The impact of the histone deacetylase inhibitor sodium butyrate on microglial polarization after oxygen and glucose deprivation

Karolina Ziabska; Justyna Gargas; Joanna Sypecka; Malgorzata Ziemka-Nalecz

doi:10.1007/s43440-022-00384-x

The impact of the histone deacetylase inhibitor sodium butyrate on microglial polarization after oxygen and glucose deprivation

Pharmacol Rep. 2022 Oct;74(5):909-919. doi: 10.1007/s43440-022-00384-x. Epub 2022 Jul 7.

Authors

Karolina Ziabska¹, Justyna Gargas¹, Joanna Sypecka¹, Malgorzata Ziemka-Nalecz²

Affiliations

¹ NeuroRepair Department, Mossakowski Medical Research Institute, Polish Academy of Sciences, 5 A. Pawinskiego Street, 02-106, Warsaw, Poland.
² NeuroRepair Department, Mossakowski Medical Research Institute, Polish Academy of Sciences, 5 A. Pawinskiego Street, 02-106, Warsaw, Poland. mnalecz@imdik.pan.pl.

PMID: 35796871
DOI: 10.1007/s43440-022-00384-x

Abstract

Background: Microglia play a major role in the development of brain inflammation after central nervous system injury. On the other hand, microglia also participate in the repair process. The dualistic role of these cells results from the fact that various states of their activation are associated with specific phenotypes. The M1 phenotype is responsible for the production of proinflammatory mediators, whereas the M2 microglia release anti-inflammatory and trophic factors and take part in immunosuppressive and neuroprotective processes. The histone deacetylase inhibitor sodium butyrate (SB) shows anti-inflammatory and neuroprotective effects in some animal models of brain injury. The aim of this study was to examine the effects of sodium butyrate on the proliferation and M1/M2 polarization of primary microglial cells after oxygen and glucose deprivation (OGD) in vitro.

Methods: Primary microglial cultures were prepared from 1-day-old rats, subjected to the OGD procedure and treated with SB (0.1 mM, 1 mM and 10 mM). The effect of OGD and SB on microglial proliferation was assessed by double immunofluorescence, and microglial phenotypes were evaluated by qPCR.

Results: The OGD procedure stimulated the proliferation of microglia after 24 h of culturing, and SB treatment reduced the division of these cells. This effect was inversely proportional to the SB concentration. The OGD procedure increased proinflammatory CD86 and IL1β gene expression and reduced the expression of the anti-inflammatory M2 markers arginase and CD200 in microglia.

Conclusions: SB can change the polarization of microglia after OGD from an unfavourable M1 to a beneficial M2 phenotype. Our results show that SB is a potential immunosuppressive agent that can modulate microglial activation stimulated by ischaemic-like conditions.

Keywords: Histone deacetylase inhibitor (HDACi); M1/M2 phenotype; Oxygen and glucose deprivation (OGD); Primary microglial culture; Sodium butyrate (SB).

MeSH terms

Animals
Arginase / metabolism
Arginase / pharmacology
Butyric Acid / metabolism
Butyric Acid / pharmacology
Glucose / metabolism
Histone Deacetylase Inhibitors / pharmacology
Immunosuppressive Agents / pharmacology
Microglia*
Neuroprotective Agents* / pharmacology
Oxygen / metabolism
Rats

Substances

Butyric Acid
Histone Deacetylase Inhibitors
Glucose
Neuroprotective Agents
Oxygen
Arginase
Immunosuppressive Agents

Grants and funding

2017/27/B/NZ3/00582/Narodowe Centrum Nauki