Chia Nan University of Pharmacy & Science Institutional Repository:Item 310902800/23436
English  |  正體中文  |  简体中文  |  全文笔数/总笔数 : 18034/20233 (89%)
造访人次 : 23769734      在线人数 : 784
RC Version 7.0 © Powered By DSPACE, MIT. Enhanced by NTU Library IR team.
搜寻范围 查询小技巧:
  • 您可在西文检索词汇前后加上"双引号",以获取较精准的检索结果
  • 若欲以作者姓名搜寻,建议至进阶搜寻限定作者字段,可获得较完整数据
    •  进阶搜寻


    jsp.display-item.identifier=請使用永久網址來引用或連結此文件: https://ir.cnu.edu.tw/handle/310902800/23436


    標題: H2O2於人類口腔細胞誘導差異蛋白之表現
    Hydrogen Peroxide Induces Differentially Expressed Proteins in the Human Normal Oral Keratinocyte
    作者: 陳意卿
    貢獻者: 王四切
    鍾景宏
    嘉南藥理科技大學:藥物科技研究所
    關鍵字: 西方墨點法
    美白試劑
    二維膠電泳
    蛋白質學研究
    氧化性物質
    two-dimensional gel electrophoresis (2D-GE)
    reactive oxygen species(ROS)
    proteomic analysis
    dental bleaching agent
    日期: 2010
    上傳時間: 2010-12-30 15:34:09 (UTC+8)
    摘要: H2O2 (Hydrogen peroxide)廣泛用於美白試劑,H2O2不僅為美白成分,同時也為氧化性物質,而氧化性物質被認為雙重角色,亦會造成自由基與抗氧化平衡失調。
    根據J. A. ImLa文獻指出,氧化性物質濃度於1~3mM可誘導SOS修復系統來保護細胞,而嚴重暴露氧化性物質之結果則會產生凋亡反應。在我們過去實驗室C.H Chiu之研究數據,觀察到人類口腔細胞 (hNOK)暴露H2O2會造成細胞死亡,核DNA氧化損傷,mtDNA4977缺失和線粒體膜電位之變化。過量的H2O2促進牙齒漂白,但也造成的細胞損傷。為了達到牙齒美白且快速清除H2O2造成的氧化壓力,故本研究目的是將hNOK暴露H2O2,並以二維膠電泳 (two-dimensional gel electrophoresis, 2D-GE) 顯示受到暴露後細胞內蛋白質量的變化情形及利用西方墨點法探討粒線體內蛋白質(ND4、ND5、ND6和COII)之變化。二維膠片影像,利用軟體分析後有變化的蛋白質再利用質譜分析得到這些蛋白質身分鑑定,作為口腔細胞對過量的H2O2造成的氧化壓力找出預防方法。
    Hydrogen peroxide (H2O2) is predominate component for Dental bleaching agents. H2O2 is not only an active bleaching component but also acts as a reactive oxygen species (ROS). ROS, which is considered as dual role, depends on the imbalance between antioxidants and free radicals. In that, in J. A. ImLay articles cited that Mode I ROS dosage (1~3mM) induced SOS response to protect cells; under severe ROS exposure results in apoptotic response.
    In our previous data from C.H Chiu research observed the phenomena regarding to hNOK cell death, nuclear DNA oxidative damage, mtDNA4977 deletion and mitochondrial membrane potential change under exposure to H2O2.
    It suggested that the function of overdose H2O2 was paradoxical. They promoted tooth-bleaching, but caused cellular damage. In order to of achieve tooth-bleaching and remove quickly H2O2 mediated oxidative stress, this work is that investigate the proteomic regulation in hNOK. The differences in the levels of proteins extracted from hNOK cells with and without exposure to H2O2, were investigated using two-dimensional gel electrophoresis (2D-GE) display and western blot to investigate the mitochondrial DNA of the proteins (ND4, ND5, ND6 and CO II ).
    First, we identified 17 and 22 proteins from the comparison between 2D-GE maps with H2O2 or control in dose and time manner respectively. The down-regulation of cytoskeleton proteins may cause the cytoskeletal dissociation in time. The differential proteins of cyclophilin, TPC-1 subunit delta, annexin A2, calmodulin like protein 3 participate in early apoptotic stage under exposure to H2O2. Low dose of H2O2 induce ND5, COII and ND4, ND6 over-expression in seven and four day respectively. Expression decreased after the peak time in addition to ND6.Comprehensive experimental results, the dental bleaching agent can cause damage whether apoptosis is not clear.
    關聯: 校內校外均不公開,學年度:98,82頁
    显示于类别:[藥學系(所)] 博碩士論文

    文件中的档案:

    档案 描述 大小格式浏览次数
    index.html0KbHTML1检视/开启


    在CNU IR中所有的数据项都受到原著作权保护.

    TAIR相关文章

    DSpace Software Copyright © 2002-2004  MIT &  Hewlett-Packard  /   Enhanced by   NTU Library IR team Copyright ©   - 回馈