| Literature DB >> 29445758 |
Lingmin Shao1, Xingping Qin1, Jia Liu1, Zhihong Jian1, Xiaoxing Xiong1, Renzhong Liu1.
Abstract
Cerebral aneurysms (CAs) have become a health burden not only because their rupture is life threatening, but for a series of devastating complications left in survivors. It is well accepted that sustained chronic inflammation plays a crucial role in the pathology of cerebral aneurysms. In particular, macrophages have been identified as critical effector cells orchestrating inflammation in CAs. In recent years, dysregulated M1/M2 polarization has been proposed to participate in the progression of CAs. Although the pathological mechanisms of M1/M2 imbalance in CAs remain largely unknown, recent advances have been made in the understanding of the molecular basis and other immune cells involving in this sophisticated network. We provide a concise overview of the mechanisms associated with macrophage plasticity and the emerging molecular targets.Entities:
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Year: 2017 PMID: 29445758 PMCID: PMC5763122 DOI: 10.1155/2017/8160589
Source DB: PubMed Journal: J Immunol Res ISSN: 2314-7156 Impact factor: 4.818
Figure 1Mechanisms of macrophage polarization. Activation of IRF/STAT signaling pathways by IFN and TLR signaling skews macrophage function toward the M1 phenotype (via STAT1), while activation of IRF/STAT (via STAT6) signaling pathways by IL-4 and IL-13 skews macrophage function toward the M2 phenotype. PPARγ and ERK 5 participate in the promotion of M2 macrophage in cerebral aneurysms. NLRP3 inflammasome may contribute to M1 polarization.
Figure 2Summary of mediators and immune cells involved in M1/M2 polarization. The proinflammatory cytokines released by neutrophil, Th1 cells, and mast cells contribute to the maintenance of classically activated macrophage. Polarized M1 cells increase inflammation gene expression, promoting the progression of cerebral aneurysm to rupture. Conversely, alternatively activated macrophages may halt aneurysm rupture by facilitating inflammation regression. MMP indicates matrix metalloproteinase.