Preventing erosion of X-chromosome inactivation in human embryonic stem cells

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Marissa Cloutier
Surinder Kumar
Emily Buttigieg
Laura Keller
Brandon Lee
Aaron Williams
Sandra Mojica-Perez
Indri Erliandri
Andre Monteiro Da Rocha
Kenneth Cadigan
Gary D. Smith
Sundeep Kalantry
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[1] University of Michigan Medical School,Department of Human Genetics
[2] University of Michigan Medical School,Department of Molecular & Integrative Physiology
[3] University of Michigan Medical School,Department of Obstetrics & Gynecology
[4] University of Michigan Medical School,Department of Urology
[5] University of Michigan Medical School,Department of Physiology
[6] University of Michigan Medical School,Department of Internal Medicine & Cardiology
[7] Cellular,Department of Molecular
[8] and Developmental Biology,Department of Pathology
[9] University of Michigan Medical School,undefined
[10] University of Michigan Medical School,undefined
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X-chromosome inactivation is a paradigm of epigenetic transcriptional regulation. Female human embryonic stem cells (hESCs) often undergo erosion of X-inactivation upon prolonged culture. Here, we investigate the sources of X-inactivation instability by deriving new primed pluripotent hESC lines. We find that culture media composition dramatically influenced the expression of XIST lncRNA, a key regulator of X-inactivation. hESCs cultured in a defined xenofree medium stably maintained XIST RNA expression and coating, whereas hESCs cultured in the widely used mTeSR1 medium lost XIST RNA expression. We pinpointed lithium chloride in mTeSR1 as a cause of XIST RNA loss. The addition of lithium chloride or inhibitors of GSK-3 proteins that are targeted by lithium to the defined hESC culture medium impeded XIST RNA expression. GSK-3 inhibition in differentiating female mouse embryonic stem cells and epiblast stem cells also resulted in a loss of XIST RNA expression. Together, these data may reconcile observed variations in X-inactivation in hESCs and inform the faithful culture of pluripotent stem cells.
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