Differences

This shows you the differences between two versions of the page.

--- gwas [2020/06/22 17:08]
trynke
+++ gwas [2021/05/27 17:21] (current)
trynke
@@ Line 2: / Line 2: @@
 GWAS is one of Lifelines' [[additional assessments]] and contains the genome-wide [[https://en.wikipedia.org/wiki/Single-nucleotide_polymorphism|SNP]] data of 15.400 adult Lifelines participants derived from the [[https://www.illumina.com/products/by-type/clinical-research-products/human-cytosnp-12.html|Illumina CytoSNP-12v2 array]].\\
-The name GWAS might be confusing, as the assessment is not a [[https://en.wikipedia.org/wiki/Genome-wide_association_study|"genome wide association study"]] in itself, but rather the formation of a database of SNP data that can be used to perform such studies.\\
+The name GWAS might be confusing, as the assessment is not a [[https://en.wikipedia.org/wiki/Genome-wide_association_study|"genome wide association study"]] in itself, but rather the formation of a database of SNP data that can be used, together with Lifelines phenotype data, to perform such studies.\\
 Note that a second set of participants is genotyped in the [[UGLI]] project.
@@ Line 18: / Line 18: @@
 | Age category 18-64                   | N=13890        |
 | Age category 65+                     | N=1510         |
+{{:gwas_age_distribution.jpg?400|}}
 ===== SNP array =====
@@ Line 23: / Line 25: @@
 The 12-sample HumanCytoSNP-12 BeadChip is a powerful, whole-genome scanning panel designed for efficient, high-throughput analysis of genetic and structural variations that are the most relevant to human disease. Many types and sizes of structural variation in the human genome that affect phenotypes can be detected with the HumanCytoSNP-12 BeadChip, including duplications, deletions, amplifications, copy-neutral LOH, and mosaicism. This BeadChip includes a complete panel of genome-wide tag SNPs and markers targeting all regions of known cytogenetic importance. It incorporates 200,000 SNPs which cover around 250 genomic regions commonly screened in cytogenetics laboratories, including subtelomeric regions, pericentromeric regions, sex chromosomes, and targeted coverage in around 400 additional disease-related genes.
-====Quality checks====
+===== Quality checks =====
 Quality controls of the data are based on SNP filtering on minor allele frequency (MAF) above 0.001, Hardy-Weinberg equilibrium (HWE) P-value >1e-4, call rate of 0.95 using Plink ((Purcell S Neale B Todd-Brown Ket al. . PLINK: A tool set for whole-genome association and population-based linkage analyses. Am J Hum Genet  2007;81:559–75)), and principal component analysis (PCA) to check for population outliers. Description and criteria for quality checks are listed in the Table 2.
@@ Line 53: / Line 55: @@
 |                                                                     |                                                                                             |                                                                                                                                                                                                                                                                      |
+===== Imputation =====
+To get more information about the genome of the participants and therefore to scale up the number of SNPs, the genotype data generated using the arrays were imputed against reference genomes obtained by means of whole genome sequencing. IMPUTE2 (ref) is a program that can predict what the missing SNPs will be based on known SNPs or haplotypes (a combination of SNPs) by mapping the known genotypes against reference genomes.
+Before imputation, the genotypes were pre-phased using SHAPEIT2 (ref)  and aligned to the reference panels using Genotype Harmonizer (www.molgenis.org/systemsgenetics) in order to resolve strand issues. Generation of cleaned pedigree files and in- and output files for different imputation algorithms: Pedigree files are created in PLINK binary format. Genotypes of SNPs not directly genotyped on the Cyto12-SNP chip, but genotyped in another study, can be inferred by imputation.
+Imputation analysis is performed through Beagle 3.1.0 and data in these formats will be made available.
+The samples were imputed using Minimac((Howie B Fuchsberger C Stephens M Marchini J Abecasis GR. Fast and accurate genotype imputation in genome-wide association studies through pre-phasing. Nat Genet  2012;44:955–59))  version 2012.10.3 against human reference genomes, i.e.
+  * the Genome of The Netherlands (GoNL) release 5((Genome of The Netherlands Consortium. Whole-genome sequence variation, population structure and demographic history of the Dutch population. Nat Genet  2014;46:818–25))
+  * the 1000 Genomes phase1 v3((1000 Genomes Project Consortium, Abecasis GR, Altshuler D, et al. A map of human genome variation from population-scale sequencing. Nature  2010;467:1061–73)) reference panels.
+G is a human reference panel which contains world-wide collected genomes. Since only a small population of Dutch people (from the North) are part of the 1000G panel, the genotyped SNP dataset from the array was also imputed against GoNL. This is a reference panel that contains genomes from individuals with Dutch ancestry (with parents born in the Netherlands). 165 genomes in this panel were collected from Lifelines participants, meaning that genome data from Northern-Dutch people are available. The GoNL panel showed more accurate genotypes when imputing European samples compared with the 1000 Genomes Phase1 v3 reference panel. The MOLGENIS compute((Byelas, H
+et al. Scaling bio-analyses from computational clusters to grids. Proceedings of Fifth International Workshop on Science Gateways (IWSG), 2013, 3–5 June. Zurich, Switzerland , 2013)) imputation pipeline was used to generate and monitor our job scripts on the distributed file system.
+In summary:\\
+  * 1000G imputed: missing genotypes of participants are imputed (or predicted) based on 1000G reference panel (taken from worldwide population) and the available generated genotypes of the SNP array\\
+  * GoNL imputed: missing genotypes of participants are imputed (or predicted) based on the GoNL reference panel (taken from the Dutch population) and the available generated genotypes of the SNP array\\
+  * Unimputed: Genotypes determined on the basis of the SNP array, not imputed against genomic reference panels.
+===== Non-Caucasian samples =====
+To prevent false-positive association, non-Caucasian samples are excluded.
+Samples are determined by:
+  * The LifeLines phenotype database (self-report)\\
+  * Outlier (IBS) analysis\\
+  * Population stratification (using Eigenstrat)
+===== Cryptic relationships =====
+Samples are selected using self reported family relations. After cleaning of the data, samples are compared with each other to determine the relationship by genetic similarity. If a pair of samples are indicated as first degree relatives, the sample with the best genotyping quality will be included.
+===== Releasing SNP genotype data =====
+The following files are available through the Lifelines workspace or HPC:
+  * files with phenotype data
+  * files with genotyped and imputed data
+  * quality control files:
+      * list of samples excluded
+      * list of SNPs excluded
+      * PCA component file
+===== Abbreviations =====
+| GWAS   | Genome Wide Association Studies                   |
+| SNP    | Single-nucleotide polymorphism                    |
+| HWE    | Hardy-Weinberg Equilibrium                        |
+| CNV    | Copy Number Variant                               |
+| MAF    | Minor allele frequency                            |
+| PLINK  | PLINK is a command line program written in C/C++  |

Lifelines Wiki

User Tools

Site Tools

Differences

Page Tools