Frequent p16-independent inactivation of p14ARF in human melanoma

Freedberg, D.E., Rigas, S.H., Russak, J., Gai, W., Kaplow, M., Osman, I., Turner, F., Randerson-Moor, J.A., Houghton, A., Busam, K., Bishop, D.T., Bastian, B.C., Newton-Bishop, J.A., Polsky, D.

January 2008

No / BACKGROUND: The tumor suppressors p14(ARF) (ARF) and p16(INK4A) (p16) are encoded by overlapping reading frames at the CDKN2A/INK4A locus on chromosome 9p21. In human melanoma, the accumulated evidence has suggested that the predominant tumor suppressor at 9p21 is p16, not ARF. However, recent observations from melanoma-prone families and murine melanoma models suggest a p16-independent tumor suppressor role for ARF. We analyzed a group of melanoma metastases and cell lines to investigate directly whether somatic alterations to the ARF gene support its role as a p16-independent tumor suppressor in human melanoma, assuming that two alterations (genetic and/or epigenetic) would be required to inactivate a gene. METHODS: We examined the p16/ARF locus in 60 melanoma metastases from 58 patients and in 9 human melanoma cell lines using multiplex ligation-dependent probe amplification and multiplex polymerase chain reaction (PCR) to detect deletions, methylation-specific PCR to detect promoter methylation, direct sequencing to detect mutations affecting ARF and p16, and, in a subset of 20 tumors, immunohistochemistry to determine the effect of these alterations on p16 protein expression. All statistical tests were two-sided. RESULTS: We observed two or more alterations to the ARF gene in 26/60 (43%) metastases. The p16 gene sustained two or more alterations in 13/60 (22%) metastases (P = .03). Inactivation of ARF in the presence of wild-type p16 was seen in 18/60 (30%) metastases. CONCLUSION: Genetic and epigenetic analyses of the human 9p21 locus indicate that modifications of ARF occur independently of p16 inactivation in human melanoma and suggest that ARF is more frequently inactivated than p16.

Animals

Cell line

Tumor

Chromosomes

Pair 9

DNA methylation

Gene deletion

Gene silencing

Genes

p16

Humans

Immunoblotting

Immunohistochemistry

Melanoma

Genetics

Pathology

Mice

Microsatellite repeats

Mutation

Neoplasm proteins

Polymerase chain reaction

Promoter regions

Tumor suppressor protein p14ARF

REF 2014

Coming full circle: the development, rise, fall, and return of the concept of anticipation in hereditary disease

Friedman, Judith Ellen

26 October 2009

This dissertation examines the history of the creation and development of the concept of anticipation, a pattern of heredity found in several diseases (e.g. Huntington’s disease and myotonic dystrophy), in which an illness manifests itself earlier and often more severely in successive generations. It reconstructs major arguments in twentieth-century debates about anticipation and analyzes the relations between different research communities and schools of thought. Developments in cutting-edge medicine, biology, and genetics are analyzed; many of these developments were centered in Britain, but saw significant contributions by people working in France, Germany, Switzerland, the Netherlands and North America. Chapter one traces precursor notions in psychiatric and hereditarian thought from 1840 to the coining of the term ‘anticipation’ by the ophthalmologist Edward Nettleship in 1905. Key roles in the following chapters are played by several figures. Prior to World War II, these include: the neuropathologist F.W. Mott, whose advocacy during 1911- 1927 led to anticipation being called “Mott’s law”; the biometrician and eugenicist Karl Pearson, who opposed Mott on methodological and political grounds; and two politically and theoretically opposed Germans – Ernst Rüdin, a leading psychiatrist and eugenicist who came to reject anticipation, and Richard Goldschmidt, a geneticist who offered a peculiar Mendelian explanation. The British psychiatrist and human geneticist, Lionel Penrose, makes a first interwar appearance, but becomes crucial to the story after World War II due to his systematic dismissal of anticipation, which discredited the notion on orthodox Mendelian grounds. The final chapters highlight the contributions of Dutch neurologist Christiaan Höweler, whose 1980s work demonstrated a major hole in Penrose’s reasoning, and British geneticist Peter Harper, whose research helped demonstrate that expanding trinucleotide repeats accounted for the transgenerational worsening without contradicting Mendel and resurrected anticipation as scientifically legitimate. Reception of the concept of anticipation is traced across the century through the examination of textbooks used in different fields. This dissertation argues against established positions regarding the history of the concept, including claims that anticipation’s association with eugenics adequately explains the rejection of the notion after 1945. Rejected, in fact, by many eugenicists from 1912, anticipation was used by physicians until the 1960s.

Eugenics

Medicine

Genetics

trinucleotide repeat disorders

Heredity

Biology

Genetic Anticipation

myotonic dystrophy

Huntington's disease

Fragile X

schizophrenia

Psychiatry

trinucleotide repeat expansion disorders

expanding trinucleotide repeats

Exploring TERRA (TElomeric Repeat-containing RNA) Expression and Regulation During Cell Growth in Saccharomyces cerevisiae

Perez Romero, Carmina Angelica

08 1900

Please find the referenced videos attached / The physical ends of eukaryotic chromosomes consist of repetitive DNA sequences, which are associated with specialized proteins forming a nucleoprotein structure essential for the integrity of the linear chromosomes, and are known as telomeres. Telomerase is an enzyme responsible for the maintenance of the telomeric repeats at the end of the chromosomes. Telomerase is a ribonucleoprotein, which contains a catalytic subunit that possesses reverse transcriptase activity, and a RNA subunit that acts as a template, since it possess the telomeric repeat sequences necessary to amplify telomere ends. Telomeres are transcribed in most eukaryotes into a non-coding RNA know as TERRA (Telomeric repeats-containing RNA). It has been proposed that TERRA may act as a regulator of telomere homeostasis, and as an inhibitor of telomerase, however, its specific function is still unknown. In Saccharomyces cerevisiae, TERRA is rapidly degraded by the 5’-3’ Rat1 exonuclease, which has hampered its study by classic biochemical experiments in yeast. In this thesis, we report the use of cytological approaches to study TERRA in budding yeast. Two different approaches were used for this purpose: the fluorescent in-situ hybridization (FISH) and the labeling of TERRA by the MS2-GFP system, which allow the visualization of TERRA transcripts form a single telomere in living cells. With these two approaches, we observed that TERRA is expressed from a single telomere and accumulates as a single perinuclear foci, in a small percentage of cells population. We also demonstrate that TERRA expression occurs due to telomere shortening. We demonstrate that TERRA interacts in vivo with the telomerase RNA (TLC1) in yeast. Telomere elongation depends on the action of several telomerase molecules that are visible as clusters, which associate with telomeres in late S phase in yeast, and mammalian cells. In adidition, we show that TERRA stimulates the nucleation of telomerase clusters. By performing time course experiments of TERRA and TLC1 RNA in live cells, we observed that TERRA acts as a scaffold for generating telomerase clusters, which are then recruited in late S phase to the telomere from which TERRA molecules originated. The recruitment of TERRA to its telomere of origin is dependent on factors that control telomerase recruitment at telomeres like: Mre11, Tel1 and the yKu complex. We propose that a short telomere expresses TERRA to assemble and organize telomerase molecules, which later on allows their recruitment at the short telomere, where elongation is needed. Finally we showed an up-regulation of TERRA, and telomerase RNA TLC1, accompanied by a predominant cytoplasmic localization as cell growth progresses from exponential growth to diauxic shift, and stationary phase. In these conditions, TERRA foci co-localize with TLC1 RNA foci, suggesting that the function of TERRA as a scaffold molecule to generate telomerase cluster is necessary for this yeast cell growth phases. / Les télomères à l’extrémité des chromosomes constituent une structure d’ADN et de protéines essentielle à l’intégrité de ces chromosomes. La télomérase est l’enzyme responsable du maintien des répétitions télomériques à l’extrémité des chromosomes. Cette enzyme est constituée d’une sous-unité catalytique, qui possède une activité de transcriptase réverse, et d’une sous-unité d’ARN, qui fourni la matrice nécessaire à la synthèse des répétitions télomériques. Les ARN contenant des répétions télomériques (ou Telomeric repeats-containing RNA; TERRA) constitue une nouvelle classe d’ARN non-codants transcrits à partir des télomères et conservée chez la plupart des eucaryotes. TERRA a été proposé d’agir comme un régulateur de l‘homéostasie des télomères et comme inhibiteur de la télomérase, mais sa fonction spécifique reste inconnue. De plus, chez la levure Saccharomyces cerevisiae, TERRA est rapidement dégradé par l’exonucléase 5’-3’ Rat1, ce qui complique l’étude de cet ARN par les méthodes biochimiques classiques. Dans cette thèse, nous rapportons l‘utilisation d’une approche cytologique pour étudier TERRA dans les cellules de levures. Deux approches sont utilisées : l’hybridation in situ en fluorescence (FISH) et l’étiquetage de TERRA à l’aide du système MS2-GFP, qui nous permet de visualiser l’expression de TERRA transcrit d’un seul télomère dans des cellules vivantes. Avec ces deux approches, nous observons que TERRA exprimé à partir d’un seul télomère s’accumule dans un faible nombre de cellules, sous la forme d’un focus périnucléaire. De plus, nous montrons que TERRA est exprimé lorsque son télomère raccourcit. Par immunoprécipitation, nous montrons que TERRA interagit in vivo avec l’ARN de la télomérase de levure, TLC1. L’élongation des télomères dépend de l‘action de multiples molécules de télomérase, qui sont visibles sous la forme de clusters de télomérases, qui s‘associent en phase S avec les télomères chez la levure et les cellules de mammifère. Nous démontrons que TERRA stimule la nucléation de ces clusters de télomérase. Par imagerie en temps réel de TERRA et de l’ARN TLC1, nous observons que TERRA agit comme molécule d’échafaudage pour générer des clusters de télomérases, qui sont par la suite recrutés, en phase S, au télomère duquel TERRA a été exprimé. Le recrutement d’un focus de TERRA à son télomère d’origine dépend des facteurs contrôlant le recrutement de la télomérase aux télomères : Mre11, Tel1 et le complexe yKu. Nous proposons qu’un télomère court exprime TERRA pour assembler et organiser les molécules de télomérase, afin que celles-ci soit puissent être recrutées au télomère court pour permettre son élongation. Enfin, nous observons une surexpression de l’ARN de la télomérase TLC1 et de TERRA, ainsi qu’une accumulation cytoplasmique de ceux-ci sous la forme de foci, lorsque la cellule passe de la phase de croissance exponentiel à la phase diauxique, puis à la phase stationnaire. Dans ces conditions, les foci d’ARN TLC1 colocalisent avec les foci de TERRA, suggérant que la fonction de TERRA comme molécule d’échafaudage pour générer des foci de télomérase est aussi nécessaire durant ces phases du cycle de croissance des levures.

Telomeric repeats-containing RNA (TERRA)

Telomere

Telomerase

ARN non-codant

Saccharomyces cerevisiae

Localisation cellulaire

Microscopie

MS2-GFP

Imagerie en cellule vivante

Croissance cellulaire

Non-coding RNA

Microscopy

Live cell imaging

Cellular localization

Logarithmic growth

Diauxic shift

Stationary phase

MECHANISMS OF TRINUCLEOTIDE REPEAT INSTABILITY DURING DNA SYNTHESIS

Chan, Kara Y.

01 January 2019

Genomic instability, in the form of gene mutations, insertions/deletions, and gene amplifications, is one of the hallmarks in many types of cancers and other inheritable genetic disorders. Trinucleotide repeat (TNR) disorders, such as Huntington’s disease (HD) and Myotonic dystrophy (DM) can be inherited and repeats may be extended through subsequent generations. However, it is not clear how the CAG repeats expand through generations in HD. Two possible repeat expansion mechanisms include: 1) polymerase mediated repeat extension; 2) persistent TNR hairpin structure formation persisting in the genome resulting in expansion after subsequent cell division. Recent in vitro studies suggested that a family A translesion polymerase, polymerase θ (Polθ), was able to synthesize DNA larger than the template DNA. Clinical and in vivo studies showed either overexpression or knock down of Polθ caused poor survival in breast cancer patients and genomic instability. However, the role of Polθ in TNR expansion remains unelucidated. Therefore, we hypothesize that Polθ can directly cause TNR expansion during DNA synthesis. The investigation of the functional properties of Polθ during DNA replication and TNR synthesis will provide insight for the mechanism of TNR expansion through generations.

DNA Translesion Polymerase-Polymerase θ

Base Excision Repair

Hairpin Bypass Synthesis

Mn2+/Mg2+

Trinucleotide Repeats Expansion

Huntington’s Disease

Biochemistry

Cell Biology

Genetic Processes

Genetics

Laboratory and Basic Science Research

Medical Genetics

Molecular Biology

Molecular Genetics

Nervous System Diseases

Signal processing for biologically-inspired gradient source localization and DNA sequence analysis

Rosen, Gail L.

12 July 2006

Biological signal processing can help us gain knowledge about biological complexity, as well as using this knowledge to engineer better systems. Three areas are identified as critical to understanding biology: 1) understanding DNA, 2) examining the overall biological function and 3) evaluating these systems in environmental (ie: turbulent) conditions. DNA is investigated for coding structure and redundancy, and a new tandem repeat region, an indicator of a neurodegenerative disease, is discovered. The linear algebraic framework can be used for further analysis and techniques. The work illustrates how signal processing is a tool to reverse engineer biological systems, and how our better understanding of biology can improve engineering designs. Then, the way a single-cell mobilizes in response to a chemical gradient, known as chemotaxis, is examined. Inspiration from receptor clustering in chemotaxis combined with a Hebbian learning method is shown to improve a gradient-source (chemical/thermal) localization algorithm. The algorithm is implemented, and its performance is evaluated in diffusive and turbulent environments. We then show that sensor cross-correlation can be used in solving chemical localization in difficult turbulent scenarios. This leads into future techniques which can be designed for gradient source tracking. These techniques pave the way for use of biologically-inspired sensor networks in chemical localization.

DNA analysis

Ficks second law

Hebbian learning

Biased random walk

Sensor cross-correlation

Delay-and-Sum beamforming

Turbulent plumes

Electronic nose

Tandem repeats

Gradient sensing

Bacterial chemotaxis navigation

Chemotaxis

Biologically-inspired computing

Signal processing

Sensor networks

Nucleotide sequence

Nervous system Degeneration

Chemotaxis

Towards Control of Dutch Elm Disease: dsRNAs and the Regulation of Gene Expression in Ophiostoma novo-ulmi / dsRNAs and the Regulation of Gene Expression in Ophiostoma novo-ulmi

Carneiro, Joyce Silva

01 August 2013

Ophiostoma novo-ulmi is the causal agent of Dutch elm disease (DED) which has had a severe impact on the urban landscape in Canada. This research program focused on developing molecular genetic strategies to control this pathogenic fungus. The first strategy involved the development of RNA interference (RNAi) for the down-regulation of genes involved in pathogenicity. An efficient RNAi cassette was developed to suppress the expression of the endopolygalacturonase (epg1) locus which encodes a cell-wall degrading enzyme. This epg1-RNAi cassette significantly reduced the amount of polygalacturonase activity in the fungus and resulted in almost complete degradation of epg1 mRNA. The need for a native promoter to selectively down-regulate specific gene loci was addressed by developing a carbon-catabolite regulated promoter (alcA) to drive the expression of the epg1-RNAi cassette. The expression of an alcA-driven epg1-RNAi cassette resulted in the down-regulation of epg expression under glucose starvation but normal levels of expression in high glucose. The expression could therefore be controlled by culture conditions. The second strategy explored the potential of using dsRNA viruses to vector disruptive RNAi cassettes. An isolate of O. novo-ulmi strain 93-1224 collected in the city of Winnipeg, was infected by two dsRNA mitoviruses which upon sequence characterization were named OnuMV1c and OnuMV7. To assess the transmissibility of this dsRNA virus the infected isolate 93-1224 was paired with three naive isolates of the related fungi O. ulmi and O. himal-ulmi. Through the use of nuclear and mitochondrial markers it was determined that the virus OnuMV1c may not rely on mitochondrial fusion for transmission but may have a cytoplasmic transmission route. This investigation of gene expression and manipulation has provided tools to help understand gene regulation in O. novo-ulmi. It has also added to our knowledge of mitoviruses, their transmission and potential use as a biological control. By enhancing our understanding of transmissible hypovirulence this work contributes to efforts to develop a new approach to target DED as well as a potential model for the control of other fungal diseases. / Graduate / 0307 / 0306 / 0369 / jscarneiro@hotmail.com

Ophiostoma novo-ulm

Dutch elm disease (DED)

RNA interference

Polygalacturonase

Alcohol dehydrogenase promoter

Gene expression

Phytopathogen

Cell wall degrading enzymes

Pectin enzyme

Mitoviruses

Pathogenicity

Virulence

Double-stranded RNA (dsRNA)

hyphal anastomosis

group I and II introns

Homing Endonuclease Genes (HEGs)

Single Sequence Repeats (SSRs)

Genetics of Russian wheat aphid (Diuraphis noxia) resistance in bread wheat (Triticum aestivum L.) accession CItr 2401

Sikhakhane, Thandeka Nokuthula

01 1900

The Russian wheat aphid (RWA) (Diuraphis noxia Kurdjumov) is one of the important insect pests of wheat (Triticum aestivum L.), barley (Hordeum vulgare L.) and other grasses. To date, there are four RWA biotypes identified in South Africa. The virulent biotypes emerged, partly due to climate change and new genetic variations within populations of RWA; hence there is a need to improve host-plant resistance, as an effective control measure. Bread wheat (Triticum aestivum L.) accession Cereal Introduction (CItr) 2401 is known to be resistant to all RWA biotypes worldwide. The goal of this study was to use a backcrossed near-isogenic line (NIL) BC5F5 mapping population, developed from a cross between CItr 2401 and susceptible Kavkaz, to identify and validate single nucleotide polymorphism (SNP) markers linked to the resistance phenotype in CItr 2401. This was achieved by (i) conducting a preliminary study that evaluated the suitability of simple sequence repeat (SSR) markers previously reported in literature for discriminating stacked RWA resistance genes and, (ii) employing SNP markers for the first time in a RWA resistance study as a future alternative to the widely used SSR markers. None of the tested SSR markers showed potential use in marker-assisted selection (MAS). The mapping population was phenotypically evaluated for RWA resistance using the four South African biotypes, viz. RWASA1, RWASA2, RWASA3 and RWASA4. Analysis of variance (ANOVA) showed significant (P<0.001) differences of genotypes after confirming the normality of residuals and homogeneity of variance. The Illumina iSelect 9,000 wheat SNP platform was used to genotype the two crossing parents and a selection of 24 NIL genotypes from the mapping population. Eight SNP markers found to be linked to the phenotype were converted to breeder-friendly and high-throughput Kompetitive allele-specific polymerase chain reaction (KASP) markers. The designed KASP markers were validated on the two crossing parents, the 24 NIL sent for SNP genotyping, on the mapping population and on the preliminary study genotypes for their effectiveness. The KASP assays developed in this study will be useful for stacking the RWA resistance from CItr 2401 with other Dn genes effective against the RWA. / Life and Consumer Sciences / M. Sc. (Life Sciences)

Gene stacking

Genotyping

KASP assay

Linkage mapping

Resistance

Russian wheat aphid

Sequencing

Simple sequence repeats

Single nucleotide polymorphism

Wheat

633.119752

Plant molecular genetics -- South Africa

Validation à grande échelle d'un modèle de simulation pour déterminer la fréquence des haplotypes Y dans la population canadienne-française

Landry, Roxane

January 2020

No description available.

UQTR Biologie cellulaire et moléculaire

ADN humain

Agressions sexuelles

Chromosome Y

Code R

Données généalogiques

Évaluation de la preuve

Fréquence des haplotypes Y

Généalogie

Génétique des populations

Haplotype Y

Hétérogénéité spatiale

Microsatellite

Modèle de simulation

Population canadienne-française

Répétition en tandem court

Science forensique

Short-tandem repeats

Simulation de population

Valeur probante

Développement et caractérisation de modèles C. elegans pour la maladie de Machado-Joseph

Fard Ghassemi, Yasmin

06 1900

Les maladies à expansion de polyglutamine sont un ensemble de troubles neurodégénératives héréditaires se développant lorsqu’il y a répétitions de trinucléotides CAG dans les gènes causatifs au-delà d’un certain seuil. L’expansion des répétitions de trinucléotides CAG entraîne des désordres neurologiques héréditaires précoces, dont de multiples formes d’ataxie spinocérébelleuse (SCA). Parmi celles-ci, le type le plus commun et dominant est l’ataxie spinocérébelleuse de type 3 (SCA3), aussi connue sous le nom de la maladie de Machado-Joseph (MMJ). Ce dernier est un désordre neurologique progressif autosomique dominant. Le gène causatif de MMJ est ATXN3 (ATAXINE-3). Plusieurs études récentes suggèrent une association entre ce gène et la modulation du stress du réticulum endoplasmique (RE). Lors de ce travail de maîtrise, des souches transgéniques de C. elegans exprimant les formes sauvage et mutante du gène ATXN3 humain ont été générées. Les résultats suggèrent des phénotypes importants chez la souche transgénique mutante associés à la pathologie humaine: défaut de motilité, longévité réduite et profil neurodégénératif considérable. Ceci dit, ces résultats nous ont poussé à vouloir déterminer si l’utilisation des composés chimiques, connus en tant que modulateurs du stress du RE et possédant des rôles neuroprotecteurs, sont capables de restaurer les phénotypes notés. Les composés utilisés, c’est-à-dire le Bleu de Méthylène, le Salubrinal et le Guanabenz, ont démontré une capacité de corriger les phénotypes rapportés dans la souche transgénique mutante. De plus, ces composés ont aussi été en mesure de prévenir une augmentation du niveau du stress oxydatif et de la réponse au stress du RE exhibé chez les vers mutants. Par le développement de nouveaux modèles C. elegans pour la MMJ, où il y a expression du gène ATXN3 complet dans les motoneurones, il a été possible de trouver qu’une modulation chimique du stress du RE peut réduire considérablement la neurodégénérescence et par conséquent, être une possible nouvelle approche thérapeutique pour traiter cette pathologie. / Polyglutamine expansion diseases are a class of dominantly inherited neurodegenerative disorders that develop when a CAG repeat in the causative genes is unstably expanded above a certain threshold. The expansion of trinucleotide CAG repeats causes hereditary adult-onset neurodegenerative disorders such as multiple forms of spinocerebellar ataxia (SCA). The most common dominantly inherited spinocerebellar ataxia is the type 3 (SCA3) also known as Machado-Joseph disease (MJD), an autosomal dominant, progressive neurological disorder. The gene causing MJD is ATXN3 (ATAXIN-3): MJD is caused by an abnormal CAG trinucleotide repeat expansion in the ATXN3 gene. Several recent studies have shown that this gene is associated with endoplasmic reticulum (ER) stress. In this study, we generated transgenic C. elegans strains expressing wild type or mutant human ATXN3 genes and tested them for recovery of locomotor phenotype, lifespan and neurodegeneration phenotypes upon treatment with compounds known to modulate ER stress and having neuroprotective roles. We observed differences between both transgenic lines and found that the motility defects, the reduced lifespan and the neurodegeneration can be rescued by methylene blue, guanabenz and salubrinal. These compounds were also able to prevent the oxidative stress and the ER stress response induced by mutant transgenic worms. We introduce novel C. elegans models for MJD based on the expression of full-length ATXN3 in GABAergic motor neurons. Using these models we discovered that chemical modulation of the ER unfolded protein response reduced neurodegeneration and could be a new therapeutic approach for the treatment of MJD.

Maladie à expansion de polyglutamine

Répétitions de trinucléotides

MMJ

Désordre neurologique

ATXN3

C. elegans

Défaut de motilité

Longévité

Motoneurones

Neurodégénérescence

Stress oxydatif

Stress du RE

Composés neuroprotecteurs

Modulateurs du stress du RE

Polyglutamine expansion diseases

MJD

Trinucleotide repeats

Neurological disorder

ATXN3

C. elegans

Motility defects

Lifespan

Motor neurons

Neurodegeneration

Oxidative stress,

ER stress

Neuroprotective compounds

ER stress modulators