Department of Immunology, Mudanjiang Medical University, Mudanjiang, Heilongjiang 157011, P.R. China.
Department of Gastroenterology, Mudanjiang Forestry Central Hospital, Mudanjiang, Heilongjiang 157000, P.R. China.
Int J Mol Med. 2018 Jul;42(1):279-289. doi: 10.3892/ijmm.2018.3600. Epub 2018 Mar 29.
Fibrosis induces a progressive loss of liver function, thus leading to organ failure. Activins are secreted proteins that belong to the transforming growth factor (TGF)‑β superfamily, which initiate signaling by binding to their two type II receptors: Activin A receptor type 2A (ACVR2A) and activin A receptor type 2B. Previous studies that have explored the mechanisms underlying immune‑induced hepatic fibrosis have mainly focused on TGF‑β signaling, not activin signaling. To investigate the role of the activin pathway in this disease, adenovirus particles containing short hairpin (sh)RNA targeting ACVR2A mRNA (Ad‑ACVR2A shRNA) were administered to mice, which were chronically treated with concanavalin A (Con A). The pathological changes in the liver were evaluated with hematoxylin/eosin staining, Masson trichrome staining and immunohistochemical assay. The results detected an increase in serum activin A and liver ACVR2A in Con A‑treated animals. Conversely, liver function was partially restored and fibrotic injury was attenuated when activin signaling was blocked. In addition, the activation of hepatic stellate cells (HSCs) in response to Con A was suppressed by Ad‑ACVR2A shRNA, as evidenced by decreased α‑smooth muscle actin, and type I and IV collagen expression. Furthermore, primary mouse HSCs (mHSCs) were activated when exposed to interleukin (IL)‑17A or IL‑17F, which are two major cytokines produced by cluster of differentiation 4+ T helper 17 cells. The levels of activin A, type I and IV collagen were determined with ELISA kits and the expression of fibrotic molecules was determined with western blot analysis. Conversely, blocking activin/ACVR2A impaired the potency of HSCs to produce collagens in response to IL‑17s. In addition, C terminus phosphorylation of Smad2 on Ser465 and Ser467, induced by either Con A in the liver or by IL‑17s in mHSCs, was partly inhibited when activin A/ACVR2A signaling was suppressed. Collectively, the present study demonstrated an involvement of activated activin A/ACVR2A/Smad2 signaling in immune‑induced hepatic fibrosis.
纤维化导致肝功能进行性丧失,从而导致器官衰竭。激活素是属于转化生长因子 (TGF)‑β超家族的分泌蛋白,通过与两种 II 型受体:激活素 A 受体 2A (ACVR2A) 和激活素 A 受体 2B 结合来启动信号转导。先前研究免疫诱导肝纤维化的机制主要集中在 TGF‑β信号转导上,而不是激活素信号转导。为了研究激活素途径在这种疾病中的作用,用含有靶向 ACVR2A mRNA 的短发夹 (sh)RNA 的腺病毒颗粒 (Ad-ACVR2A shRNA) 处理慢性用伴刀豆球蛋白 A (Con A) 处理的小鼠。通过苏木精/伊红染色、Masson 三色染色和免疫组织化学检测评估肝组织的病理变化。结果检测到 Con A 处理动物的血清激活素 A 和肝 ACVR2A 增加。相反,当阻断激活素信号时,肝功能部分恢复,纤维化损伤减轻。此外,Ad-ACVR2A shRNA 抑制了肝星状细胞 (HSCs) 对 Con A 的激活,表现为 α-平滑肌肌动蛋白和 I 型和 IV 型胶原表达减少。此外,当暴露于白细胞介素 (IL)‑17A 或 IL‑17F 时,原代小鼠 HSCs (mHSCs) 被激活,IL-17A 和 IL-17F 是由 CD4+辅助性 T 细胞 17 细胞产生的两种主要细胞因子。通过 ELISA 试剂盒测定激活素 A、I 型和 IV 型胶原的水平,并通过 Western blot 分析测定纤维化分子的表达。相反,阻断激活素/ACVR2A 会损害 HSCs 在响应 IL-17s 时产生胶原蛋白的能力。此外,当抑制激活素 A/ACVR2A 信号转导时,Con A 在肝中或 IL-17s 在 mHSCs 中诱导的 Smad2 C 端丝氨酸 465 和丝氨酸 467 的磷酸化部分受到抑制。总之,本研究表明激活的激活素 A/ACVR2A/Smad2 信号转导参与了免疫诱导的肝纤维化。
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