中国组织工程研究
中國組織工程研究
중국조직공정연구
Journal of Clinical Rehabilitative Tissue Engineering Research
2015年
37期
5961-5965
,共5页
孙鸣宇%闫承慧%田孝祥%李洋%韩雅玲
孫鳴宇%閆承慧%田孝祥%李洋%韓雅玲
손명우%염승혜%전효상%리양%한아령
组织构建%组织工程%巨噬细胞%E1A激活基因阻遏子%溶酶体%动脉粥样硬化%国家自然科学基金
組織構建%組織工程%巨噬細胞%E1A激活基因阻遏子%溶酶體%動脈粥樣硬化%國傢自然科學基金
조직구건%조직공정%거서세포%E1A격활기인조알자%용매체%동맥죽양경화%국가자연과학기금
背景:以往研究证实,CREG是一种与M6P/IGFⅡR直接结合的溶酶体蛋白,并依赖于与M6P受体的相互作用有效转运至溶酶体。<br> 目的:分析外源性CREG蛋白与溶酶体组织蛋白酶和M6P/IGFⅡR的相互作用关系及其对M6P/IGFⅡR表达变化及细胞内定位的影响。<br> 方法:应用细胞免疫荧光双染和免疫共沉淀方法,观察外源性 CREG 蛋白与溶酶体组织蛋白酶和 M6P/IGFⅡR的相互作用关系,并应用gain-of-function和loss-of-function模型,通过Western blot和细胞免疫荧光双染方法,观察CREG对M6P/IGFⅡR表达变化及细胞内定位的影响。<br> 结果与结论:细胞免疫荧光双染和免疫共沉淀方法证实外源性 CREG 蛋白与溶酶体组织蛋白酶和 M6P/IGFⅡR有直接相互作用关系;应用gain-of-function和loss-of-function模型进一步证实,CREG对M6P/IGFⅡR表达变化无影响,而影响其在细胞内的定位。提示外源性CREG蛋白定位于溶酶体,且与溶酶体组织蛋白酶和M6P/IGFⅡR有相互作用关系,并影响M6P/IGFⅡR的细胞内定位。
揹景:以往研究證實,CREG是一種與M6P/IGFⅡR直接結閤的溶酶體蛋白,併依賴于與M6P受體的相互作用有效轉運至溶酶體。<br> 目的:分析外源性CREG蛋白與溶酶體組織蛋白酶和M6P/IGFⅡR的相互作用關繫及其對M6P/IGFⅡR錶達變化及細胞內定位的影響。<br> 方法:應用細胞免疫熒光雙染和免疫共沉澱方法,觀察外源性 CREG 蛋白與溶酶體組織蛋白酶和 M6P/IGFⅡR的相互作用關繫,併應用gain-of-function和loss-of-function模型,通過Western blot和細胞免疫熒光雙染方法,觀察CREG對M6P/IGFⅡR錶達變化及細胞內定位的影響。<br> 結果與結論:細胞免疫熒光雙染和免疫共沉澱方法證實外源性 CREG 蛋白與溶酶體組織蛋白酶和 M6P/IGFⅡR有直接相互作用關繫;應用gain-of-function和loss-of-function模型進一步證實,CREG對M6P/IGFⅡR錶達變化無影響,而影響其在細胞內的定位。提示外源性CREG蛋白定位于溶酶體,且與溶酶體組織蛋白酶和M6P/IGFⅡR有相互作用關繫,併影響M6P/IGFⅡR的細胞內定位。
배경:이왕연구증실,CREG시일충여M6P/IGFⅡR직접결합적용매체단백,병의뢰우여M6P수체적상호작용유효전운지용매체。<br> 목적:분석외원성CREG단백여용매체조직단백매화M6P/IGFⅡR적상호작용관계급기대M6P/IGFⅡR표체변화급세포내정위적영향。<br> 방법:응용세포면역형광쌍염화면역공침정방법,관찰외원성 CREG 단백여용매체조직단백매화 M6P/IGFⅡR적상호작용관계,병응용gain-of-function화loss-of-function모형,통과Western blot화세포면역형광쌍염방법,관찰CREG대M6P/IGFⅡR표체변화급세포내정위적영향。<br> 결과여결론:세포면역형광쌍염화면역공침정방법증실외원성 CREG 단백여용매체조직단백매화 M6P/IGFⅡR유직접상호작용관계;응용gain-of-function화loss-of-function모형진일보증실,CREG대M6P/IGFⅡR표체변화무영향,이영향기재세포내적정위。제시외원성CREG단백정위우용매체,차여용매체조직단백매화M6P/IGFⅡR유상호작용관계,병영향M6P/IGFⅡR적세포내정위。
BACKGROUND:It has been found that cel ular repressor of E1A-stimulated genes (CREG) is a lysosomal protein binding directly to the mannose-6-phosphate (M6P)/insulin-like growth factor II receptor (IGFIIR) and depends on the interaction with M6P receptors for efficient delivery to lysosomes OBJECTIVE:To study the interactions between the exogenous CREG protein and cathepsins and M6P/IGFIIR and to confirm the effect of CREG protein on expression and distribution of M6P/IGFIIR. METHODS:Double-stained immunofluorescence and coimmunoprecipitation were applied to observe the interactions between the exogenous CREG protein and cathepsin B, cathepsin L and M6P/IGFIIR. Using gain-of-function and loss-of-function approaches, the effect of CREG on expression and distribution of M6P/IGFIIR were studied by western blot assay and immunofluorescence staining. RESULTS AND CONCLUSION:Double-stained immunofluorescence and coimmunoprecipitation analyses confirmed the direct interactions between the exogenous CREG protein and cathepsin B, cathepsin L and M6P/IGFIIR. It was verified that CREG plays a critical role not in the expression but in the distribution of M6P/IGFIIR using gain-of-function and loss-of-function approaches. These findings provide evidence that exogenous CREG protein is located in lysosomes and has interactions with cathepsins and M6P/IGFIIR, also CREG plays a critical role in the distribution of M6P/IGFIIR.
