776 research outputs found

    TiBi-3D - a Guide through the World of Epigenetics

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    In the last two decades the study of changes in the genome function that are not induced by changes in DNA has consolidated a strong research field called ”epigenetics”. Chromatin state changes play an essential role in the regulation of transcription of many genes, thus controlling cell differentiation. A large part of these changes is due to histone modifications that alter the accessibility of the DNA. Current state of the art visualization methods for the analysis of epigenetic data sets are not suited to represent the relationship between the combinatorial pattern of histone modifications and their regulatory effects

    Comparative genomics of Meloidogyne haplanaria

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    Root-knot nematodes are a scientifically and agriculturally importantgroup of plant parasites. Genomic investigations into this group have proven difficult due to a complex genomic arrangement and recent inter-species hybridisations. Here we design and employ novel bioinformatic workflows to assemble the genomes of Meloidogyne species and perform phylogenomic analyses on them. We use Meloidogyne haplanaria -an emerging crop pest recently shown to be capable of breaking cultivated resistance -as a test organism. We assemble and annotate its genome for the first time andinfer itsposition in the Meloidogynephylogeny. This will inform future investigations into diagnostic and control methods, as well as investigations into the evolutionary history of the genus. The workflows themselves will provide accessible bioinformatic tools for the reproducible assembly and phylogenomic analysis of Meloidogynegenomes to the wider scientific community. Greater elucidation of the complex genomics of the Meloidogyne genus can grant insight into many biological processes, including hybridisation,parasitic adaptation and evolution in the absence of recombination, and the effect that different parthenogenetic sexual systems can have on genomic architecture

    Augmented reality device for first response scenarios

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    A prototype of a wearable computer system is proposed and implemented using commercial off-shelf components. The system is designed to allow the user to access location-specific information about an environment, and to provide capability for user tracking. Areas of applicability include primarily first response scenarios, with possible applications in maintenance or construction of buildings and other structures. Necessary preparation of the target environment prior to system\u27s deployment is limited to noninvasive labeling using optical fiducial markers. The system relies on computational vision methods for registration of labels and user position. With the system the user has access to on-demand information relevant to a particular real-world location. Team collaboration is assisted by user tracking and real-time visualizations of team member positions within the environment. The user interface and display methods are inspired by Augmented Reality1 (AR) techniques, incorporating a video-see-through Head Mounted Display (HMD) and fingerbending sensor glove.*. 1Augmented reality (AR) is a field of computer research which deals with the combination of real world and computer generated data. At present, most AR research is concerned with the use of live video imagery which is digitally processed and augmented by the addition of computer generated graphics. Advanced research includes the use of motion tracking data, fiducial marker recognition using machine vision, and the construction of controlled environments containing any number of sensors and actuators. (Source: Wikipedia) *This dissertation is a compound document (contains both a paper copy and a CD as part of the dissertation). The CD requires the following system requirements: Adobe Acrobat; Microsoft Office; Windows MediaPlayer or RealPlayer

    XenDB: Full length cDNA prediction and cross species mapping in Xenopus laevis

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    BACKGROUND: Research using the model system Xenopus laevis has provided critical insights into the mechanisms of early vertebrate development and cell biology. Large scale sequencing efforts have provided an increasingly important resource for researchers. To provide full advantage of the available sequence, we have analyzed 350,468 Xenopus laevis Expressed Sequence Tags (ESTs) both to identify full length protein encoding sequences and to develop a unique database system to support comparative approaches between X. laevis and other model systems. DESCRIPTION: Using a suffix array based clustering approach, we have identified 25,971 clusters and 40,877 singleton sequences. Generation of a consensus sequence for each cluster resulted in 31,353 tentative contig and 4,801 singleton sequences. Using both BLASTX and FASTY comparison to five model organisms and the NR protein database, more than 15,000 sequences are predicted to encode full length proteins and these have been matched to publicly available IMAGE clones when available. Each sequence has been compared to the KOG database and ~67% of the sequences have been assigned a putative functional category. Based on sequence homology to mouse and human, putative GO annotations have been determined. CONCLUSION: The results of the analysis have been stored in a publicly available database XenDB . A unique capability of the database is the ability to batch upload cross species queries to identify potential Xenopus homologues and their associated full length clones. Examples are provided including mapping of microarray results and application of 'in silico' analysis. The ability to quickly translate the results of various species into 'Xenopus-centric' information should greatly enhance comparative embryological approaches. Supplementary material can be found at

    Computational solutions for addressing heterogeneity in DNA methylation data

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    DNA methylation, a reversible epigenetic modification, has been implicated with various bi- ological processes including gene regulation. Due to the multitude of datasets available, it is a premier candidate for computational tool development, especially for investigating hetero- geneity within and across samples. We differentiate between three levels of heterogeneity in DNA methylation data: between-group, between-sample, and within-sample heterogeneity. Here, we separately address these three levels and present new computational approaches to quantify and systematically investigate heterogeneity. Epigenome-wide association studies relate a DNA methylation aberration to a phenotype and therefore address between-group heterogeneity. To facilitate such studies, which necessar- ily include data processing, exploratory data analysis, and differential analysis of DNA methy- lation, we extended the R-package RnBeads. We implemented novel methods for calculating the epigenetic age of individuals, novel imputation methods, and differential variability analysis. A use-case of the new features is presented using samples from Ewing sarcoma patients. As an important driver of epigenetic differences between phenotypes, we systematically investigated associations between donor genotypes and DNA methylation states in methylation quantitative trait loci (methQTL). To that end, we developed a novel computational framework –MAGAR– for determining statistically significant associations between genetic and epigenetic variations. We applied the new pipeline to samples obtained from sorted blood cells and complex bowel tissues of healthy individuals and found that tissue-specific and common methQTLs have dis- tinct genomic locations and biological properties. To investigate cell-type-specific DNA methylation profiles, which are the main drivers of within-group heterogeneity, computational deconvolution methods can be used to dissect DNA methylation patterns into latent methylation components. Deconvolution methods require pro- files of high technical quality and the identified components need to be biologically interpreted. We developed a computational pipeline to perform deconvolution of complex DNA methyla- tion data, which implements crucial data processing steps and facilitates result interpretation. We applied the protocol to lung adenocarcinoma samples and found indications of tumor in- filtration by immune cells and associations of the detected components with patient survival. Within-sample heterogeneity (WSH), i.e., heterogeneous DNA methylation patterns at a ge- nomic locus within a biological sample, is often neglected in epigenomic studies. We present the first systematic benchmark of scores quantifying WSH genome-wide using simulated and experimental data. Additionally, we created two novel scores that quantify DNA methyla- tion heterogeneity at single CpG resolution with improved robustness toward technical biases. WSH scores describe different types of WSH in simulated data, quantify differential hetero- geneity, and serve as a reliable estimator of tumor purity. Due to the broad availability of DNA methylation data, the levels of heterogeneity in DNA methylation data can be comprehensively investigated. We contribute novel computational frameworks for analyzing DNA methylation data with respect to different levels of hetero- geneity. We envision that this toolbox will be indispensible for understanding the functional implications of DNA methylation patterns in health and disease.DNA Methylierung ist eine reversible, epigenetische Modifikation, die mit verschiedenen biologischen Prozessen wie beispielsweise der Genregulation in Verbindung steht. Eine Vielzahl von DNA Methylierungsdatensätzen bildet die perfekte Grundlage zur Entwicklung von Softwareanwendungen, insbesondere um Heterogenität innerhalb und zwischen Proben zu beschreiben. Wir unterscheiden drei Ebenen von Heterogenität in DNA Methylierungsdaten: zwischen Gruppen, zwischen Proben und innerhalb einer Probe. Hier betrachten wir die drei Ebenen von Heterogenität in DNA Methylierungsdaten unabhängig voneinander und präsentieren neue Ansätze um die Heterogenität zu beschreiben und zu quantifizieren. Epigenomweite Assoziationsstudien verknüpfen eine DNA Methylierungsveränderung mit einem Phänotypen und beschreiben Heterogenität zwischen Gruppen. Um solche Studien, welche Datenprozessierung, sowie exploratorische und differentielle Datenanalyse beinhalten, zu vereinfachen haben wir die R-basierte Softwareanwendung RnBeads erweitert. Die Erweiterungen beinhalten neue Methoden, um das epigenetische Alter vorherzusagen, neue Schätzungsmethoden für fehlende Datenpunkte und eine differentielle Variabilitätsanalyse. Die Analyse von Ewing-Sarkom Patientendaten wurde als Anwendungsbeispiel für die neu entwickelten Methoden gewählt. Wir untersuchten Assoziationen zwischen Genotypen und DNA Methylierung von einzelnen CpGs, um sogenannte methylation quantitative trait loci (methQTL) zu definieren. Diese stellen einen wichtiger Faktor dar, der epigenetische Unterschiede zwischen Gruppen induziert. Hierzu entwickelten wir ein neues Softwarepaket (MAGAR), um statistisch signifikante Assoziationen zwischen genetischer und epigenetischer Variation zu identifizieren. Wir wendeten diese Pipeline auf Blutzelltypen und komplexe Biopsien von gesunden Individuen an und konnten gemeinsame und gewebespezifische methQTLs in verschiedenen Bereichen des Genoms lokalisieren, die mit unterschiedlichen biologischen Eigenschaften verknüpft sind. Die Hauptursache für Heterogenität innerhalb einer Gruppe sind zelltypspezifische DNA Methylierungsmuster. Um diese genauer zu untersuchen kann Dekonvolutionssoftware die DNA Methylierungsmatrix in unabhängige Variationskomponenten zerlegen. Dekonvolutionsmethoden auf Basis von DNA Methylierung benötigen technisch hochwertige Profile und die identifizierten Komponenten müssen biologisch interpretiert werden. In dieser Arbeit entwickelten wir eine computerbasierte Pipeline zur Durchführung von Dekonvolutionsexperimenten, welche die Datenprozessierung und Interpretation der Resultate beinhaltet. Wir wendeten das entwickelte Protokoll auf Lungenadenokarzinome an und fanden Anzeichen für eine Tumorinfiltration durch Immunzellen, sowie Verbindungen zum Überleben der Patienten. Heterogenität innerhalb einer Probe (within-sample heterogeneity, WSH), d.h. heterogene Methylierungsmuster innerhalb einer Probe an einer genomischen Position, wird in epigenomischen Studien meist vernachlässigt. Wir präsentieren den ersten Vergleich verschiedener, genomweiter WSH Maße auf simulierten und experimentellen Daten. Zusätzlich entwickelten wir zwei neue Maße um WSH für einzelne CpGs zu berechnen, welche eine verbesserte Robustheit gegenüber technischen Faktoren aufweisen. WSH Maße beschreiben verschiedene Arten von WSH, quantifizieren differentielle Heterogenität und sagen Tumorreinheit vorher. Aufgrund der breiten Verfügbarkeit von DNA Methylierungsdaten können die Ebenen der Heterogenität ganzheitlich beschrieben werden. In dieser Arbeit präsentieren wir neue Softwarelösungen zur Analyse von DNA Methylierungsdaten in Bezug auf die verschiedenen Ebenen der Heterogenität. Wir sind davon überzeugt, dass die vorgestellten Softwarewerkzeuge unverzichtbar für das Verständnis von DNA Methylierung im kranken und gesunden Stadium sein werden

    RNA-seq – Revealing Biological Insights in Bacteria

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    New technologies are constantly being released and the improvements therein bring advances not only to transcriptome, the focus of this chapter, but also to diverse areas of biological research. Since the announcement and application of the RNA-seq approach, discoveries are being made in this field, but when we consider bacterial species, this progress proceeded a few years behind. However, with the application of RNA-seq derivative approaches, we can gain biological insights into the bacterial world and aspire to uncover the mysteries involving gene expression, organization and other functional genomic features

    Chromosome evolution and the genetic basis of agronomically important traits in greater yam

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    The nutrient-rich tubers of the greater yam, Dioscorea alata L., provide food and income security for millions of people around the world. Despite its global importance, however, greater yam remains an orphan crop. Here, we address this resource gap by presenting a highly contiguous chromosome-scale genome assembly of D. alata combined with a dense genetic map derived from African breeding populations. The genome sequence reveals an ancient allotetraploidization in the Dioscorea lineage, followed by extensive genome-wide reorganization. Using the genomic tools, we find quantitative trait loci for resistance to anthracnose, a damaging fungal pathogen of yam, and several tuber quality traits. Genomic analysis of breeding lines reveals both extensive inbreeding as well as regions of extensive heterozygosity that may represent interspecific introgression during domestication. These tools and insights will enable yam breeders to unlock the potential of this staple crop and take full advantage of its adaptability to varied environments
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