion

Cohesin

Schizosaccharomyces pombe

Evoluce velikosti genomu v rodě Globba (Zingiberaceae) / Genome size evolution in tropical tribe Globba (Zingiberaceae)

Pospíšilová, Monika

January 2012

The variability of the genome size reaches several grades even within relatively close groups of plants. The study of the genome size in the phylogenetic context provides interesting results which characterize the evolution of the individual groups of plants. In this respect, tropical plants have yet not been studied. Tropical genus Globba (ca. 100 species) belongs to an economically significant family Zingiberaceae. The diversity centre is found in Thailand but it spreads from east India and southern China up to Indonesia and the Philippines. It is a polyploid complex which exists in two cytotypes within one genus (2n = 32 a 2n = 48); it is characteristic minimally in three out of seven distinguished sections. The aim of this thesis has been a reconstruction of the group phylogeny, discovering the role of the polyploid and evaluation of the genome size evolution of the Globba genus in the phylogenetic context. To this end, modern biosystematic methods were used (flow cytometry, chromosome counting, sequencing of the nuclear and chloroplast DNA regions). Many types of software and statistical methods were used to process and interpret the data. In this group, the genome size was measured for the first time. Out of 87 individuals, the smallest size was measured with Globba nuda (2C = 1.11 pg). The...

Evoluce vybraných karyotypových znaků u tetrapulmonátních pavoukovců / Evolution of selected karyotype characters in tetrapulmonate arachnids

Jílková, Klára

January 2013

The class Arachnida is not thoroughly explored from the cytogenetic point of view. Previous studies suggest a high diversity of karyotypes and sex determination in arachnids. This study deals with the evolution of sex chomosomes, nucleolar organizer regions (NOR), and telomeric repeats in the tetrapulmonate clade of arachnids, particularly in groups of ancient origin. Sex chromosomes were detected in two orders. Detection of NORs in a large set of species supports the hypothesis that the ancestral karyotype of arachnids contained NOR on one pair of autosomes only. The number of NORs has increased during the evolution of some groups of Pedipalpi. The NORs are located in terminal or subterminal chromosomal regions in most tetrapulmonates. The occurrence of the "insect" telomeric motif was confirmed in majority of tetrapulmonates. Interstitital telomeric repeats were not detected with the exception of one species. Keywords: arachnids, meiosis, sex chromosomes, telomeres, nucleolar organizer, heterochromatin

Estudos cromossômicos e moleculares em Rhamdia (Pisces, Siluriformes, Heptapteridae): análise de relações evolutivas / Cromossomic and molecular studies in Rhamdia (Pisces, Siluriformes, Heptapteridae): a relationship overview

Garcia, Caroline

15 September 2009

O gênero Rhamdia, popularmente conhecido como jundiá, pertence à família Heptapteridae, uma das maiores radiações de bagres neotropicais de água doce. Estes peixes de médio porte e hábitos oportunistas e noturnos são encontrados em pequenos rios e córregos. No passado, Rhamdia foi considerado um dos gêneros mais especiosos dentro de Siluriformes, contando com cerca de 100 espécies descritas. Entretanto, após uma revisão taxonômica recente o número de espécies desse gênero foi reduzido a 12. Dados genéticos, de natureza cromossômica e molecular, caracterizam o gênero Rhamdia como um grupo que apresenta grande diversidade, sugerindo a existência de complexos de espécies, principalmente para a espécie R. quelen, a única estudada do ponto de vista citogenético até o momento. No presente trabalho, foram utilizadas diferentes metodologias com o intuito de caracterizar cromossomicamente populações de diferentes espécies de Rhamdia, bem como estabelecer as relações evolutivas entre elas, contribuindo para o reconhecimento de padrões e processos evolutivos envolvidos em sua diferenciação. Foram analisados exemplares de R. enfurnada, R. itacaiunas, R. laukidi e R. quelen, provenientes das principais bacias hidrográficas da América do Sul, sendo somadas as análises sequências de genes mitocondriais de R. cinerascens, R. guatemalensis e R. laticauda provenientes do GenBank, totalizando sete das 12 espécies reconhecidas para o gênero. A análise de cinco regiões do genoma mitocondrial identificou a existência de 15 grupos bem definidos e com altos valores de suporte para o que hoje é reconhecido como R. quelen, confirmando a existência de um complexo de espécies. A divisão das espécies de Rhamdia em um grupo Cis-Andino e um grupo Trans-Andino, proposta anteriormente, também foi recuperada, embora o gênero não tenha sido confirmado como monofilético. Os dados citogenéticos permitiram o estabelecimento de tendências de evolução cromossômica dentro do grupo e a sugestão de um possível mecanismo de origem e diferenciação dos cromossomos supranumerários. O presente trabalho reforça a importância da utilização de diferentes abordagens na realização de estudos taxonômicos e evolutivos, sugerindo uma nova revisão do gênero Rhamdia que leve em consideração os dados genéticos obtidos. / The genus Rhamdia, popularly known as jundia, belongs to the family Heptapteridae, one of the greatest radiations within neotropical freshwater catfish. This group of middle-sized fish of opportunistic behavior is found in small rivers and streams. In the past, Rhamdia was considered one of the most specious genera of Siluriformes, comprising about 100 described species. However, after a recent taxonomic review, the number of species within this genus was reduced to 12. Genetic data, whether chromosomal or molecular, have characterized the genus Rhamdia as a high diverse group, suggesting the existence of species complexes, mainly in R. quelen, the only species where cytogenetic data are available so far. In the present work, different methodologies were used in order to characterize cytogenetically populations of distinct species of Rhamdia, as well as their evolutionary relationships, thus contributing to the recognition of evolutionary patterns and processes involved in their differentiation. Specimens of R. enfurnada, R. itacaiunas, R. laukidi and R. quelen, from the main South-American hydrographic basins were analyzed, coupled with sequence analyses of the mitochondrial genes of R. cinerascens, R. guatemalensis and R. laticauda, available in the GenBank, thereby comprising seven of the 12 valid species in the genus. The analysis of five regions of mitochondrial genome identified 15 well-defined groups with high bootstrap values within the so-called R. quelen, confirming the occurrence of a species complex. The division of Rhamdia species into a Cis-Andean group and a Trans- Andean group, as previously proposed, was also revalidated, although the genus seems not to be monophyletic. The cytogenetic data allowed establishing trends of chromosomal evolution within the group and a hypothesis for the origin and differentiation of supernumerary chromosomes could be drawn. The present work reinforces the importance of distinct approaches in taxonomic and evolutionary studies, suggesting a new revision within the genus Rhamdia that takes the present genetic data into account.

Rhamdia

Rhamdia

Citogenética

Cromossomos supranumerários

Cytogenetics

DNA

Filogenia

Mithocondrial DNA

Phylogeny

Supernumerary chromosomes

Identificação, caracterização e estudo da expressão dos genes hsc70 e hsp83 em Rhynchosciara americana / Identification, characterization and study of expression of the genes hsc70 and hsp83 in Rhynchosciara americana

Andrade, Alexandre de

19 August 2005

Com a idéia de identificar proteínas envolvidas no processo de enovelamento das proteínas sintetizadas na glândula salivar de Rhynchosciara americana, no início deste projeto adotou-se como estratégia o seqüenciamento de uma biblioteca de cDNA. Esta biblioteca foi construída utilizando-se glândulas salivares de Rhynchosciara americana do período de seu desenvolvimento onde tem início a síntese de seu casulo. Mensagens de proteínas envolvidas no processo de enovelamento, transporte e proteólise foram isoladas, alguns exemplos são hsc70, hsp83, hip, hop, dnaJ, trap1 e prolil isomerase, sec61&#945;/&#946;, sec23, peptidase de sinal, rab7, partícula reconhecedora de sinal (srp), enzima conjugadora de ubiquitina e complexo regulatório proteassomo 26, cop 1 e ubiquitina ligase. A identificação destes genes permitiu o isolamento de clones genômicos através de triagem em banco de fagos e caracterização dos genes hsc70 e hsp83 para verificação de sua organização em Rhynchosciara americana. A expressão dos seus respectivos mRNAs foi avaliada em vários períodos do último estágio larval. A localização por hibridização in situ mostrou que estes genes estão localizados em regiões dos cromossomos politênicos próximas a dois pufes de DNA, C3 e C8. O estudo dos níveis de expressão das proteínas codificadas pelos genes hsc70 e hsp83 mostrou a diferença de comportamento destes genes sob condições de estresse térmico e que a expressão destas proteínas deve ser regulada pelo período de desenvolvimento das larvas de Rhynchosciara americana. Quando evidenciada por imunofluorescência a proteína Hsc70 mostra localização predominantemente no citoplasma. / With the idea of identify some of these proteins involved in the folding process of the proteins synthesized on the Rhynchosciara salivary gland, this project started adopting the shotgun cDNA sequencing strategy. This cDNA library was constructed utilizing salivary glands of Rhynchosciara americana at a developmental period where the cocoon construction begins. Messengers of important proteins involved in the folding, transport and proteolysis process were isolated, some examples are hsc70, hsp83, hip, hop, sec61 &#945;/&#946;, sec23, signal peptidase, rab7, signal recognition particle (srp), ubiquitin conjugating enzyme e 26 proteasome regulatory complex, cop 1 and ubiquitin ligase. Identification of these genes allowed the screening of genomic clones from a phage library; hsc70 and hsp83 characterization was carried out to verify the arrangement of these genes on genome of Rhynchosciara americana. The study of these genes will contribute with phylogenetic information about the specie. The mRNA expression of these genes was analyzed during several periods of the last larval developmental stage. In situ localization showed that these genes are located in polytene chromosomes regions near two DNAs puffs, C3 and C8. The expression levels of the proteins codified by genes hsc70 and hsp83 showed different behaviors of these genes under heat stress conditions and mainly, that the regulation of the proteins Hsc70 and Hsp83 can be related to the period of development of the larvae of Rhynchosciara americana. When revealed by immunofluorescence, Hsc70 protein shows localization predominantly on the cytoplasm.

Cromossomos politênicos

DNA puffs

Hsc70

Hsc70

Hsp83

Hsp83

Polytene chromosomes

Puffs de DNA

Rhynchosciara americana

Rhynchosciara americana

Organização genômica de sequências repetitivas em Pica-paus (aves piciformes)

Oliveira, Thays Duarte de

05 April 2017

Submitted by Ana Damasceno (ana.damasceno@unipampa.edu.br) on 2017-06-01T21:04:14Z No. of bitstreams: 2 license_rdf: 1232 bytes, checksum: 66e71c371cc565284e70f40736c94386 (MD5) Organização genômica de sequências repetitivas em Pica-paus (aves piciformes).pdf: 2128434 bytes, checksum: 8afa26cc3c248da9e51696791e1dadc1 (MD5) / Made available in DSpace on 2017-06-01T21:04:15Z (GMT). No. of bitstreams: 2 license_rdf: 1232 bytes, checksum: 66e71c371cc565284e70f40736c94386 (MD5) Organização genômica de sequências repetitivas em Pica-paus (aves piciformes).pdf: 2128434 bytes, checksum: 8afa26cc3c248da9e51696791e1dadc1 (MD5) Previous issue date: 2017-04-05 / A caracterização da quantidade e distribuição da fração de DNA repetitivo em genomas auxilia no entendimento de sua organização cromossômica. As Aves são conhecidas por apresentar uma baixa proporção de DNA repetitivo quando comparada a outras classes de Vertebrados. Entretanto, a ordem Piciformes se destaca por apresentar uma quantidade percentual superior dessas sequências comparado com as outras aves. Com isso, o objetivo deste estudo foi determinar a distribuição de diferentes tipos de sequências repetitivas no genoma de três espécies da família Picidae, Colaptes melanochloros (2n=84), Colaptes campestris (2n=84) e Melanerpes candidus (2n=64), por meio de hibridização in situ fluorescente (FISH) com sondas de rDNA 18S, teloméricas (TTAGGG)n e microssatélites. Os resultados mostraram, nessas três espécies, o cromossomo sexual Z como o maior do complemento, esse fato deve-se ao acúmulo de diferentes sequências de microssatélites. Entretanto o cromossomo W de C. Melanochloros, que é totalmente heterocromático, não apresentou acúmulo destas sequências. Os sítios ribossomais estão organizados em um par de cromossomos com uma constrição secundária e este teve o acúmulo da sequência (CGG)10 nas três espécies. As sondas teloméricas apresentaram marcações nas regiões terminais dos cromossomos e marcações intersticiais em alguns macrocromossomos. As marcações intersticiais indicam fusões entre cromossomos ou acúmulo de sequências repetitivas similares as teloméricas. Com as sondas de microssatélites identificou-se o mesmo padrão de hibridização nas espécies de Colaptes e padrão distinto entre Colaptes e M. candidus. As nossas análises de FISH mostraram várias sequências de microssatélites amplificadas no cromossomo Z nas três espécies analisadas, o que pode explicar o fato deste ser o maior elemento do cariótipo e desta família conter maior quantidade de sequências repetitivas comparadas com outros grupos de aves. Curiosamente, nenhuma das sequências foi encontrada acumulada no cromoss omo W, apesar de desempenharem um papel importante na diferenciação de cromossomos sexuais. Estes resultados evidenciam que, apesar da origem comum proposta para o sistema sexual ZW em aves, esses cromossomos seguiram diferentes trajetórias evolutivas em cada espécie, indicando uma alta plasticidade para a diferenciação cromossômica sexual neste grupo. Este trabalho é o primeiro passo para esclarecer o papel das sequências satélites e microssatélites na diferenciação de cromossomos sexuais. / The characterization of the amount and distribution of the repetitive DNA fractions in genomes assists in the understanding of their chromosomal organization. The Birds are characterized by presenting a low proportion of repetitive DNA when compared to other classes of Vertebrates. However, the order Piciformes stands out for having a higher percentage of these sequences compared to other birds. The objective of this study was to determine the distribution of different types of repetitive sequences in the genome of three species of the family Picidae, Colaptes melanochloros (2n = 84), Colaptes campestris (2n = 84) and Melanerpes candidus (2n = 64) by fluorescence in situ hybridization (FISH) with 18S, telomeric (TTAGGG) and microsatellite rDNA probes. The results showed, in these three species, the sexual chromosome Z as the largest of the complement, this fact is due to the accumulation of different sequences of microsatellites. However, the W chromosome of C. melanochloros, which is totally heterochromatic, did not show accumulation of these sequences. The ribosomal sites are organized on a pair of chromosomes with a secondary constriction and this had the accumulation of the sequence (CGG)10 in the three species. The telomeric probes showed markings in the terminal regions of the chromosomes and interstitial markings on some macrochromosomes. Interstitial markings indicate fusions between chromosomes or the accumulation of repetitive sequences similar to the telomeric ones. With the microsatellite probes the same pattern of hybridization was identified in the Colaptes species, distinct pattern between Colaptes and M. candidus. Our FISH analyzes showed several amplified microsatellite sequences on the Z chromosome in the three species analyzed, which may explain the fact that this is the largest element of the karyotype and that its genome contains the largest number of repetitive sequences compared to other groups of Birds. Interestingly, none of the sequences were found to be accumulated on the W chromosome, although they play an important role in the differentiation of sex chromosomes. These results show that, despite the common origin proposed for the ZW sexual system in birds, these chromosomes followed different evolutionary trajectories in each species, indicating a high plasticity for the sexual chromosome differentiation in this group. This work is the first step to clarify the role of satellites and microsatellite sequences in the differentiation of sex chromosomes.

Birds

Sex chromosomes

Telomerase

Aves

Cromossomos sexuais

Microssatélites

Telomérica

rDNA

Aves

Cromossomos sexuais

Telômero

DNA

Sequencias de DNA da estrutura cromossômica terminal de dípteros da família Sciaridae / DNA sequences at terminal chromosome structure of Sciaridae flies

Fernandes, Thiago

11 May 2012

A Ordem Diptera é constituída de milhares de espécies, cujo tempo de divergência pode chegar a 250 milhões de anos entre representantes das Sub-Ordens Brachycera e Nematocera. Esta janela temporal, no entanto, não é suficiente para explicar o aparecimento de estruturas cromossômicas terminais alternativas aos telômeros canônicos, conservados desde eucariontes unicelulares até mamíferos. Alguns autores admitem que estruturas não canônicas tenham sido geradas e selecionadas a partir de eventos mutacionais que resultaram na perda da telomerase em espécies ancestrais. Especulações deste tipo, embora pertinentes, não levam em conta que o número de espécies de dípteros estudados até aqui quanto a telômeros e sub-telômeros está longe de representar a diversidade na Ordem. Como evidência negativa não constitui prova, a possível existência de dípteros dotados de telômeros canônicos não pode ser descartada. Também neste sentido, a possível ocorrência de retrotransposons especificamente terminais, como vistos em Drosophila, em espécies ainda não estudadas pode ser vista como possibilidade em aberto apesar da evidência negativa documentada no presente trabalho em R. Americana e em T. pubescens. Outra idéia que tem ganhado corpo com dados procedentes de telômeros não canônicos refere-se à possibilidade de que um organismo apresente mais de uma sequência de DNA terminal. Pouco comentada, esta noção teve início em meados da década de 1980 quando foram publicados os primeiros trabalhos sobre o DNA telomérico de espécies da família Chironomidae. O aparecimento destes dados na literatura praticamente coincidiu com a publicação da descoberta da telomerase. Mais tarde, estudos em Drosophila têm mostrado que três retrotransposons com sequências diferentes podem compor o DNA telomérico nesta espécie. Além disto, repetições aparentemente terminais em Anopheles hibridam em um único telômero, sugerindo que sequências desconhecidas estejam presentes em outros telômeros. Dados obtidos neste trabalho mostram em R. Americana uma nova repetição em tandem que apresenta características de sequência telomérica, a exemplo de duas outras caracterizadas com antecedência nesta espécie. Assim, R. Americana poderia ser vista como exemplo adicional de organismo dotado de mais de uma sequência de DNA terminal. No final da presente exploração, não foi possível a identificação de sequências comuns às extremidades cromossômicas de T. pubescens. Os resultados obtidos sugerem que esta espécie apresenta uma estrutura cromossômica terminal distinta se comparada àquelas de dípteros estudados até então. Uma das hipóteses levantadas a partir dos resultados observados é a de que sequências teloméricas estão presentes em todas as extremidades cromossômicas de T. pubescens; o problema estaria na impossibilidade de visualizá-las através de hibridação in situ em função do comprimento do DNA telomérico que estaria abaixo do limite da técnica de detecção. Isto implicaria deixar de lado os métodos usualmente empregados pelo laboratório na busca de DNA repetitivo terminal. Caso esta espécie apresentasse repetições terminais curtas como aquelas caracterizadas em R. Americana, uma das alternativas seria a de sequênciar massivamente clones obtidos por microdissecção e DOP-PCR até encontrarmos sequências com estas características. Em seguida, o ensaio com Bal-31 seria decisivo na determinação da posição cromossômica das mesmas. Finalmente, os dados sintetizados nos três capítulos deste trabalho reforçam a afirmação de que a Ordem Diptera é uma fornte privilegiada de diversidade quanto a estruturas cromossômicas terminais. Apesar das dificuldades inerentes à exploração de organismos não modelares, a continuidade dos estudos sobre telômeros e sub-telômeros nestas espécies certamente ampliará o conhecimento sobre alternativas de manutenção da integridade cromossômica a partir de suas extremidades / The vast majority of eukaryotic organisms have short tandem repeats and telomerase as components of telomeric structures. However, in dipteran species, this structural conservation is not found. While in Drosophila telomeres are composed of specific retrotransposons, complex tandem repeats are found in the genus Anopheles and in species of Chironomus. In Rhynchosciara americana (family Sciaridae), short repetitions (16 and 22 base pairs) arranged in tandem are observed at chromosome terminal regions. Moreover, in situ hybridization using RNA probes suggests that a third repetition enriched with homopolymeric (dA)/(dT) could occupy significant portions of this chromosomal region in R. americana. In addition, a retroelement named \"RaTART\" was described at chromosomal ends of R. americana; this element enables telomeric maintenance by retrotransposon action in basal dipterans. In this thesis, we present results that rule out the possibility that the \"RaTART\" element occupies the chromosome terminal structure in R. americana. Additional analyses were performed with the sequence RaTART from GenBank and primers designed for the amplification of significant portions of the regions 5&prime;UTR, 3&prime;UTR, and the coding region for reverse transcriptase (RT) of this retroelement. The sequencing and in situ hybridization of these three fragments obtained after PCR (5&prime;UTR, 3&prime;UTR, and RT) indicate that the retroelement RaTART corresponds to a chimeric genomic clone, consisting of distinct repetitive elements, of which only one might be present at the apparent enrichedment terminal. In the second phase of this thesis, we describe a method for the isolation and characterization of the homopolymeric (dA)/(dT) sequence described in the chromosome terminal regions of R. americana. Named T-14, this sequence shares some similarity with canonical telomeric repeats, suggesting that R. americana represents an additional example of an organism where more than one DNA sequence may extend toward the chromosome terminal regions. Finally, we present the results of heterologous hybridization to elucidate structural aspects of conservation and/or divergence in Sciaridae terminal heterochromatin. Three species of the family Sciaridae were assessed by in situ hybridization of polytene chromosomes: R. americana, Rhynchosciara milleri, and Trichosia pubescens. The DNA probe used was obtained by microdissection of non-centromeric chromosome ends from R. americana and T. pubescens, followed by amplification and labeling by degenerate oligonucleotide primed (DOP-PCR). When each probe was hybridized to own chromosome complement, two patterns were observed: (i) hybridization at all non-centromeric ends (R. americana), and most surprisingly, (ii) hybridization only at the end that gave the product of microdissection (T. pubescens). Probes obtained from R. americana produced no hybridization signals on chromosomes of T. pubescens and R. milleri. Unexpected results were obtained when the probe obtained from T. pubescens was hybridized with chromosomes of R. americana and R. milleri. Surprisingly, this probe, which scored only one end in its own chromosome complement, generated hybridization signals in all non-centromeric chromosomal ends of R. americana, as well as in its pericentromeric-centromeric heterochromatin. In R. milleri, the probe from T. pubescens clearly hybridized with centromere-associated heterochromatin of its chromosome C. The data obtained in this study support a process of chromosomal divergence between these three species of Sciaridae occurred by differential amplification of sequences of heterochromatin components, and point to an unusual structure in T. pubescens compared to other dipterans studied for terminal chromosome structure

Chromosomes

Cromossomos

Diptera

Diptera

DNA terminal

Sciaridae

Sciaridae

Terminal DNA sequences

Caracterização citogenética molecular de cromossomos marcadores extranumerários / Molecular Cytogenetic Characterization of Supernumerary Marker Chromosomes

Laus, Ana Carolina

21 May 2008

Rearranjos cromossômicos envolvendo a presença de cromossomos marcadores extranumerário são achados citogenéticos freqüentes em pacientes que apresentam deficiência mental, alterações de crescimento, dismorfias e/ou malformações. A presença desse material é responsável por trissomia ou tetrassomia parcial de determinadas regiões cromossômicas, causando quadros clínicos distintos e inespecíficos. A variabilidade fenotípica está relacionada principalmente com os diferentes graus de mosaicismo, os genes presentes na região adicional, o cromossomo de origem, entre outros fatores. Sendo assim, a caracterização desse material cromossômico é de importância fundamental para a determinação do prognóstico e do aconselhamento genético dos pacientes e suas famílias. O presente estudo teve como objetivo a análise de cromossomos marcadores extranumerários por meio de técnicas de citogenética convencional e molecular. Foram selecionados onze pacientes que são acompanhados pelo o Serviço de Genética Médica do Hospital das Clínicas da Faculdade de Medicina de Ribeirão Preto USP, todos com diagnóstico citogenético convencional por bandeamentos GTG de cromossomo marcador extranumerário. Para determinação da origem e caracterização dos cromossomos marcadores foram aplicadas as técnicas de Cariótipo Espectral (SKY) e de Hibridação in situ Fluorescente (FISH). Em dez pacientes foi possível determinar a origem e composição dos marcadores. Dois pacientes apresentam cromossomos marcadores identificados como duplicações invertidas do cromossomo 15, com cariótipos definidos, respectivamente, como 47,XY,+idic(15)(pterq15::q15pter) e 47,XX,+idic(15)(pterq21::q21p11.2), um paciente possui cromossomo marcador derivativo do cromossomo 15, com cariótipo 47,XX,+der(15)(pterq21) e dois pacientes, sendo uma menina e seu pai, possuem cromossomos marcadores derivativos do cromossomo 15 com cariótipos, respectivamente, 48,XX,+2der(15)(pterq12) e 48,XY,+2der(15)(pterq12). Dois pacientes possuem cromossomos marcadores derivativos do cromossomo 9, com cariótipos definidos, respectivamente, como 47,XX,+der(9)(pterq21) e 47,XX,+der(9)(pterq32) e um paciente apresenta cromossomo derivativo do cromossomo 4 [47,XX,+der(4)(p16q21)[9]/48,XX,+der(4)(p16q21),+mar[91]]. Um paciente possui um cromossomo marcador translocado derivativo do cromossomo 22 [47,XY,+der(22)t(11;22)(q25:q11.2)] e outro paciente, um cromossomo translocado derivativo do cromossomo 15 [47,XY,+der(15)t(15;16)(q13;q13)], ambos herdados de mães portadoras de translocações aparente balanceadas. Em um caso, não foi possível a caracterização dos cromossomos marcadores por meio das técnicas aplicadas. Há uma grande variação fenotípica associada à presença de cromossomos marcadores e muitas vezes o prognóstico e o aconselhamento genético são difíceis de determinar. As técnicas de citogenética molecular são ferramentas importantes para a caracterização dos cromossomos marcadores, tanto durante o pré-natal, como para uma família que já possui um membro afetado, auxiliando no mapeamento gênico de cada região envolvida para futura correlação cariótipo-genótipo-fenótipo. / Chromosomal rearrangements involving supernumerary marker chromosomes are frequently found in patients with mental retardation, growth defects and malformations. The genetic materials presented in trisomy/tetrasomy are responsible by distinct and unspecific clinical symptoms. The phenotypic variation is related mainly to different mosaicismo degrees, genetic content and chromosomal origin. Thus, the characterization of marker chromosomes is important to determine the prognosis and genetic counseling to the patients and their families. The aim of this study was to analyze supernumerary marker chromosomes using conventional and molecular cytogenetic techniques. Eleven patients were included in this study, all assisted in Medical Genetic Division of Clinical Hospital of School of Medicine of Ribeirao Preto USP. They all presented supernumerary marker chromosomes detected by GTG band. The origin and composition were determined using Spectral Karyotype (SKY) and Fluorescence in situ Hybridization (FISH) techniques. To ten patients, the origin and composition were determined. Two patients presented inverted duplications of chromosome 15, and their karyotype were defined as 47,XY,+idic(15)(pterq15::q15pter) and 47,XX,+idic(15)(pterq21::q21p11.2), one patient had a derivative chromosome 15, with karyotype 47,XX,+der(15)(pterq21), and two patients, a girl and her father, had two derivatives chromosomes 15, with karyotypes 48,XX,+2der(15)(pterq12) e 48,XY,+2der(15)(pterq12), respectively. Two patients presented derivative chromosomes 9 and their karyotype were defined as 47,XX,+der(9)(pterq21) and 47,XX,+der(9)(pterq32), and one patient had a derivative chromosome 4, with karyotype 47,XX,+der(4)(p16q21)[9]/48,XX,+der(4)(p16q21),+mar[91]. One patient had a translocated marker chromosome, derivative 22, [47,XY,+der(22)t(11;22)(q25:q11.2)] and another patient had a translocated marker chromosome, derivative 15 [47,XY,+der(15)t(15;16)(q13;q13)]. In one case, was not possible to define the origin and composition of the marker chromosome using SKY and FISH techniques. A large phenotypic variation is associated with supernumerary marker chromosomes and many times, the prognosis and genetic counseling is difficult to determine. The molecular cytogenetic techniques are important tools to its characterization, during prenatal diagnosis or to a family with an affected person, helping the genetic mapping of each region to a future correlation karyotype-genotype-phenotype.

Correlação Cariótipo-Fenótipo.

Correlation Karyotype-Phenotype

Cromossomos Marcadores

FISH

FISH

Marker Chromosomes

SKY

SKY