Abstract

Type 1 diabetes (T1D) is an autoimmune disease resulting in the loss of insulin- producing cells. Genetic studies, including those in twins, sugget a strong genetic basis for this disease. Genome-wide association studies (GWASs) have produced large numbers of T1D-associated single-nucleotide polymorphisms (SNPs), but often fail to determine a causative mutation. This may be due to the complexity of the disease; or in part, due to many associated SNPs lying outside of gene coding regions. A recent assessment of GWASs illustrated that 45% of disease or trait associated SNPs fell in introns, while 43% lie in intergenic regions. Global methods for determining chromatin states have shown that associated SNPs can overlap distal regulatory regions such as enhancers. We have constructed enhancer maps based H3K4me1 localization in isolated, human T cells. We analyzed the T1D-associated SNPs from the NHGRI GWAS catalog for overlap with our global T helper cell enhancer predictions. Using 1000 Genomes data we identified additional SNPs in linkage disequilibrium to expand the number of T1D-associated SNPs at enhancer elements. Goal: Our goal is to functionally validate T1D-associated rSNPs. We will use a series of high- throughput assays and systematic evaluation to determine the most functionally relevant rSNPs. We will also determine the target genes of enhancers overlapping T1D SNPs in order to identify new genes important in the etiology of T1D pathogenesis. We will do so through the following specific aims.
Specific Aim 1. Determine the effect of T1D rSNPs on enhancer activity.
Specific Aim 2. Determine if TF binding is disrupted at T1D-associated enhancer SNPs.
Specific Aim 3. Identification of target genes for enhancers harboring associated SNPs.

Public Health Relevance

Type 1 diabetes is an autoimmune disease with a strong genetic basis; however many associated variants have proved uninformative due to their non-genic locations. Using genome-wide approaches to map regulatory elements in human T cells, we identified enhancers that overlap type 1 diabetes-associated SNPs. We will functionally validate enhancer SNPs by several high-throughput methods to determine enhancer gene targets, and to tests for SNP disruption of transcription factor binding and enhancer activity.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
1R01DK103667-01A1
Application #
8961219
Study Section
Genetics of Health and Disease Study Section (GHD)
Program Officer
Akolkar, Beena
Project Start
2015-08-01
Project End
2020-06-30
Budget Start
2015-08-01
Budget End
2016-06-30
Support Year
1
Fiscal Year
2015
Total Cost
$500,273
Indirect Cost
$166,661

  Institution

Name
University of Washington
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
605799469
City
Seattle
State
WA
Country
United States
Zip Code
98195

  Publications

Yizhar-Barnea, Ofer; Valensisi, Cristina; Jayavelu, Naresh Doni et al. (2018) DNA methylation dynamics during embryonic development and postnatal maturation of the mouse auditory sensory epithelium. Sci Rep 8:17348
Pasumarthy, Kalyan K; Doni Jayavelu, Naresh; Kilpinen, Lotta et al. (2017) Methylome Analysis of Human Bone Marrow MSCs Reveals Extensive Age- and Culture-Induced Changes at Distal Regulatory Elements. Stem Cell Reports 9:999-1015
Mishra, Arpit; Hawkins, R David (2017) Three-dimensional genome architecture and emerging technologies: looping in disease. Genome Med 9:87
Yu, Bo; Dong, Xiao; Gravina, Silvia et al. (2017) Genome-wide, Single-Cell DNA Methylomics Reveals Increased Non-CpG Methylation during Human Oocyte Maturation. Stem Cell Reports 9:397-407
Valensisi, Cristina; Andrus, Colin; Buckberry, Sam et al. (2017) Epigenomic Landscapes of hESC-Derived Neural Rosettes: Modeling Neural Tube Formation and Diseases. Cell Rep 20:1448-1462
Moody, James D; Levy, Shiri; Mathieu, Julie et al. (2017) First critical repressive H3K27me3 marks in embryonic stem cells identified using designed protein inhibitor. Proc Natl Acad Sci U S A 114:10125-10130