Selective proliferative response of microglia to alternative polarization signals

Giovanna Pepe; Marcella De Maglie; Lucia Minoli; Alessandro Villa; Adriana Maggi; Elisabetta Vegeto

doi:10.1186/s12974-017-1011-6

Selective proliferative response of microglia to alternative polarization signals

J Neuroinflammation. 2017 Dec 4;14(1):236. doi: 10.1186/s12974-017-1011-6.

Authors

Giovanna Pepe¹, Marcella De Maglie^{2

3}, Lucia Minoli^{2

3}, Alessandro Villa¹, Adriana Maggi¹, Elisabetta Vegeto⁴

Affiliations

¹ Center of Excellence on Neurodegenerative Diseases and Department Pharmacological and Biomolecular Sciences, University of Milan, Via Balzaretti, 9, 20133, Milan, Italy.
² Mouse and Animal Pathology Laboratory (MAPLab), Fondazione Filarete, Viale Ortles, 22/4, 20139, Milan, Italy.
³ Department of Veterinary Medicine, University of Milan, Via Celoria, 10, 20133, Milan, Italy.
⁴ Center of Excellence on Neurodegenerative Diseases and Department Pharmacological and Biomolecular Sciences, University of Milan, Via Balzaretti, 9, 20133, Milan, Italy. elisabetta.vegeto@unimi.it.

Abstract

Background: Microglia are resident myeloid cells of the central nervous system (CNS) that are maintained by self-renewal and actively participate in tissue homeostasis and immune defense. Under the influence of endogenous or pathological signals, microglia undertake biochemical transformations that are schematically classified as the pro-inflammatory M1 phenotype and the alternatively activated M2 state. Dysregulated proliferation of M1-activated microglia has detrimental effects, while an increased number of microglia with the alternative, pro-resolving phenotype might be beneficial in brain pathologies; however, the proliferative response of microglia to M2 signals is not yet known. We thus evaluated the ability of interleukin-4 (IL-4), a typical M2 and proliferative signal for peripheral macrophages, to induce microglia proliferation and compared it with other proliferative and M2 polarizing stimuli for macrophages, namely colony-stimulating factor-1 (CSF-1) and the estrogen hormone, 17β-estradiol (E₂).

Methods: Recombinant IL-4 was delivered to the brain of adult mice by intracerebroventricular (i.c.v.) injection; whole brain areas or ex vivo-sorted microglia were analyzed by real-time PCR for assessing the mRNA levels of genes related with cell proliferation (Ki67, CDK-1, and CcnB2) and M2 polarization (Arg1, Fizz1, Ym-1) or by FACS analyses of in vivo BrdU incorporation in microglia. Primary cultures of microglia and astrocytes were also tested for proliferative effects.

Results: Our results show that IL-4 only slightly modified the expression of cell cycle-related genes in some brain areas but not in microglia, where it strongly enhanced M2 gene expression; on the contrary, brain delivery of CSF-1 triggered proliferation as well as M2 polarization of microglia both in vivo and in vitro. Similar to IL-4, the systemic E₂ administration failed to induce microglia proliferation while it increased M2 gene expression.

Conclusions: Our data show that, in contrast to the wider responsiveness of peripheral macrophages, microglia proliferation is stimulated by selected M2 polarizing stimuli suggesting a role for the local microenvironment and developmental origin of tissue macrophages in regulating self-renewal following alternative activating stimuli.

Keywords: Estrogen; Interleukin-4; Microglia; Proliferation.

MeSH terms

Animals
Cell Proliferation / drug effects
Cell Proliferation / physiology
Estradiol / pharmacology
Female
Interleukin-4 / pharmacology
Macrophage Activation / drug effects*
Macrophage Colony-Stimulating Factor / pharmacology
Mice
Mice, Inbred C57BL
Microglia / cytology*
Microglia / drug effects*
Phenotype

Substances

Interleukin-4
Estradiol
Macrophage Colony-Stimulating Factor

Abstract

MeSH terms

Substances

Grants and funding