中国组织工程研究与临床康复
中國組織工程研究與臨床康複
중국조직공정연구여림상강복
JOURNAL OF CLINICAL REHABILITATIVE TISSUE ENGINEERING RESEARCH
2009年
28期
5544-5548
,共5页
田梅%易维京%余荣杰%吴雄飞
田梅%易維京%餘榮傑%吳雄飛
전매%역유경%여영걸%오웅비
晚期氧化蛋白产物%纯化%凝胶层析%人血白蛋白
晚期氧化蛋白產物%純化%凝膠層析%人血白蛋白
만기양화단백산물%순화%응효층석%인혈백단백
背景:晚期氧化蛋白产物是血液透析患者免疫功能紊乱、加速性动脉粥样硬化、透析相关性淀粉样变等长期并发症的重要致病环节.但是对于晚期氧化蛋白产物的基础性研究相对较少.主要原因之一就是不能获得高纯度且具有生物学活性的晚期氧化蛋白产物.目的:制备及纯化晚期氧化蛋白产物,并对其进行鉴定,以寻求一种制备高纯度且具生物活性的晚期氧化蛋白产物的方法.设计、时间及地点:单一样本观察,于2008-09/10在解放军第三军医大学检验系临床生化教研室完成.材料:人血白蛋白为成都容生有限公司产品,Hitrap 26/60 sephacryl S-300为GE Healthcare产品.方法:首先纯化人血白蛋白,将纯化的人血白蛋白与次氯酸体外孵育法制备晚期氧化蛋白产物一人血白蛋白,经Hitrap26/60sephacryl S-300分离纯化.并经变性及非变性电泳、分子筛蛋白标准鉴定其相对分子质量,经单核细胞肿瘤坏死因子α分泌实验鉴定其结构特征和生物学活性.主要观察指标:①人血白蛋白的纯化及电泳结果.②晚期氧化蛋白产物纯化及电泳结果.③晚期氧化蛋白产物-人血白蛋白促单核细胞肿瘤坏死因子α分泌的量效关系.结果:经变性及非变性电泳、分子筛蛋白标准鉴定其相对分子质量为670 000,能够显著刺激单核细胞肿瘤坏死因子α的分泌,时间效应显示AOPPs-HSA(1 g/L)刺激6 h,单核细胞肿瘤坏死因子α的分泌量就已显著性升高,12 h升至最高水平.结论:采用上述方法能够制备及纯化晚期氧化蛋白产物,且纯化后的晚期氧化蛋白产物具有生物学活性,为晚期氧化蛋白产物的进一步研究奠定了基础.
揹景:晚期氧化蛋白產物是血液透析患者免疫功能紊亂、加速性動脈粥樣硬化、透析相關性澱粉樣變等長期併髮癥的重要緻病環節.但是對于晚期氧化蛋白產物的基礎性研究相對較少.主要原因之一就是不能穫得高純度且具有生物學活性的晚期氧化蛋白產物.目的:製備及純化晚期氧化蛋白產物,併對其進行鑒定,以尋求一種製備高純度且具生物活性的晚期氧化蛋白產物的方法.設計、時間及地點:單一樣本觀察,于2008-09/10在解放軍第三軍醫大學檢驗繫臨床生化教研室完成.材料:人血白蛋白為成都容生有限公司產品,Hitrap 26/60 sephacryl S-300為GE Healthcare產品.方法:首先純化人血白蛋白,將純化的人血白蛋白與次氯痠體外孵育法製備晚期氧化蛋白產物一人血白蛋白,經Hitrap26/60sephacryl S-300分離純化.併經變性及非變性電泳、分子篩蛋白標準鑒定其相對分子質量,經單覈細胞腫瘤壞死因子α分泌實驗鑒定其結構特徵和生物學活性.主要觀察指標:①人血白蛋白的純化及電泳結果.②晚期氧化蛋白產物純化及電泳結果.③晚期氧化蛋白產物-人血白蛋白促單覈細胞腫瘤壞死因子α分泌的量效關繫.結果:經變性及非變性電泳、分子篩蛋白標準鑒定其相對分子質量為670 000,能夠顯著刺激單覈細胞腫瘤壞死因子α的分泌,時間效應顯示AOPPs-HSA(1 g/L)刺激6 h,單覈細胞腫瘤壞死因子α的分泌量就已顯著性升高,12 h升至最高水平.結論:採用上述方法能夠製備及純化晚期氧化蛋白產物,且純化後的晚期氧化蛋白產物具有生物學活性,為晚期氧化蛋白產物的進一步研究奠定瞭基礎.
배경:만기양화단백산물시혈액투석환자면역공능문란、가속성동맥죽양경화、투석상관성정분양변등장기병발증적중요치병배절.단시대우만기양화단백산물적기출성연구상대교소.주요원인지일취시불능획득고순도차구유생물학활성적만기양화단백산물.목적:제비급순화만기양화단백산물,병대기진행감정,이심구일충제비고순도차구생물활성적만기양화단백산물적방법.설계、시간급지점:단일양본관찰,우2008-09/10재해방군제삼군의대학검험계림상생화교연실완성.재료:인혈백단백위성도용생유한공사산품,Hitrap 26/60 sephacryl S-300위GE Healthcare산품.방법:수선순화인혈백단백,장순화적인혈백단백여차록산체외부육법제비만기양화단백산물일인혈백단백,경Hitrap26/60sephacryl S-300분리순화.병경변성급비변성전영、분자사단백표준감정기상대분자질량,경단핵세포종류배사인자α분비실험감정기결구특정화생물학활성.주요관찰지표:①인혈백단백적순화급전영결과.②만기양화단백산물순화급전영결과.③만기양화단백산물-인혈백단백촉단핵세포종류배사인자α분비적량효관계.결과:경변성급비변성전영、분자사단백표준감정기상대분자질량위670 000,능구현저자격단핵세포종류배사인자α적분비,시간효응현시AOPPs-HSA(1 g/L)자격6 h,단핵세포종류배사인자α적분비량취이현저성승고,12 h승지최고수평.결론:채용상술방법능구제비급순화만기양화단백산물,차순화후적만기양화단백산물구유생물학활성,위만기양화단백산물적진일보연구전정료기출.
BACKGROUND: Advanced oxidation protein products (AOPPs) are a crucial pathogenic link to such long-term uremic complications in hemodialysis patients as immune system dysregulation, accelerated atherosclerosis, dialysis-related amyloldosis and so on. However, basic studies on AOPPs are relatively few, and one of the main reasons is the fact that it is difficult to obtain AOPPs with high pudty and biological activity.OBJECTIVE: To prepare, pudfy and indentify AOPPs, with the hope of searching for a method of preparing AOPPs with high purity and biological activity.DESIGN, TIME AND SETTING: A single sample observation was completed in the Clinical Biochemistry Section of Ecsomatics Department, Third Military Medical University of Chinese PLA from September to November in 2008. MATERIALS: Human serum albumin (HSA) was provided by Chengdu Rongsheng Company Ltd. Hitrap 26/60 sephacryl S-300 was purchased from GE Healthcare.METHODS: Hypochloric acid was used in the oxidation of purified HSA to prepare in vitro the AOPPs-modified HSA (AOPPs-HSA), which was then isolated by Hitrap 26/60 sephacryl S-300. Relative molecular mass was determined by sodium dodecyl sulfate polyacrylamide gel electropheresis (SDS-PAGE), native polyacrylamide gel electrophoresis (PAGE) and molecular weight standards. Structural features and biological activities were identified in the experiment of tumor necrosis factor α (TNF-α) release from monocytes.MAIN OUTCOME MEASURES: ①The purification and gel electrophoresis results of HSA. ②The purification and gel electrophoresis results of AOPPs. ③The dose-effect relationship between AOPPs-HSA and TNF-α release from monocytes. RESULTS: The relative molecular mass of AOPPs-HSA was 670 000 according to SDS-PAGE, native PAGE and molecular weight standards. Moreover, AOPPs-HSA could encourage the release of TNF-α from monocytes. The time effects showed that TNF-α release volume significantly increased after 6 hours of stimulation by AOPPs-HSA (1 g/L) and reached a peak at hour 12. CONCLUSION: Highly purified and bioactive AOPPs can be successfully prepared by the above-mentioned method, which builds a basis for further study on AOPPs.
