Caracterização de rearranjos cromossômicos em pacientes com malformações congênitas múltiplas e/ou retardamento mental (MCA/MR) / Characterization of chromosome rearrangements in patients with multiple congenital malformation and/or mental retardation (MCM/MR)

Mariana Angelozzi de Oliveira

05 May 2008

As alterações cromossômicas estruturais associadas a fenótipos clínicos oferecem a oportunidade de identificação e localização de genes cujas mutações possam estar determinando essas patologias, tendo em vista a possibilidade de que esses genes podem ter sido alterados pelas quebras ou ter o número de cópias modificado. Um número cada vez maior de evidências aponta para a participação de certas seqüências do genoma na formação de rearranjos cromossômicos recorrentes e não recorrentes. Este trabalho compreendeu o estudo de duas translocações cromossômicas aparentemente equilibradas e uma duplicação do braço curto do cromossomo 20 em decorrência de mosaicismo materno. O objetivo foi determinar os pontos de quebra por hibridação in situ fluorescente (FISH) e identificar genes candidatos, alterados pelas quebras dos rearranjos e que pudessem explicar o quadro clínico dos portadores. A caracterização das seqüências nos pontos de quebra e a junção desses rearranjos é fundamental para a compreensão dos mecanismos de formação das alterações cromossômicas. A delimitação precisa dos segmentos deletados é necessária para a correlação com o quadro clínico. / Two apparently \"de novo\" balanced translocations and one duplication of the short arm of chromosome 20 were studied. Our aim was to determine the breakpoints by chromosomal analysis through fluorescentin situ hybridization (FISH) and identify candidate genes and how they were involved with the clinical phenotypes of the patients. Patient 1 carried a duplication of the short arm of chromosome 20 (p11.22p13), inherited from the mother that showed normal and dup(20) lymphocytes. The duplication was determined by FISH using BAC and PAC clones, and nine clones were duplicated except one (20p11.21). The patient shared many of the common characteristics of trisomy 20p including delay in motor development, hypertelorism, poor coordination, round face with prominent cheeks, vertebral and dental abnormalities and cranial asymmetry with high and large forehead. She also had learning difficulties, behavioral disorders and pubertal growth spurt at 12 years. As our patient is an example of pure trisomy 20p, the features are of particular importance to delineate the syndrome. Three genes were mapped on the segment that contain the duplication (20p11.2-13), one of these genes is the SSTR4 (Somatostatin receptor 4). The somatostatin is widely distributed throughout the body and is important regulator of endocrine and nervous system function. It is an inhibitor of growth hormone secretion. The second gene is the BMP2 that produce bone morphogenetic proteins and it has a direct function with the nervous system. The third gene is the GHRH that produce proteins connected with the growth hormone. These genes might have been over expressed and thus contributing to the patient\'s clinical features. Patient 2, carried a 46,XY,t(5;14)(q14.1;q31.3)de novo translocation. On chromosome 14 the breakpoint was mapped to a segment contained in BAC RP11-315O17 (14q31.3). On the chromosome 5 the breakpoint was mapped to a segment contained in BAC RP11-30D15 (5q14.1). Although the breakpoint, on the chromosome 14, has been mapped in 14q31.3, our patient shared many of the common characteristics of terminal 14q32 deletion: mental retardation, dolicocephaly, prominent ears, hypertelorism, strabismus, upturned palpebral fissures, highly arched palate, simian crease, severe myopia, coloboma and palpebral ptosis. As mental retardation and ocular abnormalities were the main patient\'s clinical features, we are suggesting that: 1) a region of segment 14q31.3 was deleted. 2) A gene inside this segment (14q31.3) could be responsible for ocular development and 3) a disrupted gene could interfere on the expression of other genes. On chromosome 5 eleven genes were localized and four of them are expressed in nervous system (AP3B1; SCAMP1; BHMT2 e CMYA5). One of these genes might have been disrupted and is contributing to the patient\'s clinical features. Patient 3 was the carrier of a 46,XY,t(1;15)(p13.2;q25.2)de novo translocation. The breakpoint on chromosome 15 was mapped to the segment contained in clone RP11-152F13 (15q25.2). The breakpoint on chromosome 1 was mapped to the segment contained in clone RP5-1037B23 (1p13.2). The genes mapped at the breakpoint regions of chromosome 1 and chromosome 15 are expressed in nervous system and muscles. Our patient shows few clinical features: speech delay, stutter and learning difficulties, probably because one or more of these genes, mapped at the breakpoint region, could be disrupted.

Genes candidatos

Pontos de quebra cromossômicos

Rearranjos cromossômicos estruturais

Candidate genes

Chromosome breakpoints

Structural chromosome rearrangements

Estudo de genes candidatos em indivíduos brasileiros com dislexia / Study of dyslexia candidates genes in brazilian individuals

Svidnicki, Maria Carolina Costa Melo, 1986-

18 August 2018

Orientador: Edi Lúcia Sartorato / Dissertação (mestrado) - Universidade Estadual de Campinas, Instituto de Biologia / Made available in DSpace on 2018-08-18T01:19:09Z (GMT). No. of bitstreams: 1 Svidnicki_MariaCarolinaCostaMelo_M.pdf: 1911302 bytes, checksum: d9763aa0db5e4721a58e8e1f714fd1d0 (MD5) Previous issue date: 2011 / Resumo: A dislexia é definida como um distúrbio, ou transtorno de aprendizagem na área da leitura, escrita e soletração, que ocorre apesar de uma adequada inteligência e oportunidade sociocultural. A etiologia desse distúrbio se deve, em parte, a um importante componente genético. Ao todo, nove loci no genoma foram identificados por meio de estudos de ligação, e sete genes proeminentes foram propostos como candidatos à dislexia: DYX1C1, KIAA0319, DCDC2, ROBO1, MRPL19, C2ORF3 e KIAA0319L, mas nenhuma mutação funcional nesses genes foi efetivamente relacionada com a causa do distúrbio até o momento. O objetivo deste estudo foi verificar a relação de dados moleculares com a manifestação do distúrbio em 49 famílias de escolares brasileiros com diagnóstico de dislexia. Para isso, foi investigada a presença de grandes deleções e duplicações em algumas regiões dos genes candidatos DCDC2, KIAA0319 e ROBO1 pela técnica de Multiplex Ligation-dependent Probe Amplification (MLPA), utilizando o kit SALSA MLPA P150 (MRC-Holland, Amsterdam, The Netherlands). E além disso, foi realizado um estudo de associação utilizando 4 SNPs (Single Nucleotyde polymorphisms) presentes no gene DYX1C1, que já haviam sido relacionados com o fenótipo na literatura. A técnica de MLPA foi aplicada pela primeira vez na pesquisa de mutações em genes candidatos para a dislexia, este método foi reprodutível e o padrão de variação total por sonda foi baixo, porém a análise não revelou nenhuma deleção ou duplicação nas regiões de ligação das sondas nos genes estudados. Algumas modificações no kit de dislexia P150 foram sugeridas ao fabricante visando o aprimoramento para estudos futuros. Na etapa seguinte, a genotipagem dos SNPs foi realizada por PCR em tempo real, e a estratégia utilizada no estudo de associação foi o Teste de Transmissão de Desequilíbrio de Ligação (TDT). Nenhuma associação foi obtida para os marcadores estudados. As aparentes discrepâncias de nossos resultados com estudos anteriores podem ser explicados pelas diferenças na definição do fenótipo, a ancestralidade da amostra, o desenho do estudo, e as interações com efeitos ambientais que diferem entre populações. Esse resultado não descarta a participação do gene DYX1C1 na etiologia da dislexia, o aumento do número da amostra e de marcadores para estudos posteriores é fundamental para que se possa fazer uma análise mais completa do envolvimento desse gene no fenótipo, o que poderá fornecer importantes informações para o entendimento da dislexia e para futuros protocolos de diagnósticos e de conduta para os indivíduos afetados / Abstract: Dyslexia or reading disability is a learning disorder associated with difficulty in learning to read, writing and spelling, despite adequate intelligence and educational opportunities, with a significant heritable trait. At least nine loci in the genome were related through linkage studies, and seven prominent genes were associated with dyslexia: DYX1C1, KIAA0319, DCDC2, ROBO1, MRPL19, C2ORF3 and KIAA0319L but no functional mutation in these genes was indeed related with the disorder cause so far. The intent of this study was access the contribution of these genes in the learning disorder molecular etiology, in a sample 49 families of dyslexic Brazilian individuals. Large deletions and duplications in the candidate genes DCDC2, KIAA0319 and ROBO1 were investigated by Multiplex Ligation-dependent Probe Amplification (MLPA) technique, using the SALSA MLPA P150 kit (MRC-Holland, Amsterdam, The Netherlands). In addition, an association study was performed using 4 SNPs (Single Nucleotyde polymorphisms) in DYX1C1 gene, which had already related to the phenotype in the literature. The MLPA technique was applied for the first time in the search for candidate genes mutations in dyslexia, this method was reproducible and the overall standard variation per probe was low, but the analysis revealed no deletion or duplication in probes binding regions in the studied genes. Some modifications in the SALSA MLPA P150 kit have been suggested to the manufacturer attempting to improve it for future studies. In the next stage, SNPs genotyping was performed by real time PCR, and the strategy used in the association study was the Transmission Disequilibrium Test (TDT). No association was obtained for the markers. The apparent discrepancies of our results with previous studies can be explained by phenotype definition differences, the sample ancestry, study design, and interactions with environmental effects that differ between populations. This result does not rule out the involvement of DYX1C1 gene in the dyslexia etiology, the increase of the sample and markers numbers for future studies is essential to make a more complete analysis of this gene involvement in phenotype, which may provide important information to the dyslexia understanding and future diagnostic protocols and conduct for affected individuals / Mestrado / Genetica Animal e Evolução / Mestre em Genética e Biologia Molecular

Dislexia

Inabilidade na leitura

Gene candidato

Dyslexia

Reading disability

Candidate genes

Genetic susceptibility to fetal alcohol syndrome in the Northern Cape coloured population: Potential roles of astrotactin and reelin

Macaulay, Shelley

19 February 2007

Student Number : 0416521T - MSc(Med) dissertation - School of Pathology - Faculty of Health Sciences / Fetal alcohol spectrum disorder (FASD) encompasses a range of conditions induced by prenatal alcohol exposure. Fetal alcohol syndrome (FAS) is the most severe of these conditions. FAS is characterised by discriminating facial features along with growth deficiencies and central nervous system abnormalities. FASD is a growing concern in South Africa, particularly in the Northern and Western Cape Provinces. In the Northern Cape, astounding prevalence rates of 122 and 73.8 per 1000 school entry children have been established for the towns of De Aar and Upington respectively. Studies involving twin concordance research and animal models have indicated that there is a genetic influence contributing towards FAS susceptibility in individuals. FAS is considered a complex disease whereby both genetic and environmental factors interact in disease pathogenesis. For this reason a case-control study involving the investigation of appropriate candidate genes was conducted. The neuronal migration pathway in the developing brain is targeted by prenatal alcohol exposure. The astrotactin (ASTN) and reelin (RELN) genes were selected for investigation based on their fundamental role in neuronal migration. A FAS case-control study involving 45 cases and 112 controls was conducted on the Northern Cape Coloured population. Four single nucleotide polymorphisms (SNPs) including missense and non-coding variants were selected within ASTN and four missense SNPs were selected within RELN. The study aimed to determine the genotype and allele frequencies of the variants within the case and control groups and to assess whether any association between the gene variants and the predisposition to FAS existed. Statistical analyses indicated a significant genotypic association (P= 0.049) between RELN’s rs607755 marker; the C/T genotype was more likely to be found amongst controls thus inferring a possible protective effect against FAS. A logistic regression model supported the above association by indicating the C/T genotype as being independently significant (P= 0.026). The most limiting factor of this study was the small sample size and consequent lack of power to detect genes with minor effects. It would therefore be suggested that the study be repeated once a larger sample size has been established. A larger sample size would increase the chances of detecting true associations between genes of minor effect and FAS, thus minimising false-positive associations from arising.

fetal alcohol syndrome

FAS

candidate genes

astrotactin

reelin

Norhtern Cape

Coloured Population

FAMILY-BASED ASSOCIATION STUDIES OF THE GENETIC DETERMINANTS OF RENAL SODIUM HANDLING

Bochud, Murielle

January 2007

No description available.

hypertension

renal sodium handling

family-based association studies

candidate genes

blood pressure

Exploring candidate genes and rhizosphere microbiome in relation to iron cycling in Andean potatoes

Xiao, Hua

05 June 2017

Fe biofortification of potato is a promising strategy to prevent Fe deficiency worldwide either through traditional breeding or biotechnological approaches. These approaches require the identification of candidate genes to uptake, transport and store Fe in potato tubers. We employed multiple approaches including SNP genotyping, QTL analysis, identifying genes orthologous to Arabidopsis ferrome, yeast complementation assay and genetic transformation to avoid the limitation from a single approach. We revealed several candidate genes potentially associated with potato plant Fe acquisition, PGSC0003DMG400024976 (metal transporter), PGSC0003DMG400013297 (oligopeptide transporter), PGSC0003DMG400021155 (IRT1) and IRTunannotated (an ortholog to the IRT gene that is not annotated in the potato genome). The microorganisms in the rhizosphere react intensely with the various metabolites released by plant roots in a variety of ways such as positive, negative, and neutral. These interactions can influence the uptake and transport of micronutrients in the plant roots. Therefore, the contribution of soil microorganisms in the rhizosphere to improve Fe supply of plants may play a key role in Fe biofortification, especially under real world field-based soil scenarios. We thus investigated rhizosphere microbial community diversity in Andean potato landraces to understand the role of plant-microbial interaction in potato Fe nutrient cycling. From the analysis of the high-throughput Illumina sequences of 16S and ITS region of ribosomal RNA gene, we found that both potato landraces with low and high Fe content in tubers and a landrace on which low or high Fe content fertilizer was applied to the leaf surface had large impacts on the rhizosphere fungal community composition. Indicator species analysis (ISA) indicated that Operational Taxonomic Units (OTUs) contributing most to these impacts were closely related to Eurotiomycetes and Leotiomycetes in the phylum Ascomycota, Glomeromycetes in the phylum Glomeromycota and Microbotryomycetes in the phylum Basidiomycota. Lots of species from these groups have been shown to regulate plant mineral nutrient cycling. Our research revealed potential candidate genes and fungal taxa involved in the potato plant Fe nutrient dynamics, which provides new insights into crop management and breeding strategies for sustainable Fe fortification in agricultural production. / Ph. D.

Solanum tuberosum

Andean potato

Iron deficiency

Fe fortification

Micronutrients

Candidate genes

Iron cycling

Rhizosphere

Microbes

Variabilité fonctionnelle de gènes candidats de la lignification chez l’eucalyptus

Mandrou, Eric

16 December 2010

La lignine représente 25% de la biomasse des végétaux terrestre. Sa quantité et sa qualité sont variables au sein des populations naturelles et sont devenues des cibles de l’amélioration génétique des eucalyptus. L’identification des polymorphismes génétiques impliqués dans la variation de ces caractères permettrait de disposer d’outils de diagnostic moléculaire pour une sélection précoce des meilleurs géniteurs et ainsi contribuer à l’augmentation des gains génétiques par unité de temps. Dans ce travail de thèse nous avons décrit la variabilité nucléotidique de gènes impliqués dans la biosynthèse des lignines, ainsi que la part de la variation génétique de ces deux caractères chez trois espèces d’Eucalyptus. En intégrant ces deux niveaux de variabilité au sein de plans de croisement factoriels, nous avons identifié des polymorphismes associés à la variation des caractères. Ces travaux posent les bases de la sélection assistée par marqueurs chez l’eucalyptus. / Lignins represent 25% of plant biomass on earth. Lignins quantity and quality vary within natural populations and have become major targets for genetic improvement of eucalyptus. Identifying genetic polymorphisms involved in the variation of these traits could provide molecular tools for early selection of plus trees and contribute to increase genetic gains expected by time units. In this thesis work, we described the nucleotide diversity of genes involved in lignin biosynthesis and the genetic part of the variation of lignins quantity and quality in three eucalyptus species. Integrating these two levels of variation in a factorial matting design, we identified Single Nucleotide Polymorphisms statistically associated to the variation of lignin quality. This work paves the way to marker assisted selection in eucalyptus.

Lignines

Eucalyptus

Génétique d'association

Polymorphisme d'un seul nucléotide

Gènes candidats

Lignins

Eucalyptus

Association study

Single Nucleotide Polymorphism

Candidate genes

Genetic control of biennial bearing in apple / Étude des déterminismes génétiques de l'alternance de production chez le pommier

Guitton, Baptiste

19 December 2011

L'alternance de production est définie comme la charge en fruit d'un arbre irrégulière sur plusieurs années consécutives. La principale hypothèse en soulignant l'alternance est que la charge en fruits d'une année en cours inhibe la formation de fleurs pour l'année suivante. Ce phénomène génère d'importants problèmes agronomiques pour les espèces fruitières comme le pommier, en réduisant la production de fruits au cours des années 'OFF' et la qualité des fruits au cours des années 'ON', tout en augmentant les coûts de gestion des vergers, en particulier pour l'éclaircissage des fruits. Une stratégie pour atténuer l'alternance est de développer de nouvelles variétés avec une production régulière. Les principaux objectifs de ma thèse étaient: (i) d'améliorer les stratégies de phénotypage et les méthodes pour caractériser l'alternance de production, (ii) de disséquer le contrôle génétique de l'alternance de production en utilisant une descendance de pommier en ségrégation et d'identifier les principales régions génétiques responsables de la variation du caractère, et (iii) d'étudier les processus physiologiques sous-jacents à l'alternance de production. J'ai combiné des méthodes comme la modélisation, la génétique quantitative, la détection de Quantitative Trait Loci (QTL) et de gènes candidats ainsi que la cartographie et l'expression de gènes.Mon étude a utilisé une population de pommier ségrégation obtenue à partir d'un croisement entre des parents contrastés pour les caractéristiques architecturales et de floraison (‘Starkrimson' x 'Granny Smith'). Le phénotypage de la population pour l'alternance de production a été réalisée à l'échelle d'arbres entiers, en observant les occurrences de floraison pendant six années consécutives, et à l'échelle locale, en observant la succession de méristèmes floraux vs végétative en position terminale de rameaux. De ces données, de nouveaux modèles ont été développés afin de quantifier l'alternance de la production, en tenant compte de la croissance ontogénétique de la production et la présence / absence de floraison entre les années successives le long des pousses courtes. Ceci nous a conduits à proposer de nouveaux descripteurs de la tendance d'un génotype à l'alternance de production dans les premiers stades de développement des arbres et ouvre des possibilités pour une évaluation plus rapide et plus précoce de ce caractère dans les programmes de sélection de fruits à pépins.Pour identifier les régions génomiques impliquées dans l'alternance, une détection de QTL a été réalisée sur la base des données phénotypiques et des valeurs de BLUP obtenues à partir des modèles. J'ai démontré que la régularité de la production est sous contrôle polygénique. J'ai extrait une liste de gènes qui sont présents au sein de ces QTL en utilisant la séquence du génome du pommier. Les principaux gènes candidats identifiés sont liés aux gibbérellines, aux auxines, et à la floraison. J'ai étudié l'expression des gènes candidats co-localisant avec des QTLs par PCR quantitative en utilisant les méristèmes prélevés sur les arbres portant une forte charge en fruits vs une faible charge. Une analyse microarray m'a permis d'obtenir un aperçu global des processus biologiques et de l'expression des gènes qui sont modulés dans le méristème lorsque des fruits sont présents. Certains gènes liés à la floraison, au développement du méristème, aux gibbérellines et aux auxines ont montré un profil d'expression affectée par la présence de fruits.Mes résultats fournissent des éclaircissements sur le contrôle physiologique et génétique de ce caractère complexe qui est l'alternance et ouvrent la perspective d'inclure la régularité de production dans les schémas de sélection de pommier et d'autres espèces fruitières / Biennial bearing is defined as the irregular crop load of a tree over consecutive years. The main assumption underlining biennial bearing is that the fruit load of a given year inhibits flower formation for the following year. This phenomenon generates major agronomic problems for fruit species such as apple, by reducing fruit production during ‘OFF' years and fruit quality during ‘ON' years, while increasing orchard management costs, especially for fruit thinning. A strategy to attenuate biennial bearing is to develop new varieties with regular production. The main objectives of my project were (i) to improve phenotyping strategy and methodology for biennial bearing characterisation, (ii) to dissect the genetic control of biennial bearing using an apple segregating progeny and to identify key genetic regions responsible for the trait variation, and (iii) to investigate physiological processes underlying biennial bearing. I combined methodologies such as modelling, quantitative genetics, candidate gene and Quantitative Trait Loci (QTL) mapping and gene expression.My study used an apple segregating population issued from a cross between contrasting parents for architectural and flowering features (‘Starkrimson' x ‘Granny Smith'). Phenotyping of the population for biennial bearing was achieved at whole tree scale by observing flowering occurrence for six consecutive years, and at local scale, by observing the succession of floral vs. vegetative meristems in terminal position of shoots. From this data, new models were constructed to quantify the alternation of production, taking into account the ontogenetic increasing trend of production and the presence/absence of flowering between successive years along short shoots. This led us to propose new descriptors of the tendency of a genotype to biennial bearing in the early stages of tree development and opens possibilities for a faster and earlier evaluation of this character in pipfruit breeding programmes and for orchard management.To identify genomic regions involved in biennial bearing, a QTL detection was performed on the basis of phenotypic data and BLUP values obtained from the models. I demonstrated that the regularity of production is under polygenic control. I mined a list of genes that are present within these QTLs using the apple genome sequence. The main candidate genes identified are related to gibberellins, auxins, and flowering.I investigated the expression of candidate genes co-locating with QTLs by quantitative PCR using meristems collected on trees bearing heavy fruit load vs. light crop. A microarray analysis enabled me to obtain a global overview of biological processes and gene expression that are modulated in the meristem when fruits are present. Some genes related to flowering, meristem development, gibberellins and auxins showed an expression profile affected by the presence of fruit.My results provide elucidation on the physiological and genetic control of the complex trait that is biennial bearing and open up the perspective of including regular bearing in breeding schemes for apple and other fruit species.

Pommier

Alternance de production

Qtl

Gènes candidats

Expression de gènes

Génétique quantitative

Apple

Biennial bearing

Qtl

Candidate genes

Gene expression

Quantitative genetics

Identification et caractérisation de gènes impliqués dans la variation de caractères quantitatifs affectés par la sécheresse chez le maïs / Identification and characterization of candidat genes influencing quantitative characters for water deficit tolerance in maize

Virlouvet, Laetitia

21 April 2011

La recherche de maïs plus tolérants au déficit hydrique est un enjeu fondamental pour la production agricole dans les prochaines décennies. Le but ce travail a été d’identifier et de caractériser des gènes impliqués dans la variation de caractères complexes affectés par le déficit hydrique chez le maïs.Nous avons tout d’abord identifié des transcrits et des protéines, dont la teneur variait entre deux mélanges de lignées recombinantes différant pour une région chromosomique influençant la croissance foliaire et la protandrie en condition de déficit hydrique. Parmi les huit gènes candidats cartographiés au niveau de la région d’intérêt, se trouvait le facteur de transcription ZmMYB31 impliqué dans la biosynthèse de la lignine. Nous avons montré que son expression était corrélée à celle de deux de ses cibles, à la teneur en lignine et à l’expression du gène ZmFatA impliqué dans la biosynthèse des acides gras, suggérant un rôle régulateur de la protéine ZmMYB31 via la synthèse de lignine et de dérivés lipidiques.Dans un second volet, nous avons montré que la sur-expression du gène candidat ZmASR1 (ZmASR1-OE) chez le maïs maintenait le rendement en condition de déficit hydrique. Des analyses transcriptomiques et protéomiques nous ont permis d’identifier 25 cibles de la protéine ZmASR1, dont sept gènes impliqués dans la biosynthèse des acides aminés branchés. Nous avons également montré qu’il existait une étroite corrélation entre 13 métabolites diminués par ZmASR1-OE, six étant connus pour être négativement corrélés à la biomasse. Enfin, des résidus phosphorylés ont été identifiés chez les protéines ZmASR1, ZmASR2 et ZmASR3, suggérant leur régulation par phosphorylation. / Maize is particularly sensitive to water deficit at reproductive stages. As such, identification of factors that confer tolerance to water deficit would pave the way for increasing agricultural productivity. The aim of this work was to identify and make up the functional characterization of candidate genes for water deficit tolerance in maize.Firstly, transcriptomic and proteomic analyses of bulked recombinant inbred lines revealed eight differentially expressed genes colocating with a chromosomal region exhibiting two QTLs for leaf growth and anthesis-silking interval sensitivities to water deficit. Among them, we identified the transcription factor ZmMYB31 gene involved in the control of lignin biosynthesis. The expression of ZmMYB31 was correlated with that of its targets genes ZmCOMT and ZmFAD9, as well as ZmFatA involved in fatty acid biosynthesis. Changes in lignin and fatty acid content allowed us to hypothesis a regulatory role of ZmMYB31 via lignin and fatty acid-derived metabolites.Secondly, we showed that transgenic maize plants overexpressing the candidate gene ZmASR1 (ZmASR1-OE) maintained kernel yield under water deficit condition in the field. Transcriptomic and proteomic analyses of ZmASR1-OE leaves allowed us to identify 25 direct or indirect target genes of ZmASR1, in particular seven genes involved in branched-chain amino acid (BCAA) biosynthesis. We also showed a tight correlation between the level of 13 decreased metabolites in ZmASR1-OE leaves, 6 of which being previously shown to be negatively correlated to biomass. Phosphoresidues were also found in ZmASR1, ZmASR2 and ZmASR3, suggesting that these proteins are regulated by phosphorylation.

Maïs

Déficit hydrique

Gènes candidats

ZmMYB31

ZmASR1

Protéomique

Phosphorylation

Maize

Water deficit

Candidate genes

ZmMYB31

ZmASR1

Proteomics

Phosphorylation

ANÁLISE DO POLIMORFISMO T102C DO RECEPTOR DE SEROTONINA (HTR2A) EM PACIENTES COM FIBROMIALGIA E CONTROLES

Alves, Fernanda Aparecida Vargas de Brito e

30 June 2012

Made available in DSpace on 2016-08-10T10:38:40Z (GMT). No. of bitstreams: 1 FERNANDA APARECIDA VARGAS DE BRITO E ALVES.pdf: 1009586 bytes, checksum: 8dc12edf912fed637ebefe39ffdd52d4 (MD5) Previous issue date: 2012-06-30 / Introduction: Fibromyalgia is a syndrome characterized by widespread chronic pain. The syndrome is chronic with dubious possibility of healing. The prevalence in the world population varies from 0,66 to 4,4 %. It is believed that fibromyalgia is the result of abnormal changes in sensory processing of pain. In this context, are inserted gene polymorphisms T102C gene HTR2A serotonin receptor. The HTR2A gene T102C polymorphism is the presence of a thymine (T) or cytosine (C), defined by a transition from T to C at nucleotide position 102. It is a silent polymorphism receptor gene HTR2A, which determine the different levels of gene expression. Objectives: To determine and compare the allele frequency and genotype of the T102C polymorphism of the serotonin receptor gene HTR2A in a group of 48 women diagnosed with fibromyalgia and 50 healthy controls. Methodology: For this we used the PCR- RFLP , from DNA extracted from peripheral blood samples obtained from control and testing. The comparison of allele and genotype frequencies was performed by Chi -square test. Results: The results showed allele frequencies obtained for both groups were: T (46,9%) and C (53,1%). The TT genotype frequencies were found (22,9%), TC (47,9%) and CC (29,2%) for patients with fibromyalgia and TT (16%), TC (70%) and CC (14%) for controls. Conclusions: The FMS is composed of multiple characteristics that reflect a diversity of causes. Our results showed a significantly higher frequency for the CC genotype in patients with FMS, partially explaining the reduced serotoninergic response observed in such patients. / Introdução: A Fibromialgia é uma síndrome reumática caracterizada por dor difusa e crônica. A síndrome é crônica com duvidosa possibilidade de cura. A prevalência na população mundial varia de 0,66 a 4,4%. Acredita-se que a fibromialgia seja o resultado de mudanças anormais no processamento sensorial da dor. Neste contexto, inserem-se os polimorfismos do gene T102C do gene do receptor de serotonina HTR2A. O polimorfismo T102C do gene HTR2A consiste na presença de uma timina (T) ou citosina (C), definida por uma transição de um T para C na posição nucleotídica 102. Trata-se de um polimorfismo silencioso do gene do receptor HTR2A, que determinam níveis de expressão gênica diferentes. Objetivos: Determinar e comparar a freqüência alélica e genotípica do polimorfismo T102C do gene do receptor de serotonina HTR2A em um grupo de 48 mulheres diagnosticadas com fibromialgia e 50 controles saudáveis. Metodologia: Para isso foi utilizada a técnica de PCR-RFLP, a partir de DNA extraído de amostras de sangue periférico obtidas do grupo controle e testes. A comparação das freqüências alélicas e genotípicas foi feita por meio de teste Chi-quadrado. Resultados: Os resultados demonstraram as freqüências alélicas obtidas para os dois grupos foram: T (46,9%) e C (53,1%). As freqüências genotípicas encontradas foram TT (22,9%); TC (47,9%) e CC (29,2%) para os pacientes com fibromialgia e TT (16%); TC (70%) e CC (14%) para os controles. Conclusões: A SFM é composta por múltiplas características que refletem em uma diversidade de causas. Nossos resultados demonstraram que o genótipo CC foi significativamente mais comum nas pacientes com a SFM, justificando parcialmente a menor resposta serotononérgica observada nesse grupo.

Gene receptor de serotonina

genes candidatos

síndrome reumática

SNP

Gene serotonin receptor

candidate genes

rheumatic syndrome

SNP

CNPQ::CIENCIAS BIOLOGICAS::GENETICA

Em busca da etiologia das displasias frontonasais / In search of the etiology of frontonasal dysplasias

Rodrigues, Melina Guerreiro

04 October 2013

A displasia frontonasal (DFN) compreende quadros de aparência facial variável, sendo clinicamente caracterizada por dois ou mais dos seguintes sinais: hipertelorismo ocular com consequente alargamento da base nasal; fissura facial mediana afetando o nariz ou o nariz e lábio superior e, por vezes, o palato; fissura alar (uni ou bilateral); ponta nasal ausente; crânio anterior bífido oculto, e implantação em 'V' dos cabelos na fronte. A DFN pode ser vista como um defeito de desenvolvimento que pode ocorrer por si só ou como parte do quadro clínico de várias síndromes. A maioria dos casos de DFN é esporádica, e em raras circunstâncias foram observadas alterações cromossômicas em alguns indivíduos. Até o momento, quatro genes foram relacionados à patogênese molecular de algumas das síndromes com DFN, EFNB1, associado a uma forma de DFN ligada ao X e os genes ALX1, ALX3 e ALX4, todos associados a formas de DFN com herança autossômica recessiva. Embora esteja claro haver heterogeneidade etiológica, na maioria dos casos de DFN a causa não é conhecida, dificultando o adequado aconselhamento genético aos pacientes e seus familiares. Sendo assim, realizamos estudos com diferentes estratégias metodológicas buscando melhor compreender as possíveis causas genéticas da DFN. Ao todo foram analisados 10 pacientes: um caso familial de DFN leve com herança aparentemente autossômica dominante, um caso clinicamente sugestivo de mutação em ALX1, e oito casos de DFN associada a atraso de desenvolvimento com ou sem outras anomalias, dos quais um apresentava um rearranjo de novo aparentemente balanceado entre os cromossomos 4 e 12. Optamos por realizar sequenciamento dos genes previamente relacionados a fenótipos com DFN em todos os casos; para aqueles em que não foram detectadas mutações patogênicas, realizamos análise de variações de número de cópias (CNV) por microarray de polimorfismos de base única e, para o paciente com rearranjo cromossômico, realizamos o mapeamento do ponto de quebra por hibridação in situ fluorescente. Constatamos uma mutação em heterozigose no gene ALX4 co-segregando com o fenótipo do caso familial, sendo esta a primeira descrição de alteração em tal gene causando uma forma de DFN com herança dominante, e sugerimos pela primeira vez um mecanismo de dominância negativa. No caso sugestivo de mutação em ALX1, o diagnóstico foi confirmado através da identificação de uma mutação em homozigose neste gene do paciente; este caso consiste no 3o da literatura mundial e evidencia pela primeira vez que mutações em ALX1 não necessariamente levam a atraso de desenvolvimento ou deficiência intelectual. Os estudos citogenéticos e moleculares dos pontos de quebra do paciente com rearranjo cromossômico sugeriram os genes ARAP2 e CAND1 como possíveis responsáveis por seu quadro clínico, enquanto o estudo de CNVs nos indivíduos com DFN associada a atraso de desenvolvimento apontou os genes DNAJB12 e ENOX2 como possíveis candidatos para explicar o fenótipo de dois dos pacientes. É preciso que novos estudos sejam realizados a fim de melhor compreender o significado de tais achados e a real contribuição de cada gene para o desenvolvimento craniofacial humano e para a etiologia da DFN. Para os casos em que não foram identificadas alterações conclusivas no presente estudo, embora causas ambientais não possam ser descartadas, é preciso que seja investigada também a existência de fatores genéticos e epigenéticos não detectáveis pelas metodologias utilizadas, bem como a hipótese de mosaicismo somático. Nossos resultados, além de corroborarem o envolvimento dos genes ALX1 e ALX4 em fenótipos com DFN, sugerem também novos genes candidatos: ARAP2, CAND1, DNAJB12 e ENOX2 / Frontonasal dysplasia (FND) is a rare group of disorders that comprises cases with a variety of facial appearances, and is clinically characterized by two or more of the following signs: ocular hypertelorism with consequent broadening of the nasal root; median facial cleft affecting the nose and/or upper lip and palate; clefting of the alae nasi (uni or bilateral); lack of formation of the nasal tip; anterior cranium bifidum occultum; and a V-shaped frontal hairline. FND is a developmental defect that can occur alone or as part of several syndromes. Most cases of FND are sporadic, and in rare circumstances chromosomal alterations were observed in affected individuals. To date, four genes have been related to the molecular pathogenesis of some syndromes with DFN, one (EFNB1) is associated with an X-linked form while the 3 others (ALX1, ALX3 and ALX4) are associated with autosomal recessive forms. Although it is clear that FND is etiologic heterogeneous, the causative mechanism is unknown in most cases which makes it hard to give proper genetic counseling to patients and their families. In order to get new insights into the genetic mechanisms leading to FND, we performed studies with different methodologies. Altogether, 10 patients were analyzed: a familial case of a mild form of FND with an apparently autosomal dominant inheritance pattern, a case clinically suggestive of mutation in ALX1, and eight cases of FND associated with developmental delay with or without other anomalies, one of which with an apparently balanced de novo rearrangement between chromosomes 4 and 12. We chose to sequence the genes previously associated with FND phenotypes in all cases; for those in which pathogenic mutations were not detected, we conducted an analysis of copy number variations (CNV) by single nucleotide polymorphisms microarrays; for the patient with chromosomal rearrangement, we also mapped the breakpoints by using fluorescence in situ hybridization. We found a heterozygous mutation in ALX4 co-segregating with the phenotype of the familial case; this is the first description of mutation in this gene causing a form of FND with dominant inheritance pattern, and we suggested for the first time a dominant negative mechanism. In the case suggestive of mutation in ALX1, the diagnosis was confirmed by the identification of a homozygous mutation in this gene; this is the third case of the literature and shows for the first time that mutations in ALX1 are not necessarily related to developmental delay or intellectual disability. Breakpoints cytogenetic and molecular studies done with the patient with chromosomal rearrangement suggested ARAP2 and CAND1 genes as causative candidates for his condition, while the study of CNVs in individuals with FND associated with developmental delay pointed DNAJB12 and ENOX2 genes as possible candidates to explain the phenotypes of two of the patients. Further studies are necessary to better understand the significance of such findings and the actual contribution of each of these genes to human craniofacial development and the etiology of FND. Although environmental causes cannot be ruled out, it should also be investigated the existence of genetic and epigenetic factors as well as the possibility of somatic mosaicism, among the cases negative for the molecular approaches used in our study. Our results corroborate the involvement of ALX1 and ALX4 in FND phenotypes, and suggest new candidate genes: ARAP2, CAND1, DNAJB12 and ENOX2.

ALX1

ALX1

ALX4

ALX4

Candidate genes

CNV

CNV

Displasia frontonasal

Frontonasal dysplasia

Genes candidatos

Rearranjos cromossômicos estruturais

Structural chromosomal rearrangements