Section of Surgery, Department of Clinical Sciences, Malmö, Sweden.
Section of Islet Pathophysiology, Department of Clinical Sciences, Malmö, Sweden.
Gastroenterology. 2015 Dec;149(7):1920-1931.e8. doi: 10.1053/j.gastro.2015.08.026. Epub 2015 Aug 22.
BACKGROUND & AIMS: Neutrophils are involved in the development of acute pancreatitis (AP), but it is not clear how neutrophil-induced tissue damage is regulated. In addition to secreting antimicrobial compounds, activated neutrophils eliminate invading microorganisms by expelling nuclear DNA and histones to form extracellular web-like structures called neutrophil extracellular traps (NETs). However, NETs have been reported to contribute to organ dysfunction in patients with infectious diseases. We investigated whether NETs contribute to the development of AP in mice.
AP was induced in C57BL/6 mice by infusion of taurocholate into the pancreatic duct or by intraperitoneal administration of L-arginine. Pancreata were collected and extracellular DNA was detected by Sytox green staining, levels of CXC chemokines, histones, and cytokines also were measured. Cell-free DNA was quantified in plasma samples. Signal transducer and activator of transcription 3 phosphorylation and trypsin activation were analyzed in isolated acinar cells. NETs were depleted by administration of DNase I to mice. Plasma was obtained from healthy individuals (controls) and patients with severe AP.
Infusion of taurocholate induced formation of NETs in pancreatic tissues of mice and increased levels of cell-free DNA in plasma. Neutrophil depletion prevented taurocholate-induced deposition of NETs in the pancreas. Administration of DNase I to mice reduced neutrophil infiltration and tissue damage in the inflamed pancreas and lung, and decreased levels of blood amylase, macrophage inflammatory protein-2, interleukin 6, and high-mobility groups protein 1. In mice given taurocholate, DNase I administration also reduced expression of integrin α M (macrophage-1 antigen) on circulating neutrophils. Similar results occurred in mice with L-arginine-induced AP. Addition of NETs and histones to acinar cells induced formation of trypsin and activation of signal transducer and activator of transcription 3; these processes were blocked by polysialic acid. Patients with severe AP had increased plasma levels of NET components compared with controls.
NETs form in the pancreata of mice during the development of AP, and NET levels are increased in plasma from patients with AP, compared with controls. NETs regulate organ inflammation and injury in mice with AP, and might be targeted to reduce pancreatic tissue damage and inflammation in patients.
中性粒细胞参与急性胰腺炎(AP)的发生发展,但中性粒细胞诱导的组织损伤如何调控尚不清楚。除了分泌抗菌化合物外,活化的中性粒细胞还通过排出核 DNA 和组蛋白形成细胞外网状结构,即中性粒细胞胞外诱捕网(NETs)来消灭入侵的微生物。然而,已有报道称 NETs 有助于感染性疾病患者的器官功能障碍。我们研究了 NETs 是否会导致小鼠发生 AP。
通过向胰管内输注牛磺胆酸钠或腹腔内注射 L-精氨酸诱导 C57BL/6 小鼠发生 AP。收集胰腺组织,通过 Sytox green 染色检测细胞外 DNA,测量 CXC 趋化因子、组蛋白和细胞因子的水平。定量分析血浆样本中的无细胞 DNA。分析分离的腺泡细胞中信号转导和转录激活因子 3 的磷酸化和胰蛋白酶激活情况。用 DNA 酶 I 处理小鼠以耗竭 NETs。采集健康个体(对照组)和重症 AP 患者的血浆。
牛磺胆酸钠输注诱导小鼠胰腺组织中形成 NETs,并增加血浆中无细胞 DNA 的水平。中性粒细胞耗竭可阻止牛磺胆酸钠诱导的 NETs 在胰腺中的沉积。用 DNA 酶 I 处理小鼠可减少胰腺和肺炎症部位的中性粒细胞浸润和组织损伤,降低血淀粉酶、巨噬细胞炎症蛋白-2、白细胞介素 6 和高迁移率族蛋白 1 的水平。在给予牛磺胆酸钠的小鼠中,DNA 酶 I 的给药还降低了循环中性粒细胞上整合素 α M(巨噬细胞-1 抗原)的表达。在 L-精氨酸诱导的 AP 小鼠中也观察到类似的结果。NETs 和组蛋白添加到腺泡细胞中诱导胰蛋白酶的形成和信号转导和转录激活因子 3 的激活;这些过程被多聚唾液酸阻断。与对照组相比,重症 AP 患者的 NET 成分血浆水平升高。
AP 发生时,小鼠胰腺中形成 NETs,与对照组相比,AP 患者的 NET 水平升高。NETs 调节 AP 小鼠的器官炎症和损伤,可能成为减少患者胰腺组织损伤和炎症的靶点。
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