在角膜上皮中，丝裂原活化蛋白激酶（MAP激酶）级联反应由血小板活化因子（PAF）激活。

A mitogen-activated protein kinase (MAP-kinase) cascade is stimulated by platelet activating factor (PAF) in corneal epithelium.

作者信息

Bazan H E, Varner L

机构信息

Louisiana State University Medical School, LSU Eye Center, New Orleans 70112, USA.

出版信息

Curr Eye Res. 1997 Apr;16(4):372-9. doi: 10.1076/ceyr.16.4.372.10699.

DOI:10.1076/ceyr.16.4.372.10699

PMID:9134327

Abstract

PURPOSE

The mitogen-activated protein kinases (MAPK) are a family of important proteins that respond to a variety of receptor-mediated stimuli and can link events occurring at the cell membrane with changes in the nucleus. In this study we investigate the effect of platelet activating factor (PAF), a lipid mediator formed in the cornea after injury, on the activation of a MAPK cascade in the rabbit corneal epithelium.

METHODS

Rabbit corneas were incubated with or without 500 nM PAF. PAF antagonists BN50730 or 50727 (10 microM) were added 10 min before PAF and the epithelium scraped and homogenated. To determine the enzymatic activity of MAPK and MAPK-kinase (MEK1 and MEK2), a 100,000 x g cytosolic fraction was used directly, fractionated by DE-52 cellulose or immunoprecipitated with antibodies. Activities of MAPK and MEK were assayed in the presence of myelin basic protein (MBP) as substrate (for MAPK) activity or inactive extracellular-signal regulated protein kinase (ERK2 or MAPK). Western blot analysis was performed using anti-ERK2, anti-MEK1, and anti-MEK2 antibodies.

RESULTS

Corneal tissue expresses ERK2 or MAPK, and both MEK1 and MEK2, the immediate upstream regulators of MAPK. PAF produces a rapid activation of MEK, as measured by in vitro kinase assays using either inactive ERK2 as substrate or a MAPK fraction obtained by DE-52 chromatography. There was a subsequent activation of MAPK, the maximal activity of which occurs 15 min after stimulation by PAF. PAF antagonists blocked the MEK/MAPK cascade, suggesting that the activation was by a receptor-mediated mechanism.

CONCLUSIONS

The evidence presented here, that a MAPK cascade is rapidly activated by PAF in the corneal epithelium, suggests that this signal transduction mechanism can be involved in the increased expression of collagenase and other protease genes, as well as in the activation of phospholipase A2, events that occur in the corneal epithelium after PAF stimuli.

摘要

目的

丝裂原活化蛋白激酶（MAPK）是一类重要的蛋白质家族，可对多种受体介导的刺激作出反应，并能将细胞膜上发生的事件与细胞核内的变化联系起来。在本研究中，我们探究了血小板活化因子（PAF）（一种损伤后在角膜中形成的脂质介质）对兔角膜上皮中MAPK级联反应激活的影响。

方法

将兔角膜在有或无500 nM PAF的条件下孵育。在加入PAF前10分钟添加PAF拮抗剂BN50730或50727（10 μM），然后刮取上皮并匀浆。为测定MAPK和MAPK激酶（MEK1和MEK2）的酶活性，直接使用100,000×g胞质组分，通过DE-52纤维素分级分离或用抗体进行免疫沉淀。在以髓鞘碱性蛋白（MBP）作为底物（用于MAPK活性）或无活性的细胞外信号调节蛋白激酶（ERK2或MAPK）存在的情况下测定MAPK和MEK的活性。使用抗ERK2、抗MEK1和抗MEK2抗体进行蛋白质免疫印迹分析。

结果

角膜组织表达ERK2或MAPK，以及MAPK的直接上游调节因子MEK1和MEK2。通过使用无活性的ERK2作为底物或通过DE-52色谱法获得的MAPK组分进行体外激酶测定，结果显示PAF可快速激活MEK。随后MAPK被激活，其最大活性在PAF刺激后15分钟出现。PAF拮抗剂阻断了MEK/MAPK级联反应，表明这种激活是通过受体介导的机制。