基于NLRP3炎症小体探讨白芍总苷胶囊改善急性肺损伤的作用机制

基于NOD样受体热蛋白结构域相关蛋白3(NOD-like receptor thermal protein domain associated protein 3,NLRP3)炎症小体信号通路探讨白芍总苷胶囊(total glucosides of White Paeony Capsules,TGP)对急性肺损伤(acute lung injury,ALI)模型小鼠的改善作用及分子机制。在小鼠原代骨髓巨噬细胞(bone marrow-derived macrophages,BMDMs)上建立NLRP3炎症小体活化模型,通过蛋白免疫印迹(Western blot,WB)、免疫荧光染色、酶联免疫吸附实验(enzyme-linked immunosorbent assay,ELISA)和流式细胞术探究其分子机制。将C57BL/6J小鼠随机分为空白组、TGP组、模型组(LPS组)、LPS+TGP低剂量组、LPS+TGP高剂量组、LPS+MCC950组、LPS+MCC950+TGP组,每组8只,建立小鼠ALI模型。最后,收集肺泡灌洗液(bronchoalveolar lavage fluid,BALF)以及肺组织。测定各组小鼠肺指数及肺重湿干比,通过苏木精-伊红(HE)染色技术分析肺部组织的病理学变化,使用流式细胞术检测各组BALF中中性粒细胞数量,采用ELISA法测定BALF中白细胞介素(interleukin,IL)-1β、IL-6、肿瘤坏死因子(tumor necrosis factor,TNF)-α含量,实时荧光定量PCR(quantitative real-time,RT-qPCR)法测定肺组织中IL-1β、IL-18、IL-6、TNF-α的基因表达。结果表明TGP通过抑制上游线粒体活性氧(mitochondrial reactive oxygen species,mtROS)的产生以及随后的凋亡相关斑点(apoptosis-associated speck,ASC)的寡聚化,显著阻断了NLRP3炎症小体的激活。此外,在小鼠ALI模型中,与空白组相比,模型组肺组织出现肺泡结构破裂,肺泡间隔增厚,肺指数及肺重湿干比明显增高,中性粒细胞数量显著增加,炎性因子水平明显升高;与模型组相比,TGP和MCC950各组的肺组织病理形态明显改善,肺指数和肺重湿干比明显减低,中性粒细胞数量显著减少,炎性因子水平显著下调;值得注意的是,与MCC950组相比,MCC950+TGP组效果无明显差异。综上,该研究揭示了白芍总苷胶囊可能是通过抑制NLRP3炎症小体的激活从而改善小鼠ALI,也提供了一种安全有效的防治ALI/ARDS的候选药物。

甘草活性成分对抗抑郁药诱导的肝损伤的防治作用

由于现代精神疾病发病率的激增,抗抑郁药的应用增加。然而,令人担忧的是,抗抑郁药诱导的肝损伤已经逐渐成为严重的健康负担。此外,由于人们对抗抑郁药肝毒性的认知大多来源于药物警戒和临床病例报告,而缺乏观察性的研究,所以对其潜在的分子机制知之甚少并且缺乏有效的治疗策略。在该研究中,抗抑郁药帕罗西汀(paroxetine)直接触发了炎症小体(inflammasome)的活化,表现为caspase-1的成熟和下游效应因子interleukin(IL)-1β的分泌,并且这种活化可以经甘草活性成分刺甘草查尔酮(echinatin)的预处理完全阻断。另外,研究还发现,刺甘草查尔酮有效地抑制了帕罗西汀诱导的炎症小体非依赖性的肿瘤坏死因子α(tumor necrosis factor-α, TNF-α)的产生。从机制上讲,线粒体活性氧(mitochondrial reactive oxygen species, mtROS)的累积是帕罗西汀诱导炎症小体活化的关键上游事件,并且可以被刺甘草查尔酮显著抑制。在脂多糖(lipopolysaccharide, LPS)介导的特异质性药物性肝损伤(idiosyncratic drug-induced liver injury, IDILI)模型中,LPS与抗抑郁药帕罗西汀共同暴露于小鼠触发了炎症小体的异常活化从而诱导了特异质肝毒性,而这种损伤可以通过刺甘草查尔酮预处理得到改善。值得注意的是,此研究还发现甘草的多种活性成分对帕罗西汀触发的炎症小体活化有显著的抑制作用,同时,多种抗抑郁药诱导的炎症小体异常活化可以被刺甘草查尔酮预处理完全阻断。总而言之,该研究为抗抑郁药诱导肝损伤的机制提供了新的见解,同时为抗抑郁药肝毒性的治疗提供了一种新的策略。

Schisandra chinensis Oil Attenuates Aristolochic Acid Ⅰ-Induced Nephrotoxicity in vivo and in vitro

Objective: To investigate the protective effects of Schisandra chinensis oil(SCEO) against aristolochic acid Ⅰ(AAⅠ)-induced nephrotoxicity in vivo and in vitro and elucidate the underlying mechanism.Methods: C57BL/6 mice were randomly divided into 5 groups according to a random number table, including control group, AAⅠ group, and AAⅠ+SCEO(0.25, 0.5 and 1 g/kg) groups(n=5 per group). Pretreatment with SCEO was done for 2 days by oral administration, while the control and AAⅠ groups were treated with sodium carboxymethyl cellulose. Mice of all groups except for the control group were injected intraperitoneally with AAⅠ(5 mg/kg) from day 3 until day 7. Histopathological examination and apoptosis of kidney tissue were observed by hematoxylin and eosin and TdT-mediated dUTP nick-end labeling(TUNEL) staining, respectively. The levels of serum alanine aminotransferase(ALT), aspartate aminotransferase(AST), blood urea nitrogen(BUN), and serum creatinine(SCr), as well as renal malondialdehyde(MDA), glutathione, r-glutamyl cysteingl+glycine(GSH), and superoxide dismutase(SOD) were analyzed using enzyme-linked immunosorbent assay(ELISA).Expressions of hepatic cytochrome P450 1A1(CYP1A1), CYP1A2, and nad(p)hquinonedehydrogenase1(NQO1) were analyzed using ELISA, quantitative real-time polymerase chain reaction(qPCR) and Western blot,respectively. In vitro, SCEO(40 μg/mL) was added 12 h before treatment with AAⅠ(40 μmol/mL for 48 h) in human renal proximal tubule cell line(HK-2), then apoptosis and reactive oxygen species(ROS) were analyzed by flow cytometry. Results: SCEO 0.5 and 1 g/kg ameliorated histopathological changes and TUNEL+ staining in the kidney tissues of mice with AAⅠ-induced nephrotoxicity, and reduced serum levels of ALT, AST, BUN and SCr(P<0.01 or P<0.05). SCEO 0.5 and 1 g/kg alleviated the ROS generation in kidney, containing MDA,GSH and SOD(P<0.01 or P<0.05). SCEO 1 g/kg increased the expressions of CYP1A1 and CYP1A2 and decreased NQO1 level in the liver tissues(P<0.01 or P<0.05). Besides, in vitro studies also demonstrated that SCEO 40 μg/mL inhibited apoptosis and ROS generation(P<0.05 or P<0.01). Conclusions: SCEO can alleviate AAⅠ-induced kidney damage both in vivo and in vitro. The protective mechanism may be closely related to the regulation of metabolic enzymes, thereby inhibiting apoptosis and ROS production.