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作 者:梁本甲[1] 高会杰[1] 刘松[1] 王奔[1] 王健[1] 彭程[1] 牛卫博[1] 牛军[1]
机构地区:[1]山东大学齐鲁医院肝胆外科,山东济南250012
出 处:《中国现代普通外科进展》2012年第10期757-761,共5页Chinese Journal of Current Advances in General Surgery
基 金:国家自然科学基金资助项目(30872460)
摘 要:目的:探讨整合素αvβ6对核转录因子Ets-1表达的影响,明确αvβ6-ERK2直接连接在该过程中发挥的作用。方法:流式细胞仪检测各结肠癌SW480细胞表面αvβ6的表达;采用Westernblotting法分别检测ERK表达、活化水平和Ets-1的表达水平。结果:SW480β6和SW480β6Del.mutant细胞均表达αvβ6;SW480β6细胞Ets-1的表达量较SW480细胞明显增多(P<0.05),同时ERK的磷酸化水平(p-ERK)也明显升高,而总ERK(t-ERK)表达水平二者无明显差异;SW480β6Del.mutant细胞ERK2的磷酸化水平较SW480β6细胞明显降低;SW480β6Del.mutant细胞和PD98059处理的SW480β6细胞Ets-1的表达水平明显低于对照组(P<0.05)。结论:整合素αvβ6通过αvβ6-ERK2直接连接提高ERK2的磷酸化水平,从而促进结肠癌SW480细胞核转录因子Ets-1表达。Objective: To explore the effects of the integrin αvβ6 on the expression of nuclear transcription factor Ets-1,and to determine the role of αvβ6-ERK2 direct binding in this process.Methods: FACScan analyses were applied to detect the αvβ6 expression in colon cancer cell SW480 groups.The expression and activation level of ERK,as well as the expression level of Ets-1 were detected by western blotting.Results: Both SW480β6 and SW480β6Del.mutant cells were expressing αvβ6.The amount of Ets-1 expression in SW480β6 cells was higher than that in SW480 cells.Compared with SW480β6 cells,the level of phosphorylated ERK(p-ERK)decreased in SW480 cells,with no significant change on total ERK(t-ERK) expression.The SW480β6Del.mutant cells lacking the ERK2 binding sites reduce the amount of phosphorylated ERK2.Both PD98059 treated SW480β6 cells and SW480β6Del.mutant cells had a lower level of Ets-1 expression than control groups.Conclusion: Integrin αvβ6 promotes the phosphorylation of ERK2 through αvβ6-ERK2 direct binding,thereby facilitating the Ets-1 expression.
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