Genetic structure and reproductive partitioning in a primitively eusocial wasp

Bolton, Alan Richard

January 2002

No description available.

590

Genetic heterogeneity

Molecular genetics of autosomal recessive spinocerebellar ataxias

Christodoulou, Kyproula

January 1995

No description available.

572.8

STRATIFIED LINKAGE ANALYSIS BASED ON POPULATION SUBSTRUCTURE

Thompson, Cheryl L.

06 April 2007

No description available.

Linkage Analysis

admixture

population stratification

genetic heterogeneity

Overcoming the Current Limitations of Next-Generation Sequencing with New Methods for Local Assembly of Genomes and High-Specificity Rare Mutation Detection

Preston, Jessica

23 February 2016

The relatively low cost of Next-Generation Sequencing (NGS) has enabled researchers to generate large amounts of sequencing data in order to identify disease-causing mutations and to assemble simple genomes. However, NGS has inherent limitations due to the short DNA read lengths and high error rate associated with the technique. The short read lengths of NGS prevent the assembly of genomes with long stretches of repetitive DNA, and the high error rate prevents the accurate detection of rare mutations in heterogeneous populations such as tumors and microbiomes. I have co-developed new NGS methods to overcome these challenges. In order to increase the effective read length of NGS reads, local de novo assembly of short reads into long contigs can be achieved through the use of Paired-End Restriction-site Associated DNA Sequencing (RAD-PE-Seq). With the RAD-PE method, I sequenced a stickleback fosmid and generated contigs with an N50 length of 480 nucleotides. In order to eliminate false-positive mutations caused by the high error rate of NGS, the Paired-End Low Error Sequencing (PELE-Seq) method was developed, which uses numerous quality control measures during the sequencing library preparation and data analysis steps in order to effectively eliminate sequencing errors. Control testing of the PELE-Seq demonstrates that the method completely eliminates false-positive mutations at sequencing read depths below 20,000X coverage, compared to a ~20% false-positive rate obtained with previous methods. The high accuracy of the PELE-Seq method allows for the detection of ultra-rare mutations in a genome, which was previously impossible with NGS. This dissertation includes previously published and unpublished co-authored material.

Blood biopsy

Evolutionary biology

Genetic heterogeneity

Minor alleles

Next-generation sequencing

Single nucleotide polymorphisms

Avaliação de novos polimorfismos nos genes TGFB3, MSX1, MYH9 e JAG2 em pacientes com fissuras lábio-palatinas não-sindrômicas / Evaluation of novel polymorphisms in genes TGFB3, MSX1, MYH9 and JAG2 in non syndromic cleft lip and palate

Aquino, Sibele Nascimento de, 1984

18 August 2018

Orientador: Hercílio Martelli Júnior / Dissertação (mestrado) - Universidade Estadual de Campinas, Faculdade de Odontologia de Piracicaba / Made available in DSpace on 2018-08-18T03:14:48Z (GMT). No. of bitstreams: 1 Aquino_SibeleNascimentode_M.pdf: 1254396 bytes, checksum: 23d834d1395b6d0cfe104c6231785589 (MD5) Previous issue date: 2011 / Resumo: Fissuras do lábio e/ou palato (FL/P) representam uma das anomalias congênitas mais comuns em humanos. A etiologia das FL/PNS é complexa e envolve a participação de inúmeros genes e fatores ambientais. Diversos estudos têm investigado genes relacionados a síndromes, que apresentam FL/P em seu espectro clínico, e/ou que são expressos durante o desenvolvimento do lábio e/ou palato. O objetivo deste estudo foi verificar se novos polimorfismos contidos nos genes relacionados ao desenvolvimento do lábio e palato, incluindo TGF?3, MSX1, MYH9 e JAG2, podem contribuir para a etiologia das FL/PNS. Seis regiões polimórficas foram genotipadas por PCR-RFLP (reação em cadeia da polimerase associada à análise de polimorfismo de fragmentos de restrição enzimática) em amostras de DNA proveniente de 367 pacientes com FL/PNS (grupo caso) e de 413 indivíduos não afetados (grupo controle). No grupo caso, 54% foram do gênero masculino e 46% do feminino, com idade média de 19,1 ± 14,9 anos e prevalência de indivíduos feodermas (42,5%) e leucodermas (42%). As fissuras lábio-palatinas (FLP) foram predominantes (54%), seguidas pela fissura labial (FL) (24%) e fissura palatina (FP) (22%). Do total de seis polimorfismos analisados neste estudo, apenas um foi confirmado nessa população: rs1057744 do gene JAG2. Para este locus polimórfico, o alelo A e o genótipo GA foi mais comum, no grupo controle e caso, não sendo encontrada diferença estatística significante. Para esse polimorfismo, a análise em um modo dominante ou recessivo também não mostrou diferenças estatísticas significantes. Assim, demonstrou-se que os polimorfismos rs34019007 e rs4252315, do gene TGF?3, rs62636562, do gene MSX1, rs11549910 e rs11549909, do gene MYH9 não foram confirmados. O polimorfismo rs1057744 do gene JAG2, embora confirmado, não apresentou associação significante com FL/PNS na população avaliada / Abstract: Cleft lip and/or cleft palate (CL/P) is one of the most common congenital anomaly in humans. NSCL/P etiology is complex and involves the participation of numerous genes and environmental factors. Several studies have investigated genes related to syndromes that have CL/P in their clinical and/or which are expressed during the development of lip and palate. The aim of this study was to determine whether polymorphisms contained genes related to the development of lip and/or palate, including TGF?3, MSX1, MYH9 and JAG2 can contribute to the etiology of NSCL/P. Six polymorphic regions were genotyped by PCR-RFLP (restriction fragment length polymorphism-polymerase chain reaction) in DNA samples from 367 patients affected by NSCL/P (experimental group) and 413 clinically normal subjects (control group). In the affected group, 54% were male and 46% female, mean age 19.1 ± 14.9 years and the prevalence of mixed black individuals (42.5%) and Caucasian (42%). The clefts of the lip with or without cleft palate (CLP) were predominant (54%), followed by cleft lip (FL) (24%) and cleft palate FP (22%). Out of 6 probable polymorphisms, only one was confirmed in this population: rs1057744 gene JAG2. For this polymorphic locus, the A allele and the genotype was slightly more common in the contr ol and experimental, without statistically signific ant differences. For this polymorphism , the analysis in a dominant or recessive mode also showed no statistically significant difference s between the group. This study demonstrated that the polymorphisms rs34019007 and rs4252315, present in the gene TGF?3, rs62636562, in the MSX1 gene, rs11549910 and rs11549909, in the MYH9 gene we re not confirmed. The rs1057744 polymorphism in JAG2 gene was confirmed in this study but not significantly associated with NSCL/P in the Brazilian population / Mestrado / Patologia / Mestre em Estomatopatologia

Anomalias craniofaciais

Frequência dos genes

Heterogeneidade genética

Craniofacial abnormalities

Gene frequency

Genetic heterogeneity

The role of chromosomal instability in therapy response of colorectal cancer

Liu, Xiyang

21 November 2017

No description available.

610

Genetic heterogeneity

herapy response

Colorectal cancer

Chromosomal instability

Medizin (PPN619874732)

Biologie (PPN619875151)

A comprehensive phenotypic and molecular analysis of congenital and childhood cataract

Gillespie, Rachel Louise

January 2015

A comprehensive molecular and phenotypic analysis of congenital and childhood cataractRachel L. Gillespie; The University of Manchester, Doctor of Philosophy, 2015Congenital and childhood cataract (CCC) is estimated to affect 3.5-6 per 10,000 children under 16 years in developed countries - a major cause of lifelong visual impairment. It is estimated that 25-50% of CCC cases are caused by genetic mutations. CCC demonstrates extreme heterogeneity with more than 100 associated genes, and may occur as an isolated anomaly of the eye (non-syndromic) or as a manifestation of a multisystem condition (syndromic). Limitations of conventional sequencing technologies have precluded precise genetic diagnosis and limited understanding of the epidemiological basis of the condition. Next generation sequencing (NGS) technologies have revolutionised the approach to the study of human disease. The aim of this research was to conduct a comprehensive molecular and phenotypic analysis of CCC using NGS.A disease-targeted NGS assay was designed to screen, in parallel, 115 genes associated with all forms of CCC. DNA from 36 patients, randomly selected from the study cohort, underwent cataract-targeted NGS. Putative cataract-causing variants were identified in 75% of individuals; 85% of non-syndromic patients and 63% of syndromic CCC patients. Cataract-targeted NGS was able to efficiently delineate disease sub-type and in some cases identified rare syndromic forms of the condition. These findings were envisaged to alter care and management of CCC patients demonstrating the potential clinical utility of the test. In a subset of cases, NGS identified CCC was a manifestation of an inborn error of metabolism. A number of these conditions were eligible for preventative treatment emphasizing the importance of early diagnosis. A strategic approach to the identification of novel recessive causes of CCC was also undertaken. Affected children from seven consanguineous families underwent pre-screening by cataract-targeted NGS to delineate those with mutations in known genes. Mutation negative patients underwent autozygosity-guided whole exome sequencing (WES) analysis. This strategic approach to disease gene discovery led to the identification three novel cataract-causing candidate genes, TRIM8, CCDC13 and GRWD1. It also led to the association of EIF2B2, known to cause adult-onset leukoencephalopathy with vanishing white matter (VWM) disease featuring pre-senile onset cataract, with childhood-onset cataract. This work demonstrated that cataract-targeted NGS offers an efficient and unbiased means of pre-screening, however, causation is difficult to assign to novel disease genes in the absence of experimental evidence. Correspondingly, in vitro analysis of a missense variant in HMX1 demonstrated the deleterious effect of the mutation on protein function. This work confirmed HMX1 as the cause of a rare oculoauricular phenotype and expanded the class of disease-causing mutations in this gene. In conclusion, this study has demonstrated that NGS is effective in the study of CCC and has provided a platform for future studies in to the genetic aetiology of the condition, as well as the molecular mechanisms underlying lens transparency and human development. The work adds to the increasing body of evidence that augurs an era of personalised genomic medicine in ophthalmology that will foresee improved patient outcomes attributable to the implementation of a stratified approach to medicine.

618.92

Genetic Heteroscedasticity for Domestic Animal Traits

Felleki, Majbritt

January 2014

Animal traits differ not only in mean, but also in variation around the mean. For instance, one sire’s daughter group may be very homogeneous, while another sire’s daughters are much more heterogeneous in performance. The difference in residual variance can partially be explained by genetic differences. Models for such genetic heterogeneity of environmental variance include genetic effects for the mean and residual variance, and a correlation between the genetic effects for the mean and residual variance to measure how the residual variance might vary with the mean. The aim of this thesis was to develop a method based on double hierarchical generalized linear models for estimating genetic heteroscedasticity, and to apply it on four traits in two domestic animal species; teat count and litter size in pigs, and milk production and somatic cell count in dairy cows. The method developed is fast and has been implemented in software that is widely used in animal breeding, which makes it convenient to use. It is based on an approximation of double hierarchical generalized linear models by normal distributions. When having repeated observations on individuals or genetic groups, the estimates were found to be unbiased. For the traits studied, the estimated heritability values for the mean and the residual variance, and the genetic coefficients of variation, were found in the usual ranges reported. The genetic correlation between mean and residual variance was estimated for the pig traits only, and was found to be favorable for litter size, but unfavorable for teat count.

Quantitative genetics

genetic heteroscedasticity of residuals

teat count in pigs

litter size in pigs

milk yield in cows

somatic cell count in cows

Hétérogénéité génétique et clonale des Syndromes Myélodysplasiques / Genetic and clonal heterogeneity of myelodysplastic syndromes

Chesnais, Virginie

15 December 2015

Les syndromes myélodysplasiques (SMD) forment un groupe de pathologies clonales de la cellule souche hématopoïétique (CSH) caractérisées par une hématopoïèse inefficace. La présence d’au moins une anomalie génétique (anomalie cytogénétique ou mutation somatique) est observée dans plus de 90% des cas. Ainsi, plusieurs clones moléculaires pouvaient coexister au moment du diagnostic de la maladie. Dans les SMD avec délétion du chromosome 5 (del(5q)), il a récemment été montré que les anomalies étaient présentes dès le stade de la CSH. Dans les SMD, la pénétrance des anomalies génétiques décrites est incomplète. De plus, peu de choses sont actuellement connues sur l’ordre d’apparition des mutations et leur impact fonctionnel sur les différents clones moléculaires dans le cas des SMD non-del(5q). Grâce au séquençage d’exome entier (WES) de patients ne présentant aucune mutation dans les gènes décrits dans les SMD, nous avons décrit l’existence de mutations dans les gènes BCOR et BCORL1, chez respectivement 4,2% et 0,8% des patients. Les mutations du gène BCOR arrivent tardivement au cours de l’évolution de la maladie et affectent le pronostic des patients. Des approches à l’échelle unicellulaire nous ont également permis d’observer que la majeure partie des mutations identifiées chez les patients sont retrouvées dès le stade CD34+CD38-. Chez les patients, plusieurs clones moléculaires coexistent à ce stade. De plus, les mutations des gènes de l’épissage et de la régulation épigénétique sont fréquemment acquises en premier dans les cellules hématopoïétiques les plus immatures des patients porteurs de SMD. Nous avons observé que certaines mutations, acquises secondairement, sont réparties inégalement dans les différents compartiments hématopoïétiques et peuvent avoir un impact sur la différenciation hématopoïétique. Enfin, nous montrons que la répartition des clones moléculaires évolue au cours du temps. En réponse au traitement par Lenalidomide, on observe également une évolution rapide de l’architecture clonale qui peut être liée au statut de réponse des patients. Ces résultats tendent à confirmer l’hétérogénéité génétique mais aussi fonctionnelle des SMD. Nous avons pu identifier de nouvelles mutations impliquées secondairement dans la physiopathologie des SMD. Il existe une dominance clonale précoce dans les SMD du fait de l’acquisition de toutes les mutations dans les cellules hématopoïétiques immatures. Cependant, les différentes populations hématopoïétiques peuvent présenter des génotypes différents. Enfin cette architecture est variable au cours de l’évolution de la maladie. / Myelodysplastic syndromes (MDS) are a group of clonal disorders of the hematopoietic stem cell (HSC) characterized by ineffective hematopoiesis. At least one genetic abnormality (cytogenetic abnormality or somatic mutation) is observed in more than 90% of cases. Thus, it has been observed several molecular clones which could coexist at diagnosis of the disease. In MDS with deletion of chromosome 5 (del (5q)), it has recently been shown that defects were present in the HSC. In MDS, the penetrance of genetic abnormalities described is incomplete. In addition, little is currently known about the order of appearance of mutations and their functional impact on different molecular clones in the case of non-del (5q) MDS. Through the whole exome sequencing (WES) of patients without mutation in the genes described in MDS, we described the existence of mutations in genes BCOR and BCORL1, in respectively 4.2% and 0.8% of patients. Mutations in the gene BCOR were acquired lately during the course of the disease and affect the prognosis of patients. Approaches at the single cell level have also allowed us to observe that most of the mutations identified in patients are found at the immature differentiation stage CD34+CD38-. In patients, several molecular clones could coexist at this stage. In addition, mutations in gene splicing and epigenetic regulation are frequently first acquired in the most immature hematopoietic cells of MDS patients. We found that certain mutations, acquired in a second time, are distributed unevenly in different hematopoietic compartment and may have an impact on hematopoietic differentiation. Finally, we showed that the distribution of molecular clones evolves over time. In response to treatment with Lenalidomide, it has also been observed a rapid evolution of clonal architecture that can be linked to patient response status. These results tend to confirm the genetic but also functional heterogeneity in MDS. We have identified new mutations involved in the pathogenesis of MDS. We observed an early clonal dominance in MDS because of the acquisition of all mutations in immature hematopoietic cells. However, different hematopoietic populations can have different genotype. Finally, the architecture of mutations could be modifying during the course of the disease.

Syndromes Myélodysplasiques

Mutations

Hétérogénéité génétique

Oligoclonalité

Myelodysplastic

Mutations

Genetic heterogeneity

Oligoclonality

616.15

Evidências moleculares da transmissão horizontal do vírus da hepatite C (VHC) entre cônjuges / Molecular evidences for horizontal transmission of HCV inside couples

Mello, Isabel Maria Vicente Guedes de Carvalho

09 November 2006

A transmissão do VHC vem diminuindo após a implementação de diretrizes de triagem de doadores de sangue e adoção de políticas sociais para reduzir o risco de infecção em UDI, entretanto o VHC ainda constitui um grave problema de saúde pública mundial. Em torno de 10% dos pacientes infectados com VHC não referem exposição a nenhum fator de risco conhecido. Alguns estudos demonstraram a presença de RNA em diferentes secreções, sugerindo a existência de outras rotas de transmissão do VHC. Este estudo teve como objetivo analisar as relações filogenéticas de diferentes regiões genômicas do VHC de cônjuges portadores crônicos e correlacioná-las com seqüências de portadores crônicos não relacionados atendidos no mesmo ambulatório. Foram selecionados 18 pacientes (9 casais) com genótipo concordante entre eles e 42 controles (14 de cada genótipo encontrados nos casais). Foram amplificadas e seqüenciadas as regiões NS3 (~620nt) e NS5B (~360nt). As seqüências foram alinhadas usando o programa Clustal X e Bioedit 6.0.7. A presença do sinal filogenético, nas regiões estudadas, foi analisado através do mapeamento da verossimilhança pelo programa Tree-Puzzle. Os modelos evolucionários foram estimados pelo teste de razão de verossimilhança com o auxílio do programa Modeltest e utilizados para as análises das seqüências NS3, NS3+NS5B (TrN+I+G) e NS5B(TrNef+I+G). Foram empregados os métodos de distância com algoritmo de agrupamento de vizinhos e máxima verossimilhança com o algoritmo de rearranjo dos braços, seccionando a árvore em dois pedaços e ligando em outras partes, para a construção das árvores, pelo programa PAUP*4b10. Foram calculados os valores de bootstrap, com 1000 réplicas, para a verificação da sustentação de ramos nas topologias. Nas análises foram incluídas seqüências referencia do Genbank de diferentes genótipos. Todos os casais tiveram a região NS5B amplificada e seqüenciada, entretanto, não foi possível amplificar e seqüênciar a região NS3 de amostras de 2 casais. Considerando-se as três análises o sinal filogenético foi de 90.5% (NS5B - 199 nt), 92.9% (NS5B - 344 nt), 94.8% (NS3 - 619 nt ) e 96.1% (NS5B + NS3). Como esperado, o melhor sinal filogenético foi obtido com as seqüências das duas regiões concatenadas NS3+NS5B. As análises filogenéticas sugerem fortemente que os vírus dos casais 3, 4, 6, 7, e 8 têm a mesma origem. Na maioria das análises as seqüências dos vírus destes casais formaram um grupo monofilético com valores de bootstrap acima de 70. As seqüências dos outros casais, em algumas situações, apresentaram grupos monofiléticos, contudo os valores de bootstrap não foram significativos. A utilização de seqüências de duas regiões genômicas diferentes suportam a hipótese de que os vírus dos casais 3, 4, 6, 7 e 8 têm a mesma origem. A inclusão de seqüências controle, dos mesmos subtipos encontrados nas amostras dos casais, foram fundamentais para a confirmação dos resultados. Estes resultados indicam fortemente a possibilidade de transmissão entre casais. / HCV transmission has decreased with the adoption of universal blood donors screening and social policies to reduce risk of infection in IVDU, but HCV is still a worldwide health problem. The epidemiological route of infection cannot be identified in a significant proportion of patients. Some studies demonstrated the presence of viral RNA in different secretions, suggesting the existence of other routes for HCV transmission. The aim of this study was to evaluate the phylogenetical relationships among sequences from different HCV genomic regions from sexual partners of chronic infected patients when analyzed among themselves and when analyzed conjointly with sequences from virus found in non related chronic infected patients attended in the same clinic. Eighteen individuals (9 couples with stable relationship without other risk factors for HCV infection) and forty-two control patients (fourteen from each genotype found in the couples) were selected. NS3 (~620 nts) and NS5B (~360 nts) regions were amplified and sequenced. Sequences were aligned using clustal X 1.81 and Bioedit 6.0.7. Phylogenetic signal/noise ratio in the data set was investigated with a likelihood mapping analysis with the program TREE-PUZZLE. Evolutionary models were chosen by Hierarchical Likelihood Ratio Test (hLRTs) using Modeltest 3.06 and used for analyze NS3, NS3+NS5B (TrN+I+G) and NS5B (TrNef+I+G) sequences. Distance and maximum-likelihood (ML) phylogenetical analyses were performed with PAUP*4b10 and the trees were constructed with NJ and heuristic search. Tree bisection and reconnection (TBR) algorithm respectively.Robustness of trees was evaluated by analyzing 1000 bootstrap replicates. Genbank reference sequences from different genotypes were included in data analysis. Sequences from NS5B region were obtained for all samples while it was not possible to get NS3 sequences from only 2 couples. Considering the three analysis, phylogenetical signals were 90.5% (NS5B - 199 nt), 92.9% (NS5B - 344 nt), 94.8% (NS3 - 619 nt ) and 96.1% (NS5B + NS3). As expected, the best phylogenetical signal was obtained with concatened NS3+NS5B sequences. Phylogenetical analysis strongly suggested that virus from couples 3, 4, 6, 7 and 8 had a common origin. In the majority of the analysis, sequences inside these couples clustered in the same monophyletical group with bootstrap values higher than 70. For the other couples, monophyletical groups were observed but these results were not supported by the bootstrap analysis. In conclusion, using sequencing from two different viral genomic regions, we have strongly supported a common source of infection for the two members of five couples. Control sequences from the same subtypes than the couples were crucial to confirm the results. These data strongly support HCV transmission inside couples.

Chronic C hepatitis

Disease transmission horizontal

Fatores de risco

Filogenia

Genetic heterogeneity

Genótipo

Genotype

Hepatite C crônica

Heterogeneidade genética

Phylogeny

Risk factors

Transmissão horizontal de doença