| Literature DB >> 32573495 |
Daniel Neiman1, David Gillis2, Sheina Piyanzin1, Daniel Cohen1, Ori Fridlich1, Joshua Moss1, Aviad Zick3, Tal Oron4, Frida Sundberg5, Gun Forsander5, Oskar Skog6, Olle Korsgren6, Floris Levy-Khademi7, Dan Arbel8, Saar Hashavia9, A M James Shapiro10, Cate Speake11, Carla Greenbaum11, Jennifer Hosford12, Amanda Posgai13, Mark A Atkinson12,13, Benjamin Glaser14, Desmond A Schatz12, Ruth Shemer1, Yuval Dor1.
Abstract
It has been proposed that unmethylated insulin promoter fragments in plasma derive exclusively from β cells, reflect their recent demise, and can be used to assess β cell damage in type 1 diabetes. Herein we describe an ultrasensitive assay for detection of a β cell-specific DNA methylation signature, by simultaneous assessment of 6 DNA methylation markers, that identifies β cell DNA in mixtures containing as little as 0.03% β cell DNA (less than 1 β cell genome equivalent). Based on this assay, plasma from nondiabetic individuals (N = 218, aged 4-78 years) contained on average only 1 β cell genome equivalent/mL. As expected, cell-free DNA (cfDNA) from β cells was significantly elevated in islet transplant recipients shortly after transplantation. We also detected β cell cfDNA in a patient with KATP congenital hyperinsulinism, in which substantial β cell turnover is thought to occur. Strikingly, in contrast to previous reports, we observed no elevation of β cell-derived cfDNA in autoantibody-positive subjects at risk for type 1 diabetes (N = 32), individuals with recent-onset type 1 diabetes (<4 months, N = 92), or those with long-standing disease (>4 months, N = 38). We discuss the utility of sensitive β cell cfDNA analysis and potential explanations for the lack of a β cell cfDNA signal in type 1 diabetes.Entities:
Keywords: Beta cells; Endocrinology; Epigenetics; Metabolism; Molecular diagnosis
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Year: 2020 PMID: 32573495 PMCID: PMC7453897 DOI: 10.1172/jci.insight.136579
Source DB: PubMed Journal: JCI Insight ISSN: 2379-3708