Levels of circulating insulin cell-free DNA in women with polycystic ovary syndrome - a longitudinal cohort study

Pernille Bækgaard Udesen; Anja Elaine Sørensen; Mugdha V Joglekar; Anandwardhan A Hardikar; Marie Louise Muff Wissing; Anne-Lis Mikkelsen Englund; Louise Torp Dalgaard

doi:10.1186/s12958-019-0478-7

Levels of circulating insulin cell-free DNA in women with polycystic ovary syndrome - a longitudinal cohort study

Reprod Biol Endocrinol. 2019 Apr 5;17(1):34. doi: 10.1186/s12958-019-0478-7.

Authors

Pernille Bækgaard Udesen¹, Anja Elaine Sørensen², Mugdha V Joglekar³, Anandwardhan A Hardikar³, Marie Louise Muff Wissing⁴, Anne-Lis Mikkelsen Englund⁴, Louise Torp Dalgaard²

Affiliations

¹ Fertility Clinic, Dept. of Gynecology and Obstetrics, Zealand University Hospital, Lykkebækvej 14, 4600, Køge, Denmark. pernilleudesen@hotmail.com.
² Department of Natural Science and Environment, Universitetsvej 1, 4000, Roskilde, Denmark.
³ Diabetes and Islet Biology Group, NHMRC Clinical Trials Centre, University of Sydney, 92 Parramatta Road, Sydney, NSW, 2050, Australia.
⁴ Fertility Clinic, Dept. of Gynecology and Obstetrics, Zealand University Hospital, Lykkebækvej 14, 4600, Køge, Denmark.

Abstract

Background: Women with Polycystic Ovary Syndrome (PCOS) present a heterogeneous reproductive and metabolic profile with an increased lifetime risk of Type 2 Diabetes (T2D). Early biomarkers of these metabolic disturbances in PCOS women have not been identified. The abundance of circulating insulin gene promotor cell-free DNA (INS cfDNA) was shown to be valuable as a predictive biomarker of β-cell death in individuals with Type 1 diabetes (T1D) as well as with gestational diabetes. Since β-cell death is common to the development of T1D as well as in T2D, we aimed to investigate if insulin-coding DNA is more abundant in circulation of PCOS women (vs Controls) and if their levels change after 6 yr. follow-up as a potential measure to predict future T2D.

Methods: A cohort of 40 women diagnosed with PCOS according to Rotterdam 2003 criteria and eight healthy controls were examined at baseline and 6 years follow-up. Clinical measurements for evaluation of glucose homeostasis as well as blood/serum samples were obtained at each visit. Methylated and unmethylated INS cfDNA were quantified using droplet digital PCR. Differences between groups were assessed using Kruskall-Wallis test and Wilcoxon Signed rank test.

Results: At baseline, there was no detectable difference in copy number (copies/μL) of methylated (p = 0.74) or unmethylated INS cfDNA (p = 0.34) between PCOS and Control groups. At follow up, neither methylated (p = 0.50) nor unmethylated INScfDNA levels (p = 0.48) differed significantly between these groups. Likewise, when pooling the groups, there was no difference between baseline and follow up, in terms of copies of methylated or unmethylated INS cfDNA (p = 0.38 and p = 0.52, respectively). There were no significant correlations between counts of unmethylated or methylated cfDNA and the clinical measurements of β-cell function and pre-diabetes.

Conclusion: The circulating level of unmethylated and methylated INScfDNA is similar between PCOS and Controls and cannot be used to predict islet β-cell loss and progression to Type 2 diabetes in a 6-year follow-up.

Trial registration: The Danish Data Protection Agency (REG-31-2016. Approval: 01-12-2015) and by the Danish Scientific Ethical committee of Region Zealand (Journal no. SJ-525. Approval: 13-06-2016), Clinicaltrials.gov, ( NCT03142633 , registered 1. March, 2017, Retrospectively registered).

Keywords: Androgens; Circulating free DNA; Demethylation; Glucose tolerance; Insulin promoter CpG methylation; PCOS; Testosterone.

MeSH terms

Adult
Biomarkers / blood
Cell-Free Nucleic Acids / blood*
DNA Methylation
Diabetes Mellitus, Type 2 / diagnosis*
Female
Humans
Insulin / genetics*
Longitudinal Studies
Polycystic Ovary Syndrome / metabolism*

Substances

Biomarkers
Cell-Free Nucleic Acids
Insulin

Associated data

ClinicalTrials.gov/NCT03142633