Dr RACHEL CLIFFORD R.Clifford@nottingham.ac.uk
ANNE MCLAREN FELLOW
Investigating genome wide DNA methylation in bronchial and lung fibroblasts from healthy individuals and individuals with COPD
Clifford, R.L.; Fishbane, N.; Rajasekar, P.; MacIsaac, J.L.; McEwen, L.M.; Fisher, A.; Kobor, M.; Knox, A.J.; Hackett, T.-L.
Authors
N. Fishbane
Mrs POOJITHA RAJASEKAR Poojitha.Rajasekar@nottingham.ac.uk
RESEARCH ASSOCIATE
J.L. MacIsaac
L.M. McEwen
A. Fisher
M. Kobor
A.J. Knox
T.-L. Hackett
Abstract
Rationale: Lung fibroblasts are implicated in respiratory disease pathology including chronic obstructive pulmonary disease (COPD). Phenotypic differences between fibroblasts isolated from the bronchi versus the lung parenchyma have been described but no studies have compared the cell types on a genome wide scale. DNA methylation is a reversible modification of the DNA structure with the ability to affect cell function via the alteration of gene expression. Here we compared genome wide DNA methylation profiles from bronchial and lung fibroblasts and assessed modification to these profiles in cells isolated from individuals with COPD.
Methods: DNA was isolated from lung (LgF) and bronchial fibroblasts (BrF) at passage 4 and bisulphite treated. Site specific, quantitative genome wide methylation was determined using the Illumina 450K Infinium Methylation BeadChip array. Linear modelling and DMRcate functions identified differentially methylated sites and regions respectively between BrF and LgF and from cells isolated from healthy individuals versus those with COPD.
Results: 3980 CpG (methylation) sites significantly differed, following Bonferroni correction, between BrF and LgF isolated from healthy individuals. These sites had a broad distribution of effect size, with 240 CpG sites displaying a difference in methylation of >50%. 78 of these sites were validated in a second cohort of matched BrF and LgF isolated from the same individuals. There was genomic proximity to these sites and DMRcate was used to refine the individual CpG sites to 5 regions of interest associated with 5 genes; HLX, TWIST1, CREB5, SKAP2 and PRDM16. Differences in methylation were less pronounced when comparing cells isolated from healthy individuals to those with COPD. In BrF 47 DMRcate regions were identified with a maximum difference in methylation of at least 20%. In LgF 3 DMRcate regions were identified with a maximum difference in methylation of at least 20%.
Conclusions: DNA methylation profiles are significantly different between BrF and LgF but only small modifications are associated with COPD. Future work will focus on validating a methylation based marker of lung versus bronchial fibroblasts to differentiate cell types by validating our differential DNA methylation observations with gene/protein expression.
Citation
Clifford, R., Fishbane, N., Rajasekar, P., MacIsaac, J., McEwen, L., Fisher, A., Kobor, M., Knox, A., & Hackett, T.-L. Investigating genome wide DNA methylation in bronchial and lung fibroblasts from healthy individuals and individuals with COPD. Presented at American Thoracic Society 2017 International Conference
Conference Name | American Thoracic Society 2017 International Conference |
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End Date | May 24, 2017 |
Acceptance Date | Feb 15, 2017 |
Publication Date | May 23, 2017 |
Deposit Date | Dec 14, 2017 |
Publicly Available Date | Dec 14, 2017 |
Peer Reviewed | Peer Reviewed |
Article Number | A6939 |
Public URL | https://nottingham-repository.worktribe.com/output/861759 |
Publisher URL | http://www.atsjournals.org/doi/abs/10.1164/ajrccm-conference.2017.195.1_MeetingAbstracts.A6939 |
Contract Date | Dec 14, 2017 |
Files
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