Parallel target selection by trinucleotide threading

Zajac, Pawel

January 2009

DNA is the code for all life. Via intermediary RNA the information encoded by the genome is relayed to proteins executing the various functions in a cell. Together, this repertoire of inherently linked biological macromolecules determines all characteristics and features of a cell. Technological advancements during the last decades have enabled the pursuit of novel types of studies and the investigation of the cell and its constituents at a progressively higher level of detail. This has shed light on numerous cellular processes and on the underpinnings of several diseases. For the majority of studies focusing on nucleic acids, an amplification step has to be implemented before an analysis, scoring or interrogation method translates the amplified material into relevant biological information. This information can, for instance, be the genotype of particular SNPs or STRs, or the abundance level of a set of interesting transcripts. As such, amplification plays a significant role in nucleic acid assays. Over the years, a number of techniques – most notably PCR – has been devised to meet this amplification need, specifically or randomly multiplying desired regions. However, many of the approaches do not scale up easily rendering comprehensive studies cumbersome, time-consuming and necessitating large quantities of material.Trinucleotide threading (TnT) – forming the red thread throughout this thesis – is a multiplex amplification method, enabling simultaneous targeted amplification of several nucleic acid regions in a specific manner. TnT begins with a controlled linear DNA thread formation, each type of thread corresponding to a segment of interest, by a gap-fill reaction using a restricted trinucleotide set. The whole collection of created threads is subsequently subjected to an exponential PCR amplification employing a single primer pair. The generated material can thereafter be analyzed with a multitude of readout and detection platforms depending on the issue or characteristic under consideration.TnT offers a high level of specificity by harnessing the inherent specificities of a polymerase and a ligase acting on a nucleotide set encompassing three out of the four nucleotide types. Accordingly, several erroneous events have to occur in order to produce artifacts. This necessitates override of a number of control points.The studies constituting this thesis demonstrate integration of the TnT amplification strategy in assays for analysis of various aspects of DNA and RNA. TnT was adapted for expression profiling of intermediately-sized gene sets using both conventional DNA microarrays and massively parallel second generation 454 sequencing for readout. TnT, in conjunction with 454 sequencing, was also employed for allelotyping, defined as determination of allele frequencies in a cohort. In this study, 147 SNPs were simultaneously assayed in a pool comprising genomic DNA of 462 individuals. Finally, TnT was recruited for parallel amplification of STR loci with detection relying on capillary gel electrophoresis. In all investigations, the material generated with TnT was of sufficient quality and quantity to produce reliable and accurate biological information.Taken together, TnT represents a viable multiplex amplification technique permitting parallel amplification of genomic segments, for instance harboring polymorphisms, or of expressed genes. In addition to these, this versatile amplification module can be implemented in assays targeting a range of other features of genomes and transcriptomes. / QC 20100819

trinucleotide threading

multiplex amplification

expression profiling

microarray

generic tag

short tandem repeat

microsatellite

electrophoresis

single nucleotide polymorphism

allelotyping

454

Pyrosequencing

Genteknik inkl. funktionsgenomik

Development of Y-STR genotyping systems suitable for sexual assault cases in South Africa

Cloete, Kevin Wesley

January 2010

Magister Scientiae - MSc / Sexual assault is a significant problem facing the South African society. In this context, efficient but also affordable genotyping systems are needed for positive identification of criminals in incidences of sexual violence. The aim of this study was therefore to develop non-commercial Y-STR genotyping systems suitable for sexual assault cases in South Africa. Y-chromosome STR loci constituting the minimal haplotype are still the most widely used loci in investigating sexual assault cases despite the fact that DYS391 and DYS392 have shown low levels of polymorphism in Xhosa populations in Cape Town. The minimal haplotype was, therefore, further investigated in the Cape Muslim population. The Cape Muslim population generally exhibited high GD values among all the South African populations. These values were higher than 0.5 for most loci, and ranged from 0.447 for DYS391 to 0.957 for DYS385. The highest number of alleles in most loci was also recorded in this population. The overall assessment of the minimal haplotype has shown that this system is still a useful in investigating sexual assault case in many South African subpopulations. Therefore the exercise of internal validation of the minimal haplotype system was successfully carried out in the laboratory. The properties of additional novel and widely used STRs were also investigated in this study. Loci were successfully sequenced and allele nomenclature was assigned to them according to the ISFG guidelines. / South Africa

Forensics

Short tandem repeat (STR)

Y-loci

Minimal haplotype (MinHt)

YHRD

Polymerase chain reaction (PCR)

Electrophoresis

Multiplex PCR

Genotyping

Gene diversity

Polymorphism

Ein bronzezeitlicher Familienclan als genetisches Archiv – Morphologisch-paläogenetische Bearbeitung des Skelettkollektivs aus der Lichtensteinhöhle / A Bronze Age family clan as genetic archive – Morphological-paleogenetical analysis of the skeletal remains from the Lichtenstein Cave

Seidenberg, Verena

29 September 2016

Die Lichtensteinhöhle ist eine Klufthöhle im Berg Lichtenstein in den Harzausläufern. Im anthropogenen Teil der Höhle wurden größere Mengen disoloziert vorliegender Menschenknochen gefunden. Über assoziierte archäologische Artefakte und 14C-Datierungen erfolgte eine Einordnung ins 10.–9. Jh. v. Chr.. Aufgrund eines Überzuges mit Gipssinter und konstant niedriger Temperaturen war ein herausragend guter Erhaltungszustand der Knochen und der enthaltenen aDNA gegeben. Dies ermöglichte umfangreiche anthropologische Forschungsarbeiten an den menschlichen Überresten aus der Lichtensteinhöhle. Eine zentrale Fragestellung zu Beginn der Forschungsarbeiten war, ob es sich um eine Opferstätte oder einen Bestattungsplatz handelt. Es konnte für die zunächst identifizierten 40 Individuen ein ausgewogenes Geschlechterverhältnis und eine Altersverteilung über alle Altersklassen hinweg nachgewiesen werden. Zudem konnten mittels molekulargenetischer Methoden verwandtschaftliche Beziehungen zwischen den Individuen aufgedeckt werden. Die Verwandtschaftsrekonstruktion ergab den Stammbaum eines Familienclans. Damit lagen eindeutige Hinweise für eine Nutzung als Bestattungsplatz vor. Während molekulargenetischer Reihenuntersuchungen verschiedener Skelettelemente und morphologischer Zuordnungen von Skelettelementen zu Individuen wurde deutlich, dass Knochen von mehr Individuen als den 40 bislang identifizierten vorhanden waren. Zudem deutete sich an, dass für nahezu alle Individuen nicht alle Knochen in der Höhle aufgefunden worden waren. Das Fehlen von Skelettelementen warf die Frage auf, ob es sich bei der Lichtensteinhöhle nicht um einen Primär- sondern um einen Sekundärbestattungsplatz handeln könnte. Im aktuell durchgeführten Forschungsprojekt wurden, unter Verwendung morphologischer und molekulargenetischer Methoden, die Zuordnungen der dislozierten Knochen zu Individuen zu Ende geführt. Die rekonstruierten Individuen wurden umfassend morphologisch und molekulargenetisch untersucht, mit dem Ziel, die demografische Struktur der Population zu erschließen und die Verwandtschaftsrekonstruktion auszuweiten. Zudem wurde den Fragen der Nutzungsdauer und der genauen Nutzungsart der Höhle nachgegangen. Es konnten 60 Individuen identifiziert werden. Nur für zwei der Individuen wurden alle bei den Zuordnungen berücksichtigten Skelettelemente vorgefunden. An den Knochen zeigten sich nur wenige Fälle degenerativer Veränderungen. Dies ließ darauf schließen, dass die in der Lichtensteinhöhle bestatteten Menschen nicht übermäßig harter körperlicher Belastung ausgesetzt waren. Spuren massiver Gewalteinwirkung fehlten vollständig. Dies macht es unwahrscheinlich, dass die bestattete Population in kriegerische Auseinandersetzungen involviert war. Einige wenige verheilte Frakturen an Rippen oder Schlüsselbein lassen sich problemlos auf Alltagsunfälle zurückführen. Spuren von Mangel- oder Stressphasen waren nur in Einzelfällen nachweisbar. Dies deutet darauf hin, dass die Bestatteten zu Lebzeiten kontinuierlichen Zugang zu ausreichenden Nahrungsressourcen hatten. Das Geschlechterverhältnis war ausgewogen und die Altersverteilung entsprach in den Grundzügen der für eine historische Population zu erwartenden. Eine fesgestellte Unterrepräsentanz von Individuen der Altersklasse Infans I könnte als Hinweis darauf interpretiert werden, dass tatsächlich Sekundärbestattungen praktiziert wurden und die sehr kleinen, fragilen Knochen der Infans I Individuen zum Zeitpunkt der Umbettungen bereits vergangen waren. In begleitenden Arbeiten durchgeführte statistischen Analysen verschiedener Merkmale, wie z.B. Unterschiede im Grad der DNA-Degradierung, lieferten weitere Hinweise in die Richtung, dass es sich bei der Lichtensteinhöhle um einen Sekundärbestattungsplatz handeln dürfte. Für alle neu identifizierten Inividuen wurden mittels molekulargenetischer Analysen die genetischen Fingerabdrücke sowie die mitochondraialen und Y-chromosomalen Haplotypen bestimmt. Die anschließende Verwandtschaftsrekonstruktion ergab einen erweiterten Stammbaum, in dem für 47 der 60 Individuen entweder direkte Verwandtschaft oder aber Verwandtschaft in mütterlicher oder väterlicher Familienlinie belegt ist. Der Stammbaum umfasst insgesamt sechs Generationen. Dies entspricht – bei einer angenommenen Generationendauer von 20 Jahren – einer Nutzungsdauer von 120 Jahren und passt somit gut zum archäologisch ermittelten Nutzungszeitraum. Die Auswertung der Diversität der mitochondrialen und Y-chromosomalen Haplotypen ergab Hinweise auf eine patrilokale Gesellschaftsform. In begleitenden Arbeiten wurden weitere genetische Marker – z.B. für die Augen- und Haarpigmentierung, die immungenetische Ausstattung oder auch für den Laktosetoleranzstatus – analysiert. Insgesamt zeigte sich, dass sich in vielerlei Hinsicht die genetische Ausstattung heutiger Populationen im Vergleich zu der vor 3.000 Jahren nicht grundlegend unterscheidet. Lediglich für die Frequenz des Laktosetoleranz verursachenden Allels war eine deutliche Zunahme seit der Bronzezeit zu verzeichnen.

570

Anthropologie

ancient DNA

aDNA

Lichtensteinhöhle

Bronzezeit

short tandem repeat

STR

mtDNA

Y-chromosomale Haplotypen

Verwandtschaft

Genealogie

Laktosetoleranz

Blutgruppen

Haarfarbe

Augenfarbe

Immungenetik

Paläodemografie

Alter

Geschlecht

anthropology

ancient DNA

aDNA

Lichtenstein Cave

Bronze Age

short tandem repeat

STR

mtDNA

Y-chromosomal haplotypes

kinship

genealogy

lactose tolerance

blood groups

hair color

eye color

immunogenetics

paleodemography

age

sex

Biologie (PPN619462639)

Characterisation of Eight Non-Codis Ministrs in Four South African Populations to Aid The Analysis of Degraded Dna.

Ismail, Aneesah.

January 2009

<p>In many forensic cases, such as mass disasters reconstruction cases, the recovered DNA is highly degraded. In such incidences, typing of STR loci has become one of the most powerful tools for retrieving information from the degraded DNA. However, as DNA degradation proceeds, three phenomena occur consecutively: loci imbalance, allele dropout and no amplification. To solve the problem of degraded DNA, redesigned primer sets have been developed in which the primers were positioned as close as possible to the STR repeat region. These reduced primer sets were called Miniplexes. Unfortunately, a few of the CODIS STR loci cannot be made into smaller amplicons. For this reason non-CODIS miniSTRs have been developed. The present study was undertaken for the population genetic analysis of microsatellite variation in four South African populations / Afrikaner, Xhosa, Mixed Ancestry and Asian Indian using eight non-CODIS miniSTR loci. These miniSTRs loci were characterized within the populations by estimating the levels of diversity of the markers, estimating the population genetic parameters, and studying the inter-population relationships. All of the miniSTRs were amplified successfully and the genetic variability parameters across all loci in Afrikaner, Mixed Ancestry, Asian Indian and Xhosa were estimated to be in the range of 3 (D4S2364) to 12 (D9S2157) alleles, the total number of alleles over all loci ranged from 100 to 204, the allelic richness ranged from 3.612 to 10.307 and the heterozygosity ranged from 0.4360 to 0.8073. Genetic distance was least between Afrikaner and Asian Indian and highest between Xhosa and Mixed Ancestry. Deviations from Hardy-Weinberg equilibrium were not observed for most of the loci. The low mean FIS (-0.027) and FIT (-0.010) and FST (0.017) values across the populations indicated low level of inbreeding within (FIS) and among (FST) the populations. The Asian Indian population showed higher levels of the inbreeding coefficient, indicating less gene exchange between it and other populations. These 8 markers can be used for genetic investigations and assessing population structure. The study contributed to the knowledge and genetic characterization of four South African populations. In addition, these MiniSTRs prove to be useful in cases where more genetic information is needed.</p>

Short Tandem Repeat (STR)

Microsatellites

Loci

Combined DNA Index System (CODIS)

Degraded DNA

Mitochondrial DNA (mtDNA)

MiniSTR

Polymerase Chain Reaction (PCR)

Electrophoresis

Genotyping

Polymorphic Information Content (PIC)

Fixation Indexes.

Characterisation of Eight Non-Codis Ministrs in Four South African Populations to Aid The Analysis of Degraded Dna.

Ismail, Aneesah.

January 2009

<p>In many forensic cases, such as mass disasters reconstruction cases, the recovered DNA is highly degraded. In such incidences, typing of STR loci has become one of the most powerful tools for retrieving information from the degraded DNA. However, as DNA degradation proceeds, three phenomena occur consecutively: loci imbalance, allele dropout and no amplification. To solve the problem of degraded DNA, redesigned primer sets have been developed in which the primers were positioned as close as possible to the STR repeat region. These reduced primer sets were called Miniplexes. Unfortunately, a few of the CODIS STR loci cannot be made into smaller amplicons. For this reason non-CODIS miniSTRs have been developed. The present study was undertaken for the population genetic analysis of microsatellite variation in four South African populations / Afrikaner, Xhosa, Mixed Ancestry and Asian Indian using eight non-CODIS miniSTR loci. These miniSTRs loci were characterized within the populations by estimating the levels of diversity of the markers, estimating the population genetic parameters, and studying the inter-population relationships. All of the miniSTRs were amplified successfully and the genetic variability parameters across all loci in Afrikaner, Mixed Ancestry, Asian Indian and Xhosa were estimated to be in the range of 3 (D4S2364) to 12 (D9S2157) alleles, the total number of alleles over all loci ranged from 100 to 204, the allelic richness ranged from 3.612 to 10.307 and the heterozygosity ranged from 0.4360 to 0.8073. Genetic distance was least between Afrikaner and Asian Indian and highest between Xhosa and Mixed Ancestry. Deviations from Hardy-Weinberg equilibrium were not observed for most of the loci. The low mean FIS (-0.027) and FIT (-0.010) and FST (0.017) values across the populations indicated low level of inbreeding within (FIS) and among (FST) the populations. The Asian Indian population showed higher levels of the inbreeding coefficient, indicating less gene exchange between it and other populations. These 8 markers can be used for genetic investigations and assessing population structure. The study contributed to the knowledge and genetic characterization of four South African populations. In addition, these MiniSTRs prove to be useful in cases where more genetic information is needed.</p>

Short Tandem Repeat (STR)

Microsatellites

Loci

Combined DNA Index System (CODIS)

Degraded DNA

Mitochondrial DNA (mtDNA)

MiniSTR

Polymerase Chain Reaction (PCR)

Electrophoresis

Genotyping

Polymorphic Information Content (PIC)

Fixation Indexes.

Characterisation of eight non-codis Ministrs in four South African populations to aid the analysis of degraded DNA

Ismail, Aneesah

January 2009

Magister Scientiae - MSc / In many forensic cases, such as mass disasters reconstruction cases, the recovered DNA is highly degraded. In such incidences, typing of STR loci has become one of the most powerful tools for retrieving information from the degraded DNA. However, as DNA degradation proceeds, three phenomena occur consecutively: loci imbalance, allele dropout and no amplification. To solve the problem of degraded DNA, redesigned primer sets have been developed in which the primers were positioned as close as possible to the STR repeat region. These reduced primer sets were called Miniplexes. Unfortunately, a few of the CODIS STR loci cannot be made into smaller amplicons. For this reason non-CODIS miniSTRs have been developed. The present study was undertaken for the population genetic analysis of microsatellite variation in four South African populations; Afrikaner, Xhosa, Mixed Ancestry and Asian Indian using eight non-CODIS miniSTR loci. These miniSTRs loci were characterized within the populations by estimating the levels of diversity of the markers, estimating the population genetic parameters, and studying the inter-population relationships. All of the miniSTRs were amplified successfully and the genetic variability parameters across all loci in Afrikaner, Mixed Ancestry, Asian Indian and Xhosa were estimated to be in the range of 3 (D4S2364) to 12 (D9S2157) alleles, the total number of alleles over all loci ranged from 100 to 204, the allelic richness ranged from 3.612 to 10.307 and the heterozygosity ranged from 0.4360 to 0.8073. Genetic distance was least between Afrikaner and Asian Indian and highest between Xhosa and Mixed Ancestry. Deviations from Hardy-Weinberg equilibrium were not observed for most of the loci. The low mean FIS (-0.027) and FIT (-0.010) and FST (0.017) values across the populations indicated low level of inbreeding within (FIS) and among (FST) the populations. The Asian Indian population showed higher levels of the inbreeding coefficient, indicating less gene exchange between it and other populations. These 8 markers can be used for genetic investigations and assessing population structure. The study contributed to the knowledge and genetic characterization of four South African populations. In addition, these MiniSTRs prove to be useful in cases where more genetic information is needed. / South Africa

Short Tandem Repeat (STR)

Microsatellites

Loci

Combined DNA Index System (CODIS)

Degraded DNA

Mitochondrial DNA (mtDNA)

MiniSTR

Polymerase Chain Reaction (PCR)

Electrophoresis

Genotyping

Polymorphic Information Content (PIC)

Fixation indexes