[黄芪甲苷调节Snail1的乳酸化和乙酰化，介导巨噬细胞极化，改善心肌梗死]。

细胞与分子免疫学杂志 Pub Date : 2025-04-01

Shaopeng Chen, Rudian Kang, Xinbao Hong, Yilong Liu

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RAW246.7 cell-conditioned medium (CM) was co-cultured with H9c2 cells to assess the protective effects of AS-IV on macrophage CM-mediated H9c2 damage. RAW246.7 cells were induced to differentiate into M1-like macrophages using LPS (100 ng/mL) + IFN-γ (20 ng/mL), and Snail1 was overexpressed in M1 macrophages. Transfected M1 macrophage CM was co-cultured with H9c2 cells to validate the mechanisms of AS-IV in MI. An MI rat model was established by ligation of the left anterior descending coronary artery (LAD), and was treated with AS-IV. Cardiac function, myocardial cell apoptosis, and cardiac tissue pathology were studied using echocardiography, TUNEL, and HE staining, respectively. Results Compared to the OGD group, AS-IV treatment promoted cell viability, reduced apoptosis and decreased LDH release. LPS upregulated lactate levels in the supernatant of RAW246.7 cell cultures and induced polarization of RAW246.7 cells to the M1 phenotype. 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引用次数: 0

摘要

目的探讨黄芪甲苷（Astragaloside-IV, as - iv）通过巨噬细胞依赖机制调节Snail1的乳酸化、乙酰化及转化生长因子β (TGF-β)通路对心肌梗死（MI）进展的影响。方法采用氧糖剥夺法（OGD）建立大鼠心肌细胞（H9c2）体外心肌缺血模型，并给予AS-IV处理。CCK-8检测细胞活力，流式细胞术检测细胞凋亡，LDH水平检测细胞损伤。采用LPS处理RAW246.7细胞，ELISA法检测上清乳酸水平，Western blot法检测巨噬细胞表型标志物表达。RAW246.7细胞条件培养基（CM）与H9c2细胞共培养，评估AS-IV对巨噬细胞CM介导的H9c2损伤的保护作用。LPS (100 ng/mL) + IFN-γ (20 ng/mL)诱导RAW246.7细胞向M1样巨噬细胞分化，Snail1在M1巨噬细胞中过表达。转染后的M1巨噬细胞CM与H9c2细胞共培养，验证AS-IV在心肌梗死中的作用机制。结扎左冠状动脉前降支（LAD）建立心肌梗死大鼠模型，并给予AS-IV治疗。分别采用超声心动图、TUNEL染色、HE染色观察大鼠心功能、心肌细胞凋亡及心脏组织病理变化。结果与OGD组相比，AS-IV处理可提高细胞活力，减少细胞凋亡，降低LDH释放。LPS上调RAW246.7细胞培养上清中的乳酸水平，诱导RAW246.7细胞向M1表型极化。AS-IV可减弱RAW246.7细胞CM对H9c2细胞的损伤作用。Snail1在M1巨噬细胞中的过表达减弱了AS-IV对H9c2细胞的保护作用。体内研究结果显示，与心肌梗死组相比，AS-IV处理可降低心肌梗死大鼠心脏乳酸水平，改善心功能和心肌损伤，减轻心肌细胞凋亡。结论AS-IV通过抑制Snail1的乳酸化和乙酰化，以巨噬细胞依赖的方式抑制TGF-β通路的激活，从而减轻心肌梗死后心肌细胞的损伤。

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[Astragaloside IV regulates Snail1 lactylation and acetylation to mediate macrophage polarization and improve myocardial infarction].

Objective To investigate the impact of Astragaloside-IV (AS-IV) on the progression of myocardial infarction (MI) through macrophage-dependent mechanisms by regulating Snail1 lactylation and acetylation, as well as the transforming growth factor β (TGF-β) pathway. Methods Oxygen glucose deprivation (OGD) was used to establish an in vitro myocardial ischemia model in rat cardiomyocytes (H9c2), which were then treated with AS-IV. Cell viability was assessed using CCK-8, apoptosis was evaluated by flow cytometry, and LDH levels were measured to assess cellular damage. RAW246.7 cells were treated with LPS, and lactate levels in the supernatant were measured using ELISA, while expression of macrophage phenotype markers was evaluated using Western blot. RAW246.7 cell-conditioned medium (CM) was co-cultured with H9c2 cells to assess the protective effects of AS-IV on macrophage CM-mediated H9c2 damage. RAW246.7 cells were induced to differentiate into M1-like macrophages using LPS (100 ng/mL) + IFN-γ (20 ng/mL), and Snail1 was overexpressed in M1 macrophages. Transfected M1 macrophage CM was co-cultured with H9c2 cells to validate the mechanisms of AS-IV in MI. An MI rat model was established by ligation of the left anterior descending coronary artery (LAD), and was treated with AS-IV. Cardiac function, myocardial cell apoptosis, and cardiac tissue pathology were studied using echocardiography, TUNEL, and HE staining, respectively. Results Compared to the OGD group, AS-IV treatment promoted cell viability, reduced apoptosis and decreased LDH release. LPS upregulated lactate levels in the supernatant of RAW246.7 cell cultures and induced polarization of RAW246.7 cells to the M1 phenotype. AS-IV attenuated the damaging effects of RAW246.7 cell CM on H9c2 cells . Overexpression of Snail1 in M1 macrophages weakened the protective effects of AS-IV on H9c2 cells . In vivo study, results showed that, compared to the MI group, AS-IV treatment reduced lactate levels in the hearts of MI rats, improved cardiac function and myocardial injury and attenuated myocardial cell apoptosis. Conclusion AS-IV inhibits TGF-β pathway activation through the suppression of Snail1 lactylation and acetylation in a macrophage-dependent manner, thereby mitigating myocardial cell damage following MI.

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细胞与分子免疫学杂志

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