Zhou Jian, Menko A Sue
Department of Pathology, Anatomy and Cell Biology, Thomas Jefferson University, Philadelphia, Pennsylvania 19107, USA.
Invest Ophthalmol Vis Sci. 2004 Jul;45(7):2314-23. doi: 10.1167/iovs.03-1210.
The goals of this study were to determine whether MAP kinase signaling pathways play a role in the formation of lens cataracts and to examine the potential signaling relationship between Src and MAP kinases in signaling the induction of lens opacities.
Embryonic day (E)10 chick lenses were cultured in Medium 199 containing 10% fetal bovine serum. The activation state of Src kinases and the MAP kinases extracellular signal-regulated protein kinase (ERK), c-jun N-terminal kinase (JNK), and p38 in the lens epithelium was determined over a time course from 10 minutes to 10 days in culture by immunoblot analysis. Src kinase activation was suppressed by exposure to the Src family kinase-specific inhibitor PP1. To examine the role of specific MAP kinases in the development of lens opacities, lenses were grown for 10 days in the presence or absence of inhibitors of ERK (U0126), JNK (SP600125), and p38 (SB203580). Lenses were observed and photographed daily, and the degree of opacification was quantified by using image-analysis software.
Within a short time after placing embryonic lenses in culture conditions that induce the formation of cataracts, there occurred a great increase in the activation state of the MAP kinase ERK. Activation of ERK was both rapid and transient. No activation of the MAP kinase JNK was observed in the cataract cultures beyond that which occurred in normal lens epithelium, even though JNK activation is often linked to the cellular response to stress. In contrast, although p38 activation was barely detected in the normal embryonic lens, this stress-activated protein kinase exhibited a robust activation in cataract cultures that was sustained throughout the culture period. Studies conducted to map the cataract signaling pathways indicate that the p38 MAP kinase functions upstream of the Src kinase. To analyze the potential role of ERK, JNK, and p38 in cataract induction, lenses were cultured in the presence of specific MAP kinase inhibitors. Although the inhibitors of ERK and JNK did not interfere with the formation of cataract, p38 inhibitors blocked the development of lens opacities with an efficacy similar to that of the Src kinase inhibitor PP1.
Activation of both Src and p38 kinases lead to the induction of cataract.
本研究的目的是确定丝裂原活化蛋白激酶(MAP)信号通路是否在晶状体白内障形成中起作用,并研究Src与MAP激酶之间在晶状体混浊诱导信号传导中的潜在信号关系。
将胚胎第10天(E10)的鸡晶状体在含有10%胎牛血清的199培养基中培养。通过免疫印迹分析,在培养10分钟至10天的时间过程中,测定晶状体上皮中Src激酶以及MAP激酶细胞外信号调节蛋白激酶(ERK)、c-Jun氨基末端激酶(JNK)和p38的活化状态。通过暴露于Src家族激酶特异性抑制剂PP1来抑制Src激酶活化。为了研究特定MAP激酶在晶状体混浊发展中的作用,将晶状体在有或无ERK抑制剂(U0126)、JNK抑制剂(SP600125)和p38抑制剂(SB203580)的情况下培养10天。每天观察并拍摄晶状体,使用图像分析软件对混浊程度进行量化。
在将胚胎晶状体置于诱导白内障形成的培养条件后的短时间内,MAP激酶ERK的活化状态大幅增加。ERK的活化既迅速又短暂。在白内障培养物中,未观察到MAP激酶JNK的活化超过正常晶状体上皮中的活化,尽管JNK活化通常与细胞对应激的反应相关。相反,尽管在正常胚胎晶状体中几乎未检测到p38活化,但这种应激激活的蛋白激酶在白内障培养物中表现出强烈活化,并在整个培养期间持续存在。绘制白内障信号通路的研究表明,p38 MAP激酶在Src激酶的上游发挥作用。为了分析ERK、JNK和p38在白内障诱导中的潜在作用,在存在特定MAP激酶抑制剂的情况下培养晶状体。尽管ERK和JNK抑制剂不干扰白内障的形成,但p38抑制剂以与Src激酶抑制剂PP1相似的效力阻断晶状体混浊的发展。
Src和p38激酶的活化均导致白内障的诱导。
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