Seizure progression and inflammatory mediators promote pericytosis and pericyte-microglia clustering at the cerebrovasculature

被引:57
作者
Klement, Wendy [1 ]
Garbelli, Rita [3 ]
Zub, Emma [1 ]
Rossini, Laura [3 ]
Tassi, Laura [4 ]
Girard, Benoit [2 ]
Blaquiere, Marine [1 ]
Bertaso, Federica [2 ]
Perroy, Julie [2 ]
de Bock, Frederic [1 ]
Marchi, Nicola [1 ]
机构
[1] Univ Montpellier, Inst Funct Genom, Lab Cerebrovasc Mech Brain Disorders, UMR CNRS INSERM 5203 U1191, Montpellier, France
[2] Univ Montpellier, Inst Funct Genom, Lab Pathophysiol Synapt Transmiss, UMR CNRS INSERM 5203 U1191, Montpellier, France
[3] Fdn IRCCS, Inst Neurol C, Clin Epileptol & Expt Neurophysiol Unit, Milan, Italy
[4] Osped Niguardo, C Munari Epilepsy Surg Ctr, Milan, Italy
关键词
Pericytes; Blood-brain barrier; Inflammation; Microglia; Epilepsy; BLOOD-BRAIN-BARRIER; CONSENSUS CLASSIFICATION; MICROVASCULAR PERICYTES; STATUS EPILEPTICUS; ADAPTIVE IMMUNITY; TASK-FORCE; CELLS; EPILEPTOGENESIS; NEUROGENESIS; ELIMINATION;
D O I
10.1016/j.nbd.2018.02.002
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
Background: Cerebrovascular dysfunction and inflammation occur in epilepsy. Here we asked whether pericytes, a pivotal cellular component of brain capillaries, undergo pathological modifications during experimental epileptogenesis and in human epilepsy. We evaluated whether pro-inflammatory cytokines, present in the brain during seizures, contribute to pericyte morphological modifications. Methods: In vivo, unilateral intra-hippocampal kainic acid (KA) injections were performed in NG2DsRed/C57BL6 mice to induce status epilepticus (SE), epileptogenesis, and spontaneous recurrent seizures (SRS). NG2DsRed mice were used to visualize pericytes during seizure progression. The effect triggered by recombinant IL-1 beta, TNF alpha, or IL-6 on pericytes was evaluated in NG2DsRed hippocampal slices and in human-derived cell culture. Human brain specimens obtained from temporal lobe epilepsy (TLE) with or without sclerosis (HS) and focal cortical dysplasia (FCD-IIb) were evaluated for pericyte-microglial cerebrovascular assembly. Results: A disarray of NG2DsRed pericyte soma and ramifications was found 72 h post-SE and 1 week post-SE (epileptogenesis) in the hippocampus. Pericyte modifications topographically overlapped with IBA1(+) microglia clustering around the capillaries with cases of pericytes lodged within the microglial cells. Microglial clustering around the NG2DsRed pericytes lingered at SRS. Pericyte proliferation (Ki67(+)) occurred 72 h post-SE and during epileptogenesis and returned towards control levels at SRS. Human epileptic brain tissues showed pericyte-microglia assemblies with IBA1/HLA microglial cells outlining the capillary wall in TLE-HS and FCD-IIb specimens. Inflammatory mediators contributed to pericyte modifications, in particular IL-1 beta elicited pericyte morphological changes and pericyte-microglia clustering in NG2DsRed hippocampal slices. Modifications also occurred when pro-inflammatory cytokines were added to an in vitro culture of pericytes. Conclusions: These results indicate the occurrence of pericytosis during seizures and introduce a pericyte-microglial mediated mechanism of blood-brain barrier dysfunction in epilepsy.
引用
收藏
页码:70 / 81
页数:12
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