中华实验外科杂志
中華實驗外科雜誌
중화실험외과잡지
CHINESE JOURNAL OF EXPERIMENTAL SURGERY
2012年
11期
2159-2161
,共3页
张中林%艾勇彪%张吉发%袁玉蜂%刘志苏%何跃明
張中林%艾勇彪%張吉髮%袁玉蜂%劉誌囌%何躍明
장중림%애용표%장길발%원옥봉%류지소%하약명
血管生成素2%噬菌体抗体展示肽库%单链抗体
血管生成素2%噬菌體抗體展示肽庫%單鏈抗體
혈관생성소2%서균체항체전시태고%단련항체
Angiopoietin 2%Phage display peptide library%Single-chain antibody
目的 用纯化的人血管生成素2(Ang2)蛋白,通过噬菌体展示技术从非免疫小鼠噬菌体展示抗体库中淘选、鉴定Ang2单链抗体.方法 以纯化的人Ang2蛋白为抗原,对非免疫小鼠噬菌体展示抗体库进行富集和筛选,获得Ang2单链抗体,利用十二烷基硫酸钠-聚丙烯酰胺凝胶电泳(SDS-PAGE)和Western blot法检测目的蛋白的表达并测序.结果 经过3轮富集和筛选,获得了1个能特异性识别Ang2蛋白的阳性噬菌体克隆,DNA测序表明其含有完整的单链抗体基因片段,大小约750 bp,表达蛋白相对分子质量约33.7×103;通过SDS-PAGE进一步实现Ang2单链抗体(phage-Ang2-scFv)的鉴定.结论 成功分离并鉴定人Ang2-scFv,为进一步的功能学研究奠定了基础.
目的 用純化的人血管生成素2(Ang2)蛋白,通過噬菌體展示技術從非免疫小鼠噬菌體展示抗體庫中淘選、鑒定Ang2單鏈抗體.方法 以純化的人Ang2蛋白為抗原,對非免疫小鼠噬菌體展示抗體庫進行富集和篩選,穫得Ang2單鏈抗體,利用十二烷基硫痠鈉-聚丙烯酰胺凝膠電泳(SDS-PAGE)和Western blot法檢測目的蛋白的錶達併測序.結果 經過3輪富集和篩選,穫得瞭1箇能特異性識彆Ang2蛋白的暘性噬菌體剋隆,DNA測序錶明其含有完整的單鏈抗體基因片段,大小約750 bp,錶達蛋白相對分子質量約33.7×103;通過SDS-PAGE進一步實現Ang2單鏈抗體(phage-Ang2-scFv)的鑒定.結論 成功分離併鑒定人Ang2-scFv,為進一步的功能學研究奠定瞭基礎.
목적 용순화적인혈관생성소2(Ang2)단백,통과서균체전시기술종비면역소서서균체전시항체고중도선、감정Ang2단련항체.방법 이순화적인Ang2단백위항원,대비면역소서서균체전시항체고진행부집화사선,획득Ang2단련항체,이용십이완기류산납-취병희선알응효전영(SDS-PAGE)화Western blot법검측목적단백적표체병측서.결과 경과3륜부집화사선,획득료1개능특이성식별Ang2단백적양성서균체극륭,DNA측서표명기함유완정적단련항체기인편단,대소약750 bp,표체단백상대분자질량약33.7×103;통과SDS-PAGE진일보실현Ang2단련항체(phage-Ang2-scFv)적감정.결론 성공분리병감정인Ang2-scFv,위진일보적공능학연구전정료기출.
Objective To identify and purifyt single-chain antibody against angiopoietin 2 (Ang2-scFv) by phage display technology from non-immune mouse antibody phage display library by purified human angiopoietin2 protein,which will lay foundation for further functional studies of Ang2-scFv.Methods By using purified human angiopoietin2 protein as antigen,Ang2-scFv was screened from the non-immune mice phage display antibody library.The target protein expression was detected by using sodium dodecyl sulfate polyacrylamide gel electropheresis (SDS-PAGE) and Western blotting,and DNA of the 750 bp Ang2-scFv gene was sequenced.Results After three rounds of planning,one positive clone with specifically binding ability to angiopoietin2 protein was obtained.DNA sequencing showed that it contained a complete single-chain antibody fragment.Identification and purification of the Ang2-scFv was realized by SDSPAGE technique.Conclusion We successfully separated and purified the Ang2-scFv protein,which lay the foundation for the further functional studies of the single-chain antibody.
