Identification and functional analysis of single nucleotide polymorphisms that affect human cancer

Grochola, Lukasz Filip

January 2011

Aims: The p53 regulatory network is crucial in directing the suppression of cancer formation and mediating the response to commonly used cancer therapies. Functional genetic variants in the genes comprising this network could help identify individuals at greater risk for cancer and patients with poorer responses to therapies, but few such variants have been identified as yet. Methods: We first develop and apply three different screens that utilize known characteristics of functional single nucleotide polymorphisms (SNPs) in the p53 network to search for variants that associate with allelic differences in (i) recent natural selection, (ii) chemosensitivity profiles, and (iii) the gender- and age- dependent incidence of soft-tissue sarcoma. Secondly, we study and explore the functional mechanisms associated with the identified variants. Results: We identify SNPs in the PPP2R5E, CD44, YWHAQ and ESR1 genes that associate with allelic differences in the age of tumour diagnosis (up to 32.5 years, p=0.031), cancer risk (up to 8.1 odds ratio, p=0.004) and overall survival (up to 2.85 relative risk, p=0.011) in sarcomas, ovarian and pancreatic cancers, and exhibit allelic differences in the cellular responses to cytotoxic chemotherapeutic agents (up to 5.4-fold, p=5.6x10^-47). Lastly, we identify candidate causal SNPs in those genes and describe the regulatory mechanisms by which they might affect human cancer. Conclusions: Together, our work suggests that the inherited genetics of the p53 pathway have a great potential to further define populations in their abilities to react to stress, suppress tumor formation and respond to therapies.

616.994071

Étude de facteurs génétiques prédictifs dans le neuroblastome, en particulier les anomalies du chromosmoe 14q

Arsenault, Marie-Pier

08 1900

Le neuroblastome (NB) représente 8% de tous les cancers pédiatriques et est caractérisé par sa grande hétérogénéité clinique. Afin d’évaluer son pronostic, plusieurs facteurs génétiques sont utilisés : amplification de MYCN, délétion 1p, gain 11q et gain 17q. Les buts de notre travail étaient d’abord de vérifier si l’hybridation in situ en fluorescence (FISH) permet une analyse complète de ces anomalies et ensuite, en utilisant une analyse globale du génome telle le polymorphisme nucléotidique simple (SNP), de vérifier la concordance avec les résultats de la FISH et le pronostic potentiel des anomalies du 14q, en particulier du gène AKT. Nous avons donc établi un panel de sondes pour la FISH qui a été appliqué sur 16 tumeurs non-fixées. Après isolation de l’ADN de 36 tumeurs, nous avons effectué une analyse génotypique par SNP utilisant les puces « Affymetrix Genome-Wide Human SNP Array 6.0 » contenant 945,826 sondes non polymorphiques et 906,000 sondes polymorphiques. Nos résultats ont démontré que la FISH permet l’évaluation complète des anomalies génétiques importantes du NB et que les anomalies déséquilibrées sont détectées très précisément par SNP. Les anomalies du 14q tendent à être associées avec des facteurs cliniques comme le grade et l’évolution, contrairement aux anomalies d’AKT. L’analyse du 14q a révélé trois gènes d’intérêt, MAX, BCL11B et GPHN, qui devraient être analysés sur un plus grand échantillon. Ainsi, l’étude par FISH semble adaptée pour détecter les anomalies génétiques classiques du NB, alors que celles retrouvées en 14q représentent de potentielles cibles thérapeutiques pour cette tumeur. / Neuroblastoma (NB) accounts for 8% of all childhood cancers and is characterized by its clinical heterogeneity. To evaluate its prognostic, many genetic markers are used: MYCN amplification, 1p deletion, 11q gain and 17q gain. Our goals were first to verify if fluorescence in situ hybridization (FISH) allows a complete analysis of these abnormalities and, second, using a global genomic analysis as single nucleotide polymorphism (SNP), to verify the concordance with FISH results and the prognostic potential of 14q abnormalities, especially these of AKT gene. We then established a FISH panel that has been applied on 16 unfixed tumors. After DNA isolation of 36 tumors, we made a genotypic analysis by SNP using « Affymetrix Genome-Wide Human SNP Array 6.0 » containing 945,826 nonpolymorphic probes and 906,000 polymorphic probes. Our results have demonstrated that FISH allows a complete evaluation of the NB’s important genetic abnormalities and that unbalanced abnormalities are detected very precisely by SNP. 14q abnormalities seem to be associated with clinical factors such as tumor grading and evolution, unlike AKT abnormalities. Analysis of 14q abnormalities revealed three genes of interest, MAX, BCL11B and GPHN, which should be analyzed on a larger sample. Thereby, FISH study seems appropriate to detect the NB’s classic genetic abnormalities, while those found in 14q represent potential therapeutic targets for this tumor.

Neuroblastome

Neuroblastoma

FISH

SNP

14q

AKT

Aquaculture genomics, genetics and breeding in the United States: current status, challenges, and priorities for future research

Abdelrahman, Hisham, ElHady, Mohamed, Alcivar-Warren, Acacia, Allen, Standish, Al-Tobasei, Rafet, Bao, Lisui, Beck, Ben, Blackburn, Harvey, Bosworth, Brian, Buchanan, John, Chappell, Jesse, Daniels, William, Dong, Sheng, Dunham, Rex, Durland, Evan, Elaswad, Ahmed, Gomez-Chiarri, Marta, Gosh, Kamal, Guo, Ximing, Hackett, Perry, Hanson, Terry, Hedgecock, Dennis, Howard, Tiffany, Holland, Leigh, Jackson, Molly, Jin, Yulin, Khalil, Karim, Kocher, Thomas, Leeds, Tim, Li, Ning, Lindsey, Lauren, Liu, Shikai, Liu, Zhanjiang, Martin, Kyle, Novriadi, Romi, Odin, Ramjie, Palti, Yniv, Peatman, Eric, Proestou, Dina, Qin, Guyu, Reading, Benjamin, Rexroad, Caird, Roberts, Steven, Salem, Mohamed, Severin, Andrew, Shi, Huitong, Shoemaker, Craig, Stiles, Sheila, Tan, Suxu, Tang, Kathy F. J., Thongda, Wilawan, Tiersch, Terrence, Tomasso, Joseph, Prabowo, Wendy Tri, Vallejo, Roger, van der Steen, Hein, Vo, Khoi, Waldbieser, Geoff, Wang, Hanping, Wang, Xiaozhu, Xiang, Jianhai, Yang, Yujia, Yant, Roger, Yuan, Zihao, Zeng, Qifan, Zhou, Tao

20 February 2017

Advancing the production efficiency and profitability of aquaculture is dependent upon the ability to utilize a diverse array of genetic resources. The ultimate goals of aquaculture genomics, genetics and breeding research are to enhance aquaculture production efficiency, sustainability, product quality, and profitability in support of the commercial sector and for the benefit of consumers. In order to achieve these goals, it is important to understand the genomic structure and organization of aquaculture species, and their genomic and phenomic variations, as well as the genetic basis of traits and their interrelationships. In addition, it is also important to understand the mechanisms of regulation and evolutionary conservation at the levels of genome, transcriptome, proteome, epigenome, and systems biology. With genomic information and information between the genomes and phenomes, technologies for marker/causal mutation-assisted selection, genome selection, and genome editing can be developed for applications in aquaculture. A set of genomic tools and resources must be made available including reference genome sequences and their annotations (including coding and non-coding regulatory elements), genome-wide polymorphic markers, efficient genotyping platforms, high-density and high-resolution linkage maps, and transcriptome resources including non-coding transcripts. Genomic and genetic control of important performance and production traits, such as disease resistance, feed conversion efficiency, growth rate, processing yield, behaviour, reproductive characteristics, and tolerance to environmental stressors like low dissolved oxygen, high or low water temperature and salinity, must be understood. QTL need to be identified, validated across strains, lines and populations, and their mechanisms of control understood. Causal gene(s) need to be identified. Genetic and epigenetic regulation of important aquaculture traits need to be determined, and technologies for marker-assisted selection, causal gene/mutation-assisted selection, genome selection, and genome editing using CRISPR and other technologies must be developed, demonstrated with applicability, and application to aquaculture industries. Major progress has been made in aquaculture genomics for dozens of fish and shellfish species including the development of genetic linkage maps, physical maps, microarrays, single nucleotide polymorphism (SNP) arrays, transcriptome databases and various stages of genome reference sequences. This paper provides a general review of the current status, challenges and future research needs of aquaculture genomics, genetics, and breeding, with a focus on major aquaculture species in the United States: catfish, rainbow trout, Atlantic salmon, tilapia, striped bass, oysters, and shrimp. While the overall research priorities and the practical goals are similar across various aquaculture species, the current status in each species should dictate the next priority areas within the species. This paper is an output of the USDA Workshop for Aquaculture Genomics, Genetics, and Breeding held in late March 2016 in Auburn, Alabama, with participants from all parts of the United States.

Aquaculture

Genetic resources

Genome

Transcriptome

QTL

RNA-Seq

SNP

Fish

Shellfish

FUNCTIONAL AND BIOCHEMICAL CONSEQUENCES OF SINGLE NUCLEOTIDE POLYMORPHISMS IN THE HUMAN VESICULAR MONOAMINE TRANSPORTER 1 GENE (SLC18A1) By Sally Gamal Shukry, B.S.

Shukry, Sally Gamal

02 May 2012

Abstract FUNCTIONAL AND BIOCHEMICAL CONSEQUENCES OF SINGLE NUCLEOTIDE POLYMORPHISMS IN THE HUMAN VESICULAR MONOAMINE TRANSPORTER 1 GENE (SLC18A1) By Sally Gamal Shukry, B.S. A thesis submitted in partial fulfillment of the requirements for the degree of Master of Science in Biology at Virginia Commonwealth University. Virginia Commonwealth University, 2012 Major Advisor: Jennifer K. Stewart Associate Professor and Graduate Director, Department of Biology Single nucleotide polymorphisms (SNP) in the human VMAT1 gene (SLC18A1) have been associated with schizophrenia in three different populations: Han Chinese, Western European and Japanese. Effects of these mutations on transport function of the hVMAT1 protein have not been reported. The goal of this study was to investigate functional and biochemical differences in human VMAT1 proteins with a threonine or proline at amino acid position 4 (Thr4Pro) and a serine or threonine at position 98 (Ser98Thr). COS1 cells were transfected with variant SNPs coding for 4Thr/98Ser, 4Pro/98Ser, or 4Thr98Thr. Western blotting demonstrated robust over expression of the genes and no differences in electrophoretic mobility of the proteins. Maximal transport of serotonin by the VMAT1 protein with 4Pro/98Ser was less than that of the 4Thr/98Ser or the 4Thr/98Thr. Response of the 4Pro/Ser98 to the VMAT inhibitor reserpine was lower than that of the 4Thr/98Thr. These findings suggest mechanisms for human VMAT1 links to schizophrenia.

SNP

VMAT1

SLC18A1

Vesicular Monoamine Transporter 1

Single Nucleotide Polymorphisms

Schizophrenia

Bipolar Disorder

Biology

Life Sciences

Y chromosomální charakteristika současné vesnické populace na Klatovsku / Y Chromosomal Characteristics of the Modern Rural Population in Klatovy Region

Doležalová, Veronika

January 2015

Usage of genetic markers in non-recombining part of chromosome Y has been shown as a eligible tool for a study of history, diversity and migration of population. Applicable markers of chromosome Y are SNP and STR polymorphisms. There were collected 53 unique samples of DNA as a object of this work from unrelated origin males from 9 villages around Klatovy. Samples have been analyzed and its values have been determined by using the 17 STR markers by AmpFLSTR® Yfiler® Direct Kit. In total I have observed 7 different haplogroups. I have resulted samples from villages around Klatovy and they were analyzed by AMOVA. I have compared samples with the surrounding populations in neighborly Federal Republic of Germany, Austria, Central and South Bohemia. There were no significant differences founded in the genetic profile of this population to the surrounding populations.

Studium interakcí vybraných anthokyanidinů s farnesoidním X receptorem / Interaction of selected anthocyanidins with farnesoid X receptor

Jeřábková, Jana

January 2013

Charles University in Prague Faculty of Pharmacy in Hradec Králové Department of Pharmacology & Toxicology Student: Jana Jeřábková Supervisor: Doc. PharmDr. Petr Pávek, Ph.D. Title of diploma thesis: Interaction of selected anthocyanidins with farnesoid X receptor Human farnesoid X receptor (FXR) is a member of nuclear receptor superfamily that act as ligand-activated transcription factors. FXR binds to specific regulatory DNA regions and induces expression of many target genes. These regulated genes are involved in bile acid metabolism and transport, maintaining blood lipids, liporoteins and glucose homeostasis and also contribute to maintain intestinal bacterial balance, hepatoprotection and liver regeneration. The interest of recent studies is to test the range of FXR ligands for treatment and prevention of many diseases such as cholestais, cholesterol gallstone disease, steato-hepatitis, dyslipidemia, atherosclerosis, type 2 diabetes mellitus, metabolic syndrome, liver cancer and other forms of cancer such as breast cancer. In this experimental diploma thesis we are focused on testing of potencial ligands of human farnesoid X receptor from the group of natural plant pigments anthocyanidins (cyanidin, delphinidin, malvidin, pelargonidin, peonidin and petunidin) using the human hepatoma cell line...

Interaktion zwischen dem humanen Cytomegalievirus, Aspergillus fumigatus, dendritischen Zellen und neutrophilen Granulozyten / Interaction of the human cytomegalovirus, Aspergillus fumigatus, dendritic cells and polymorphonuclear neutrophils

Mezger, Markus

January 2007

Immunsupprimierte Patienten besitzen ein erhöhtes Risiko für opportunistische Infektionen, die hauptsächlich durch das humane Cytomegalievirus (HCMV) und den Schimmelpilz Aspergillus fumigatus verursacht werden. Aufgrund ihrer Lokalisation in den Geweben unterhalb von Lungenepithelien und des Gastrointestinaltraktes werden dendritische Zellen (DCs) als diejenigen Zellen betrachtet, die während der frühen Phase einer Infektion in Kontakt mit HCMV und A. fumigatus kommen und eine Aktivierung von angeborenen und adaptiven Abwehrmechanismen vermitteln. Im Rahmen der vorliegenden Dissertation wurde die Bedeutung von humanen DCs bei der Bekämpfung von HCMV und A. fumigatus näher untersucht. Um mit dem klinisch relevanten HCMV Stamm TB40E arbeiten zu können, musste zuerst ein geeignetes Zellkultursystem zur Anzucht von HCMV etabliert werden. Die aus Fibroblasten aufgereinigten Viren eigneten sich zur erfolgreichen Infektion von DCs, was durch verschiedene Färbemethoden nachgewiesen werden konnte. Aus diesem Grund war es möglich, in Abhängigkeit der Zeit ein Expressionsprofil von Klasse I Interferonen (IFN-alpha, IFN-beta), ausgesuchten Cytokinen (CXCL10, CXCL11, Rantes) und den wichtigen Immunrezeptoren Toll-like Rezeptor 3 (TLR3) und dendritic cell-specific ICAM3-grabbing nonintegrin (DC-SIGN) zu erstellen. Nachdem ein RNA Interferenz (RNAi) System zur erfolgreichen Transfektion von DCs mit small interfering RNA (siRNA) etabliert werden konnte, gelang es die Expression von TLR3 signifikant herunterzuregulieren. Stimulationsexperimente mit dem synthetisch hergestellten Polymer poly I:C identifizierten TLR3 als den Rezeptor, der die Expression von IFN-beta vermittelt. Ferner konnte nachgewiesen werden, dass TLR9 bei ex vivo generierten DCs keine Funktion besitzt. Eine direkte Aktivierung von TLR3 durch HCMV konnte mittels siRNA nicht nachgewiesen werden. Durch den Einsatz von genomweiten Microarray-Analysen konnten eine Vielzahl an Genen gefunden werden, die nach Co-Kultivierung von DCs und lebenden A. fumigatus Keimschläuchen (KS) differentiell exprimiert waren. Dabei wurde ein breites Spektrum an Cytokinen (TNF-alpha, IL-6, IL-10, IL-12), Chemokinen (IL-8, CCL20, CXCL10), Co-stimulatorischen Molekülen (CD40, CD80, CD83, CD86), Prostaglandin Synthese Genen (PTGS2) und Immunrezeptoren (PTX-3, TLR2, TLR4) gefunden, deren zeitabhängiges Expressionsprofil mittels qRT-PCR eindeutig bestätigt wurde. Als Wachen des Immunsystems müssen DCs Krankheitserreger zu einem frühen Zeitpunkt der Infektion erkennen. Die Erkennung von Pilzen wird durch die unterschiedlichen Rezeptoren vermittelt, die TLRs, C-Typ Lektine und Pentraxine umfassen, wobei ihre Bedeutung für humane DCs bisher nur unzureichend geklärt ist. Durch den Einsatz von siRNA konnte die Expression von TLR2, TLR4, myeloid differentiation primary response gene 88 (MyD88), DC-SIGN, Pentraxin-3 (PTX-3) und caspase recruitment domain family member 9 (Card-9) signifikant verringert werden. Für TLR2, TLR4, PTX-3 und DC-SIGN konnte durch den Einsatz der RNAi aufgezeigt werden, dass diese Rezeptoren nicht an der Induktion einer pro-inflammatorischen Immunantwort von DCs nach Infektion mit A. fumigatus beteiligt sind. Sowohl die Stimulierung mit den TLR Liganden Zymosan und LPS, als auch mit A. fumigatus, führte zu einer erhöhten Expression von TNF-alpha und IL-12 (Light Cycler), die sich in einer vermehrten Cytokinfreisetzung (ELISA) bemerkbar machte. Im Gegensatz zur TLR4 siRNA Transfektion und LPS-Stimulation war keine Reduktion der Expression von TNF-alpha und IL-12 nach TLR2 und TLR4 siRNA Transfektion und anschließender Pilzinfektion zu beobachten. Auch der Einsatz von gegen TLRs gerichteten Antikörpern konnte eine mögliche Signaltransduktion bei DCs nicht unterbinden. Anstelle von TLR2 und TLR4 wurde Dectin-1 als DC-Immunrezeptor für A. fumigatus KS identifiziert. Mit Hilfe eines spezifischen Antikörpers gegen Dectin-1 war es möglich, die Freisetzung von TNF-alpha und IL-12 nach Pilzinfektion zu blockieren. In einem unabhängigen Experiment mit siRNA wurde Dectin-1 als Rezeptor für A. fumigatus bestätigt. Wie fortführende Experimente mit Candida albicans KS und Zymosan gezeigt haben, handelt es sich bei Dectin-1 auf humanen DCs um einen generellen Rezeptor für Pilze. Die durchgeführten SNP-Analysen (single nucleotide polymorphism) zur Ermittlung eines Zusammenhanges mit einem erhöhten Virus- und Pilzinfektionsrisiko für Patienten nach Stammzelltransplantation erbrachten die Erkenntnis darüber, dass zwei Marker (rs735240, rs2287886) in DC-SIGN mit einer erhöhten Empfänglichkeit für HCMV, und drei Marker (rs1554013, rs3921, rs4257674) in CXCL10 mit einem vergrößerten Riskio für eine invasive Aspergillose assoziiert waren. Ein Screening von Patienten auf das Vorhandensein dieser definierten SNPs könnte helfen, die individuelle Gefahr für HCMV und A. fumigatus nach nach allogener Stammzelltransplantation abzuschätzen. / Patients after allogenic stem cell transplantation (alloSCT) have an increased risk to suffer from viral and fungal infections, which are mainly caused by the human cytomegalovirus (HCMV) and the mold Aspergillus fumigatus. Due to their localization in tissues under lung epithelia and the gastrointestinal tract, dendritic cells (DCs) are considered to be the first cells coming into close contact with HCMV and A. fumigatus for the activation of innate and adaptive immune mechanisms. Within the scope of this dissertation, the role of human monocyte-derived DCs in the abatement of HCMV and A. fumgatus was analyzed. In order to work with HCMV, a cell culture system for effective culturing of the clinical relevant HCMV strain TB40E had to be established first. The viral particles up-cleaned from lung fibroblasts were used for infection of DCs and successful infection was approved by different staining methods. For this reason, it was possible to determine a time-dependent expression profile of class I interferons (IFN-alpha, IFN-beta), selected cytokines (CXCL10, CXCL11, Rantes) and immunoreceptors (TLR3, DC-SIGN). A RNA interference (RNAi) system for human DCs was established to significantly knock-down expression of TLR3 without the induction of an unwanted pro-inflammatory cytokine response. Stimulation experiments with the synthetic polymer poly I:C (which resembles dsRNA of infectious viruses) identified TLR3 as a receptor for triggering expression of IFN-beta. However, whether there is a direct activation of TLR3 through dsRNA intermediates, possibly emerging during replication of HCMV, can not be answered to date definitively, because TLR3 small interfering RNA (siRNA) transfection prior to HCMV infection did not result in minor expression of IFN-beta. Gene expression pattern of DCs after co-cultivation with living A. fumigatus germ tubes was studied by whole genome microarray analysis and real-time PCR, demonstrating an upregulation of a broad spectrum of cytokines (TNF-alpha, IL-6, IL-10, IL-12), chemokines (IL-8, CCL20, CXCL10), co-stimulatory molecules (CD40, CD80, CD83, CD86), prostaglandin synthesis genes (PTGS2), as well as genes involved in fungal recognition (PTX-3, TLR2, TLR4) and cytoskeleton organization / phagocytosis. As the sentries of the immune system, DCs must recognize fungi at an early step of infection. Pathogen detection is mediated by different receptors comprising TLRs, C-type lectins and Pentraxines (PTX), but only little is known about their relevance for DCs. Using specific siRNAs, expression of TLR2, TLR4, myeloid differentiation primary response gene 88 (MyD88), dendritic cell-specific ICAM3-grabbing nonintegrin (DC-SIGN), Pentraxin-3 (PTX-3) and caspase recruitment domain family member 9 (Card-9) was significantly diminished, respectively. In contrast to control experiments with TLR4 siRNA and LPS stimulation, A. fumigatus induced expression of pro-inflammatory cytokines (TNF-alpha, IL-12) was not reduced when TLR2 and TLR4 expression was knocked-down by specific siRNAs prior to infection. However, using siRNAs directed against Dectin-1 allowed demonstration of an interaction between Dectin-1 and A. fumigatus germlings, Candida albicans germ tubes and Zymosan. In an independent approach, cytokine secretion could be blocked by anti-Dectin-1 antibody treatement prior to fungal exposure. In conclusion, Dectin-1 was identified as an important fungal receptor on DCs whereas TLR2 and TLR4 seemed to play a negligible role. Single nucleotide polymorphisms (SNPs) in various cellular receptor genes are associated with the susceptibility to and severity of infectious diseases. In this study, genetic polymorphisms in genes encoding for virus entry receptors have been analyzed for their association to HCMV reactivation and disease in patients after allogeneic stem cell transplantation. A comparison of different genotyping methods highlighted the advantages of the Light Cycler system, the cycle-suequencing and the matrix-assisted laser desorption ionization mass spectrometry (MALDI-MS) when using small quantities of patients’ DNA. Two markers (rs735240, rs2287886) in the promoter region of DC-SIGN were found to be significantly associated with an increased susceptibility to HCMV. In addition, three SNPs (rs1554013, rs3921, rs4257674) in CXCL10 elevated the risk for the development of invasive aspergillosis. Screening of patients after alloSCT for the presence of these defined genetic polymorphisms may help to predict the individual risk to suffer from HCMV and A. fumigatus after alloSCT.

Aspergillus fumigatus

Cytomegalie-Virus

Dendritische Zelle

Granulozyt

SNP

Microarray

Toll-like-Rezeptoren

RNS-Interferenz

ddc:500

Haplotypenbasierte Assoziationsanalyse der COMT-Gen-Region bei schizophrenen Psychosen in einem polydiagnostischen Ansatz / Haplotype based association analysis of the COMT locus further supports a complex genetic interaction with schizophrenic psychoses

Putz, Evelyn

January 2008

In den vergangenen Jahren wurde vermehrt das Gen, welches für Catechol-O-Methyltransferase codiert, als starker Kandidat für ein erhöhtes Schizophrenierisiko diskutiert. Grund dafür ist die zentrale Rolle der Catechol-O-Methyltransferase beim Katecholaminabbau im menschlichen präfrontalen Cortex. Aufgrund der zunehmend akzeptierten Tatsache, daß die singuläre Betrachtung einzelner Marker bei der komplexen genetischen Textur von Kandidatengenen nur wenig zur Erhellung komplexer Erkrankungen beizutragen vermag (Licinio, 2003), untersuchten wir neben dem Val108/158Met-Polymorphismus (rs4680) vier weitere, die COMT-Gen-Region umspannende SNPs (rs2097603, rs740603, rs4818, rs165599) an einer Stichprobe von 459 Schizophrenen und 150 Kontrollpersonen. Zwar ergab sich für den Marker rs740603 auf Intron 1 eine signifikante Allel- (p = 0.0060) und Genotypassoziation (p = 0.019), der funktionelle Val108/158Met-Polymorphismus (rs4680) zeigte aber keinen signifikanten Zusammenhang mit der Erkrankung. Zudem fand sich in unserer Haplotypanalyse keine Markerkombination, die in überdurchschnittlichem Zusammenhang mit schizophrenen Psychosen stand. Für die Untergruppe der zykloiden Psychosen ließ sich bei einem p-Wert von 0.031 eine 4-Marker-Kombination ermitteln, die die SNPs rs740603, rs4818, rs4680 und rs165599 einschliesst und die Region von Intron 1 bis 3´-UTR umspannt. Zusätzlich ergab sich in der Subgruppe der zykloiden Psychosen ein geschlechtsspezifischer Effekt im Sinne eines signifikanten 3-Marker-Haplotypen (rs4818-rs4680-rs165599) (p = .0044) in der Gruppe der Frauen (n = 27) mit rs165599 als stärkstem Einzelmarker. Aufgrund des komplexen genetischen Zusammenhangs zwischen den untersuchten Markern und der Erkrankung sollte auch in der zukünftigen Forschung eine differenzierte Betrachtung der verschiedenen schizophrenen Zustandsbilder angestrebt werden, wie dies die Klassifikation nach Leonhard ermöglicht. Neben gewebsspezifischen Transkriptionsfaktoren könnten auch epigenetische Faktoren, wie die Cytosinmethylierung von CpG-Stellen in promotorregulierenden Regionen, einen Erklärungsansatz für die Entstehung schizophrener Störungsbilder darstellen. / Since several years, the gene encoding catechol-O-methyltransferase (COMT) at chromosome 22q11 is discussed as a strong candidate for schizophrenia susceptibility due to its key function in degredation of catecholamines in the prefrontal cortex, a critical region of the human brain, involved in cognitive control processes, monitoring of information in working memory and in active judgments on information (Petrides, 2005). To test the association of the COMT gene locus with schizophrenia, we analysed five SNPs (rs2097603, rs740603, rs4818, rs4680, rs165599) spanning from the P2 promotor region (MB-COMT) to the 3´-UTR in 459 index cases, which fulfilled diagnistic criteria of schizophrenia according to DSM IV as well as 150 blood donors as population controls. According to differentiated psychopathology (Leonhard, 1999) probands were categorized into cycloid psychosis, unsystematic schizophrenia and systematic schizophrenia prior to genotyping. In intron 1 the marker rs740603 showed significant allele (p = 0.0060) and genotype (p = 0.019) association, but the functional Val105/158Met variant (rs4680) failed significant association with disease. Considering COMT haplotypes none of the marker combinations showed evidence for an association with schizophrenia. In the subgroup of cycloid psychosis we found 4-locus marker combinations rs740603-rs4818-rs4680-rs165599 associated with disease at p-level 0.031, spanning a region from intron 1 to the 3´-UTR. In conclusion, the genetic interaction of COMT SNPs and haplotypes and schizophrenia susceptibility appears complex across different populations and psychopathological phenotypes. Particularly structures potentially involved in mRNA expression levels need further scrutiny.

Haplotyp

Gen

Kandidatengen

SNP

Assoziationsanalyse

Schizoaffektive Psychose

Leo

ddc:610

Mutationsanalyse der Gene KIAA0027/MLC1 und KIAA0767/DIP als Kandidatengene für die periodische Katatonie / Mutation analysis of the genes KIAA0027/MLC1 and KIAA0767/DIP as candidate genes for periodic catatonia

Kohlmann, Bernd

January 2008

In dieser Arbeit wurde die systematische Suche nach krankheitsassoziierten Genen bei periodischer Katatonie fortgeführt. Für diese Erkrankung war die klinische Abgrenzbarkeit und die familiäre Häufung signifikant und ließ aufgrund der vertikalen Transmission und dem Auftreten über mehrere Generationen und hinweg auf einen Hauptgeneffekt schließen. Nach der Durchführung von Kopplungs-Analysen kristallisierten sich zwei koppelnde Regionen auf den Chromosomen 15 und 22 heraus. Mittels Haplotypanalyse konnte der Genort auf Chromosom 22q13 auf einen knapp 5 Mbp großen Bereich eingeschränkt werden. Im kodierenden Bereich des MLC1-Genes segregierte im mit periodischer Katatonie assoziierten Haplotyp eine Variante (p.Leu309Met). Da Mutationen im MLC1-Gen bereits im Zusammenhang mit Megalenzephaler Leukoenzephalopathie beschrieben worden waren, wurden in dieser Arbeit zunächst fünf Patienten mit dieser Erkrankung auf Mutationen in kodierenden Bereichen von MLC1 systematisch untersucht. Daran schloss sich eine Analyse dieses Gens bei 140 Patienten mit periodischer Katatonie an. Ein Zusammenhang zwischen Mutationen in MLC1 und dem Auftreten von Megalenzephaler Leukoenzephalopathie wurde untermauert, wohingegen die Ergebnisse eindeutig gegen eine Assoziation mit periodischer Katatonie sprachen. Ein weiteres im Gehirn exprimiertes Kandidatengen (KIAA0767/DIP) wurde in dieser Arbeit untersucht. Dabei wurden sechs SNPs im exonnahen intronischen Bereich entdeckt sowie eine Variante im Exonbereich (p.Glu156Asn). Dies ist eine seltene Normvariante, eine Assoziation zur periodischen Katatonie wurde in einer Fall-Kontroll-Studie ausgeschlossen. Insgesamt wurde durch die systematische Mutationsanalyse die Kandidatenregion auf Chromosom 22q13.3 weiter eingeengt. Gegen einen Zusammenhang zwischen MLC1 und periodischer Katatonie sprechen die vorgestellten validen Ergebnisse. / The present dissertation has carried on the systematic screening for genes involved in periodic catatonia. The clinical definition and the familial clustering of this disorder were of statistical significance. Its vertical transmission and the occurrence across generations led to the conclusion of it being a major gene effect. Linkage scans discovered two linking regions on chromosome 15 and chromosome 22. Using haplotype analysis it was possible to restrict the candidate region on chromosome 22q13 to region of 5 Mbp. In the coding region of the MLC1 gene a variant (p.Leu309Met) segregated in the haplotype associated with periodic catatonia. As detailed descriptions of mutations in the MLC1 gene in connection with megalencephalic leucoencephalopathy already exist, for the present dissertation five patients with the aforesaid disorder were systematically screened for mutations in the coding regions of MLC1. This was followed by an analysis of the according gene in 140 patients with periodic catatonia, which substantiated a correlation between mutations in MLC1 and the occurrence of megalencephalic leucoencephalopathy, whereas the results definitely did not support an association with periodic catatonia. Additionally, a further brain-expressed candidate gene (KIAA0027/DIP) was screened in this dissertation discovering six single nucleotide polymorphisms in the intronic exon-near region and a variant in the exonic region (p.Glu156Asn). This is a rare normal variant, an association with periodic catatonia was excluded in a case-control study. Altogether the systematic mutation analysis enabled a further reduction of the candidate region on chromosome 22q13.3. The research results, which meet the criterion of validity, do not support a correlation between MLC1 and periodic catatonia.

Schizophrenie

Katatonie

SNP

Molekulargenetik

Genmutation

Polymorphismus

RFLP

Leuk

ddc:610

Genetická determinace a dědičnost kraniofaciálních znaků na základě vybraných lokusů DNA / Genetic determination and heredity of craniofacial traits based on specific DNA loci

Králíková, Kristýna

January 2018

Introduction: Genetic determination of human face is clearly visible in family members. The resemblance between monozygotic twins who are genetically identical is especially remarkable. So far the possibilities of reliable prediction of the complex morphology of facial traits on the basis of genome analysis and the ability to capture the variability of human facial morphology through genotype variability are highly limited. Complete genetic basis of the physiological variability of craniofacial traits remains more or less unknown. This master's thesis was created as a pilot study of the shared project of the Laboratory of 3D Imagining and Analytical Methods and the Laboratory of Molecular Anthropology on Department of Anthropology and Human Genetics. Material and Methods: The specimen collection is composed of DNA samples derived from 30 families (29 with 4 members, 1 with 5 members) who fulfilled required criteria. Nine single nucleotide polymorphisms were chosen based on the available information. Eight of them are linked to normal facial variability and one was chosen based on the assumed function of the gene where the polymorphism is located. There were two methods of genotyping: RFLP method with the use of restriction endonuclease and SNaPshot method. Morphological data were provided by the...