过氧化物酶体增殖物激活受体-γ 的激活与减少肝脏缺血再灌注损伤和改变组织驻留巨噬细胞极化有关在一个小鼠模型。
PPAR-gamma activation is associated with reduced liver ischemia-reperfusion injury and altered tissue-resident macrophages polarization in a mouse model.
机构信息
Multi Organ Transplant Program, Toronto General Hospital, Toronto, ON, Canada.
Consejo Nacional de Ciencia y Tecnología, México City, México.
出版信息
PLoS One. 2018 Apr 4;13(4):e0195212. doi: 10.1371/journal.pone.0195212. eCollection 2018.
BACKGROUND
PPAR-gamma (γ) is highly expressed in macrophages and its activation affects their polarization. The effect of PPAR-γ activation on Kupffer cells (KCs) and liver ischemia-reperfusion injury (IRI) has not yet been evaluated. We investigated the effect of PPAR-γ activation on KC-polarization and IRI.
MATERIALS AND METHODS
Seventy percent (70%) liver ischemia was induced for 60mins. PPAR-γ-agonist or vehicle was administrated before reperfusion. PPAR-γ-antagonist was used to block PPAR-γ activation. Liver injury, necrosis, and apoptosis were assessed post-reperfusion. Flow-cytometry determined KC-phenotypes (pro-inflammatory Nitric Oxide +, anti-inflammatory CD206+ and anti-inflammatory IL-10+).
RESULTS
Liver injury assessed by serum AST was significantly decreased in PPAR-γ-agonist versus control group at all time points post reperfusion (1hr: 3092±105 vs 4469±551; p = 0.042; 6hr: 7041±1160 vs 12193±1143; p = 0.015; 12hr: 5746±328 vs 8608±1259; p = 0.049). Furthermore, liver apoptosis measured by TUNEL-staining was significantly reduced in PPAR-γ-agonist versus control group post reperfusion (1hr:2.46±0.49 vs 6.90±0.85%;p = 0.001; 6hr:26.40±2.93 vs 50.13±8.29%; p = 0.048). H&E staining demonstrated less necrosis in PPAR-γ-agonist versus control group (24hr:26.66±4.78 vs 45.62±4.57%; p = 0.032). The percentage of pro-inflammatory NO+ KCs was significantly lower at all post reperfusion time points in the PPAR-γ-agonist versus control group (1hr:28.49±4.99 vs 53.54±9.15%; p = 0.040; 6hr:5.51±0.54 vs 31.12±9.58%; p = 0.009; 24hr:4.15±1.50 vs 17.10±4.77%; p = 0.043). In contrast, percentage of anti-inflammatory CD206+ KCs was significantly higher in PPAR-γ-agonist versus control group prior to IRI (8.62±0.96 vs 4.88 ±0.50%; p = 0.04). Administration of PPAR-γ-antagonist reversed the beneficial effects on AST, apoptosis, and pro-inflammatory NO+ KCs.
CONCLUSION
PPAR-γ activation reduces IRI and decreases the pro-inflammatory NO+ Kupffer cells. PPAR-γ activation can become an important tool to improve outcomes in liver surgery through decreasing the pro-inflammatory phenotype of KCs and IRI.
背景
过氧化物酶体增殖物激活受体-γ (PPAR-γ) 在巨噬细胞中高度表达,其激活影响巨噬细胞的极化。PPAR-γ 激活对枯否细胞(KCs)和肝缺血再灌注损伤(IRI)的影响尚未得到评估。我们研究了 PPAR-γ 激活对 KC 极化和 IRI 的影响。
材料和方法
诱导 70%的肝脏缺血 60 分钟。再灌注前给予 PPAR-γ 激动剂或载体。使用 PPAR-γ 拮抗剂阻断 PPAR-γ 激活。再灌注后评估肝损伤、坏死和细胞凋亡。流式细胞术确定 KC 表型(促炎型一氧化氮+,抗炎型 CD206+和抗炎型 IL-10+)。
结果
与对照组相比,再灌注后所有时间点的血清天冬氨酸转氨酶(AST)评估的肝损伤在 PPAR-γ 激动剂组均显著降低(1 小时:3092±105 比 4469±551;p=0.042;6 小时:7041±1160 比 12193±1143;p=0.015;12 小时:5746±328 比 8608±1259;p=0.049)。此外,与对照组相比,PPAR-γ 激动剂组再灌注后肝凋亡(通过 TUNEL 染色测量)显著减少(1 小时:2.46±0.49 比 6.90±0.85%;p=0.001;6 小时:26.40±2.93 比 50.13±8.29%;p=0.048)。H&E 染色显示 PPAR-γ 激动剂组比对照组的坏死更少(24 小时:26.66±4.78 比 45.62±4.57%;p=0.032)。与对照组相比,再灌注后所有时间点的促炎型一氧化氮+ KC 的百分比在 PPAR-γ 激动剂组均显著降低(1 小时:28.49±4.99 比 53.54±9.15%;p=0.040;6 小时:5.51±0.54 比 31.12±9.58%;p=0.009;24 小时:4.15±1.50 比 17.10±4.77%;p=0.043)。相反,在 IRI 之前,PPAR-γ 激动剂组抗炎型 CD206+ KC 的百分比明显高于对照组(8.62±0.96 比 4.88±0.50%;p=0.04)。给予 PPAR-γ 拮抗剂逆转了 AST、细胞凋亡和促炎型一氧化氮+ KC 的有益作用。
结论
PPAR-γ 激活可减轻 IRI,并减少促炎型一氧化氮+ KC。PPAR-γ 激活可通过减少 KC 的促炎表型和 IRI,成为改善肝外科治疗效果的重要手段。
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