金属蛋白酶 22 通过激活 ERK 信号加速新生内膜形成。
A disintegrin and metalloprotease 22 accelerates neointima formation by activating ERK signaling.
机构信息
Department of Cardiology, Beijing Anzhen Hospital, Capital Medical University, National Clinical Research Center for Cardiovascular Diseases, Beijing, China.
Department of Cardiology, Beijing Anzhen Hospital, Capital Medical University, National Clinical Research Center for Cardiovascular Diseases, Beijing, China; Department of Geriatric Cardiology, Chinese PLA General Hospital, Beijing, China.
出版信息
Atherosclerosis. 2019 Apr;283:92-99. doi: 10.1016/j.atherosclerosis.2019.02.002. Epub 2019 Feb 11.
BACKGROUND AND AIMS
Despite the advantage of arterial expansion for life-threatening vascular pathologies, the occurrence of neointima formation remains a prominent complication, with the underlying mechanisms largely unknown. A disintegrin and metalloprotease 22 (ADAM22) belongs to the family of ADAMs that possesses various biological capacities regulating vascular physiopathology. However, little is known about ADAM22 in vascular smooth muscle cell (VSMC)-mediated neointima formation. Here, we aimed to evaluate the potential functional regulation of ADAM22 in neointima formation and to further explore the underlying mechanisms.
METHODS
In our study, platelet-derived growth factor-BB (PDGF-BB)-induced VSMC proliferation was examined using a 5-bromo-2'-deoxyuridine (BrdU) incorporation assay and a cell counting kit-8 (CCK8) assay, while VSMC migration was detected using a modified Boyden chamber method and a scratch-wound assay. The functional role of ADAM22 in neointima formation was evaluated based on a left carotid artery wire injury model in mice at 14 and 28 days.
RESULTS
ADAM22 was significantly up-regulated in both PDGF-BB-challenged VSMCs and restenotic arteries of mice. When ADAM22 was overexpressed in VSMCs, cell proliferation, migration and phenotypic switching were simultaneously aggravated, whereas the opposite was observed when ADAM22 was knocked down in vitro. In ADAM22 heterozygote mice, wire-injury induced neointima formation was significantly ameliorated compared to wild-type control mice. Mechanistically, significantly up-regulated ERK phosphorylation is closely involved in the regulatory effects of ADAM22 in neointima formation. Interestingly, an ERK inhibitor largely reversed the aggravated VSMCs migration, proliferation and phenotypic switching induced by ADAM22 overexpression.
CONCLUSIONS
Our results indicate that ADAM22 accelerates neointima formation by enhancing VSMC migration, proliferation and phenotypic switching via promoting ERK phosphorylation. Suppressing ADAM22 expression may be an effective strategy for ameliorating neointima formation.
背景与目的
尽管动脉扩张对于危及生命的血管病变具有优势,但新生内膜形成仍然是一个突出的并发症,其潜在机制在很大程度上尚不清楚。解整合素金属蛋白酶 22(ADAM22)属于 ADAMs 家族,具有调节血管病理生理学的多种生物学能力。然而,关于 ADAM22 在血管平滑肌细胞(VSMC)介导的新生内膜形成中的作用知之甚少。在这里,我们旨在评估 ADAM22 在新生内膜形成中的潜在功能调节作用,并进一步探讨其潜在机制。
方法
在我们的研究中,使用 5-溴-2'-脱氧尿苷(BrdU)掺入测定法和细胞计数试剂盒-8(CCK8)测定法检测血小板衍生生长因子-BB(PDGF-BB)诱导的 VSMC 增殖,使用改良 Boyden 室法和划痕愈合试验检测 VSMC 迁移。根据 14 天和 28 天小鼠左颈动脉线损伤模型,评估 ADAM22 在新生内膜形成中的功能作用。
结果
ADAM22 在 PDGF-BB 刺激的 VSMC 和小鼠再狭窄动脉中均显著上调。当 ADAM22 在 VSMC 中过表达时,细胞增殖、迁移和表型转换同时加重,而在体外敲低 ADAM22 时则观察到相反的结果。与野生型对照小鼠相比,ADAM22 杂合子小鼠的线损伤诱导的新生内膜形成明显改善。从机制上讲,ERK 磷酸化的显著上调与 ADAM22 在新生内膜形成中的调节作用密切相关。有趣的是,ERK 抑制剂在很大程度上逆转了 ADAM22 过表达引起的 VSMC 迁移、增殖和表型转换的加剧。
结论
我们的结果表明,ADAM22 通过促进 ERK 磷酸化来加速新生内膜形成,从而增强 VSMC 的迁移、增殖和表型转换。抑制 ADAM22 表达可能是改善新生内膜形成的有效策略。
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