TREM2 sustains microglial expansion during aging and response to demyelination
Pietro Luigi Poliani, … , Susan Gilfillan, Marco Colonna
Pietro Luigi Poliani, … , Susan Gilfillan, Marco Colonna
Published April 20, 2015
Citation Information: J Clin Invest. 2015;125(5):2161-2170. https://doi.org/10.1172/JCI77983.
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Research Article Neuroscience

TREM2 sustains microglial expansion during aging and response to demyelination

Abstract

Microglia contribute to development, homeostasis, and immunity of the CNS. Like other tissue-resident macrophage populations, microglia express the surface receptor triggering receptor expressed on myeloid cells 2 (TREM2), which binds polyanions, such as dextran sulphate and bacterial LPS, and activates downstream signaling cascades through the adapter DAP12. Individuals homozygous for inactivating mutations in TREM2 exhibit demyelination of subcortical white matter and a lethal early onset dementia known as Nasu-Hakola disease. How TREM2 deficiency mediates demyelination and disease is unknown. Here, we addressed the basis for this genetic association using Trem2–/– mice. In WT mice, microglia expanded in the corpus callosum with age, whereas aged Trem2–/– mice had fewer microglia with an abnormal morphology. In the cuprizone model of oligodendrocyte degeneration and demyelination, Trem2–/– microglia failed to amplify transcripts indicative of activation, phagocytosis, and lipid catabolism in response to myelin damage. As a result, Trem2–/– mice exhibited impaired myelin debris clearance, axonal dystrophy, oligodendrocyte reduction, and persistent demyelination after prolonged cuprizone treatment. Moreover, myelin-associated lipids robustly triggered TREM2 signaling in vitro, suggesting that TREM2 may directly sense lipid components exposed during myelin damage. We conclude that TREM2 is required for promoting microglial expansion during aging and microglial response to insults of the white matter.

Authors

Pietro Luigi Poliani, Yaming Wang, Elena Fontana, Michelle L. Robinette, Yoshinori Yamanishi, Susan Gilfillan, Marco Colonna

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Figure 3

Trem2 deficiency impairs microglial response to demyelination.

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Trem2 deficiency impairs microglial response to demyelination. Corpus c...
Corpus callosum sections were stained with Iba-1 to detect microgliosis. (A) Representative images of Iba-1 staining. (B) Iba-1+ microglial frequencies per HPF. (C and D) Microglial morphology after cuprizone treatment. (C) Morphological assessment of WT and Trem2–/– microglia after 12 weeks of cuprizone treatment. Fragmentation, beading (arrowheads), and spheroid formation (asterisks) are indicated. (D) Surface area of Iba-1+ microglia is quantified. **P ≤ 0.01; ***P ≤ 0.001; ****P ≤ 0.0001, 2-way ANOVA. Original magnification, ×20 (A); ×60 (A, insets; C, middle and bottom images); and ×40 (C, top images). Scale bars: 100 μm (A); 30 μm (C, middle and bottom images); 50 μm (C, top images). Data represent 3 to 8 mice (B) and 4 mice per group (D) for a total of 2 experiments. An average of 10 HPF per mouse were evaluated for B. An average of 50 cells in 10 HPF per mouse were evaluated for D. Error bars represent mean ± SEM.