Genetic background modulates the effect of glucocorticoids on proliferation, differentiation and myelin formation of oligodendrocyte lineage cells

Author:

Gigliotta Adrien12,Mingardi Jessica123,Cummings Sarah4,Alikhani Vida125,Trontti Kalevi12,Barbon Alessandro6,Kothary Rashmi4,Hovatta Iiris12

Affiliation:

1. SleepWell Research Program, Faculty of Medicine University of Helsinki Helsinki Finland

2. Department of Psychology and Logopedics, Faculty of Medicine University of Helsinki Helsinki Finland

3. School of Medicine and Surgery University of Milano‐Bicocca Monza Italy

4. Regenerative Medicine Program Ottawa Hospital Research Institute and University of Ottawa Ottawa Ontario Canada

5. Department of Physiology, Faculty of Medicine Mashhad University of Medical Science Mashhad Iran

6. Department of Molecular and Translational Medicine University of Brescia Brescia Italy

Abstract

AbstractAnxiety disorders are prevalent mental disorders. Their predisposition involves a combination of genetic and environmental risk factors, such as psychosocial stress. Myelin plasticity was recently associated with chronic stress in several mouse models. Furthermore, we found that changes in both myelin thickness and node of Ranvier morphology after chronic social defeat stress are influenced by the genetic background of the mouse strain. To understand cellular and molecular effects of stress‐associated myelin plasticity, we established an oligodendrocyte (OL) model consisting of OL primary cell cultures isolated from the C57BL/6NCrl (B6; innately non‐anxious and mostly stress‐resilient strain) and DBA/2NCrl (D2; innately anxious and mostly stress‐susceptible strain) mice. Characterization of naïve cells revealed that D2 cultures contained more pre‐myelinating and mature OLs compared with B6 cultures. However, B6 cultures contained more proliferating oligodendrocyte progenitor cells (OPCs) than D2 cultures. Acute exposure to corticosterone, the major stress hormone in mice, reduced OPC proliferation and increased OL maturation and myelin production in D2 cultures compared with vehicle treatment, whereas only OL maturation was reduced in B6 cultures. In contrast, prolonged exposure to the synthetic glucocorticoid dexamethasone reduced OPC proliferation in both D2 and B6 cultures, but only D2 cultures displayed a reduction in OPC differentiation and myelin production. Taken together, our results reveal that genetic factors influence OL sensitivity to glucocorticoids, and this effect is dependent on the cellular maturation stage. Our model provides a novel framework for the identification of cellular and molecular mechanisms underlying stress‐associated myelin plasticity.

Funder

Research Council of Finland

Sigrid Juséliuksen Säätiö

Helsingin Yliopisto

Alfred Kordelinin Säätiö

Jalmari ja Rauha Ahokkaan Säätiö

Publisher

Wiley

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