乙醇和乙醛对胰腺星状细胞的激活作用:是否由丝裂原活化蛋白激酶信号通路介导?
Pancreatic stellate cell activation by ethanol and acetaldehyde: is it mediated by the mitogen-activated protein kinase signaling pathway?
作者信息
McCarroll J A, Phillips P A, Park S, Doherty E, Pirola R C, Wilson J S, Apte M V
机构信息
Pancreatic Research Group, The University of New South Wales, Sydney, Australia.
出版信息
Pancreas. 2003 Aug;27(2):150-60. doi: 10.1097/00006676-200308000-00008.
BACKGROUND
Pancreatic fibrosis is a characteristic feature of alcoholic chronic pancreatitis. Recent studies suggest that activated pancreatic stellate cells (PSCs) are the major cell-type involved in pancreatic fibrogenesis. Cultured PSCs become activated when exposed to ethanol or its metabolite acetaldehyde (as indicated by increased alpha-smooth muscle actin [alpha-SMA] expression and increased collagen synthesis). However the intracellular signaling mechanisms responsible for ethanol- or acetaldehyde-induced PSC activation remain to be fully elucidated. One of the major signaling pathways known to regulate protein synthesis in mammalian cells is the mitogen-activated protein kinase (MARK) pathway.
AIMS
To examine the effects of ethanol and acetaldehyde on the MAPK pathway (by assessing the activities of the 3 major subfamilies (extracellular-regulated kinases 1 and 2 [ERK 1/2], JNK and p38 kinase) in PSCs and to examine the role of p38 kinase in mediating the ethanol- and acetaldehyde-induced increase in alpha-SMA expression in activated rat PSCs.
METHODS
Rat PSCs were incubated with ethanol (50 mM) or acetaldehyde (200 microM) for 15 min, 30 min, 60 min, and 24 h; and activities of ERK 1/2, JNK, and p38 kinase were assessed in cell lysates using kinase assays and Western blot. In addition, rat PSCs were treated with the specific p38 MAPK inhibitor SB203580 in the presence or absence of ethanol or acetaldehyde for 24h, and activation of the downstream protein kinase MAPKAP kinase-2 (an indicator of p38 MAPK activity) was assessed by Western blot. Specific inhibitors were also used to inhibit the activity of ERK 1/2 and JNK. Following inhibition of the above signaling pathways, alpha-SMA expression by PSCs was assessed by Western blot.
RESULTS
Ethanol and acetaldehyde increased the activation of all 3 subfamilies (ERK 1/2, JNK and p38 kinase) of the MAPK pathway in PSCs. Treatment of PSCs with SB203580 abolished the ethanol- and acetaldehyde-induced increase in p38 MAPK activity and also prevented the induction of alpha-SMA expression in PSCs. However, inhibition of ERK 1/2 and JNK had no effect on ethanoland acetaldehyde-induced alpha-SMA expression in PSCs.
CONCLUSIONS
(1) The MAP kinase pathway is induced in PSCs after exposure to ethanol or acetaldehyde and this induction is sustained for at least 24h. (2) The p38 MAPK pathway mediates the activation (as indicated by increased alpha-SMA expression) of PSCs by ethanol or acetaldehyde.
背景
胰腺纤维化是酒精性慢性胰腺炎的一个特征性表现。最近的研究表明,活化的胰腺星状细胞(PSC)是参与胰腺纤维化形成的主要细胞类型。培养的PSC在暴露于乙醇或其代谢产物乙醛时会被激活(表现为α-平滑肌肌动蛋白[α-SMA]表达增加和胶原蛋白合成增加)。然而,负责乙醇或乙醛诱导的PSC激活的细胞内信号传导机制仍有待充分阐明。已知调节哺乳动物细胞蛋白质合成的主要信号通路之一是丝裂原活化蛋白激酶(MARK)通路。
目的
研究乙醇和乙醛对MAPK通路的影响(通过评估PSC中3个主要亚家族(细胞外调节激酶1和2[ERK 1/2]、JNK和p38激酶)的活性),并研究p38激酶在介导乙醇和乙醛诱导的活化大鼠PSC中α-SMA表达增加中的作用。
方法
将大鼠PSC与乙醇(50 mM)或乙醛(200 μM)孵育15分钟、30分钟、60分钟和24小时;使用激酶测定法和蛋白质印迹法评估细胞裂解物中ERK 1/2、JNK和p38激酶的活性。此外,在存在或不存在乙醇或乙醛的情况下,用特异性p38 MAPK抑制剂SB203580处理大鼠PSC 24小时,并通过蛋白质印迹法评估下游蛋白激酶MAPKAP激酶-2(p38 MAPK活性的指标)的活化情况。还使用特异性抑制剂抑制ERK 1/2和JNK的活性。在抑制上述信号通路后,通过蛋白质印迹法评估PSC的α-SMA表达。
结果
乙醇和乙醛增加了PSC中MAPK通路所有3个亚家族(ERK 1/2、JNK和p38激酶)的活化。用SB203580处理PSC消除了乙醇和乙醛诱导的p38 MAPK活性增加,也阻止了PSC中α-SMA表达的诱导。然而,抑制ERK 1/2和JNK对乙醇和乙醛诱导的PSC中α-SMA表达没有影响。
结论
(1)PSC在暴露于乙醇或乙醛后诱导MAP激酶通路,且这种诱导至少持续24小时。(2)p38 MAPK通路介导乙醇或乙醛对PSC的激活(表现为α-SMA表达增加)。
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