Alcohol exposure–induced neurovascular inflammatory priming impacts ischemic stroke and is linked with brain perivascular macrophages
Antoine Drieu, Anastasia Lanquetin, Damien Levard, Martina Glavan, Francisco Campos, Aurélien Quenault, Eloïse Lemarchand, Mikaël Naveau, Anne Lise Pitel, José Castillo, Denis Vivien, Marina Rubio
Antoine Drieu, Anastasia Lanquetin, Damien Levard, Martina Glavan, Francisco Campos, Aurélien Quenault, Eloïse Lemarchand, Mikaël Naveau, Anne Lise Pitel, José Castillo, Denis Vivien, Marina Rubio
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Research Article Inflammation Neuroscience

Alcohol exposure–induced neurovascular inflammatory priming impacts ischemic stroke and is linked with brain perivascular macrophages

Abstract

Alcohol abuse is a major public health problem worldwide, causing a wide range of preventable morbidity and mortality. In this translational study, we show that heavy drinking (HD) (≥6 standard drinks/day) is independently associated with a worse outcome for ischemic stroke patients. To study the underlying mechanisms of this deleterious effect of HD, we performed an extensive analysis of the brain inflammatory responses of mice chronically exposed or not to 10% alcohol before and after ischemic stroke. Inflammatory responses were analyzed at the parenchymal, perivascular, and vascular levels by using transcriptomic, immunohistochemical, in vivo 2-photon microscopy and molecular MRI analyses. Alcohol-exposed mice show, in the absence of any other insult, a neurovascular inflammatory priming (i.e., an abnormal inflammatory status including an increase in brain perivascular macrophages [PVM]) associated with exacerbated inflammatory responses after a secondary insult (ischemic stroke or LPS challenge). Similar to our clinical data, alcohol-exposed mice showed larger ischemic lesions. We show here that PVM are key players on this aggravating effect of alcohol, since their specific depletion blocks the alcohol-induced aggravation of ischemic lesions. This study opens potentially new therapeutic avenues aiming at blocking alcohol-induced exacerbation of the neurovascular inflammatory responses triggered after ischemic stroke.

Authors

Antoine Drieu, Anastasia Lanquetin, Damien Levard, Martina Glavan, Francisco Campos, Aurélien Quenault, Eloïse Lemarchand, Mikaël Naveau, Anne Lise Pitel, José Castillo, Denis Vivien, Marina Rubio

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Figure 7

Perivascular macrophages (PVM) mediate the aggravating effect of chronic alcohol consumption on ischemic stroke in mice.

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Perivascular macrophages (PVM) mediate the aggravating effect of chronic...
(A) Experimental design to study the effects of chronic alcohol exposure on PVM. (B) Representative photomicrographs of PVM CD206+Iba1 (arrowheads) cells in control and alcohol-exposed mice. (C) Quantification of PVM (CD206+ cells). Scale bars: 20 μm. (D) Experimental design to deplete PVM in control and alcohol-exposed mice. (E) Representative in vivo Z stack of CX3CR1GFP+/– PBS/CLO–injected mice. Blood vessels are visualized through the i.v. injection of FITC-Dextran. Twenty-four hours after the i.c.v. injection of TRITC-Dextran, PVM can be in vivo visualized (note the absence of TRITC-Dextran signals in CLO-treated mice). Microglia are positive for GFP in CX3CR1GFP+/– mice. Scale bar: 100 μm. (F) Colocalization of CD206 and phagocyted TRITC-Dextran in PVM (epifluorescence microscopy). Three-dimensional visualization of a double-positive TRITC-Dextran and CD206 PVM for. Scale bar: 10 μm. (G) Representative photomicrographs of GFP+ microglial cells and CD206+ PVMs in PBS- and CLO-treated mice. Scale bar: 20 μm. (H and I) Quantification of PVM depletion by TRITC+ cell counting (H) and CD206+ counting (I). (J) The number of microglial cells remained unchanged after CLO treatment. (K) Representative T2-weighted MRI images showing ischemic lesions in PBS- and CLO-treated naive and alcohol-exposed mice 24 hours after stroke onset. (L) Quantification of lesion volumes. n = 5–6 mice per group; **P < 0.01, *P < 0.05 versus PBS; #P < 0.05 versus control. Mann-Whitney U test.