生物技术通讯
生物技術通訊
생물기술통신
LETTERS IN BIOTECHNOLOGY
2013年
4期
457-461
,共5页
樊红艳%刘树玲%房婷%杨秀旭%于长明
樊紅豔%劉樹玲%房婷%楊秀旭%于長明
번홍염%류수령%방정%양수욱%우장명
人前列腺干细胞抗原%单克隆抗体%可变区序列%5'RACE
人前列腺榦細胞抗原%單剋隆抗體%可變區序列%5'RACE
인전렬선간세포항원%단극륭항체%가변구서렬%5'RACE
human prostate stem cell antigen%monoclonal antibody%variable region%5′RACE
目的:克隆并分析抗人前列腺干细胞抗原单克隆抗体轻链和重链的可变区基因。方法:从分泌抗人前列腺干细胞抗原单克隆抗体的杂交瘤细胞株中提取总RNA,根据小鼠IgG恒定区序列设计特异性引物,通过5′RACE法扩增其轻链和重链的可变区基因,克隆入pMD18-T载体,测序并分析其可变区序列。结果:3株抗人前列腺干细胞抗原单克隆抗体的重链可变区基因序列全长均为423 bp,编码141个氨基酸残基;轻链可变区基因序列全长均为393 bp,编码131个氨基酸残基;在GenBank中对氨基酸序列进行比对分析,均符合小鼠IgG可变区基因的特征;根据Kabat法则对3株抗体轻链和重链可变区氨基酸序列进行分析,确定了3个抗原互补决定区、4个框架区和前导肽。结论:通过5'RACE法得到了3株抗人前列腺干细胞抗原单克隆抗体轻链与重链可变区基因,为进一步研究抗体三维结构、人源化改造奠定了基础。
目的:剋隆併分析抗人前列腺榦細胞抗原單剋隆抗體輕鏈和重鏈的可變區基因。方法:從分泌抗人前列腺榦細胞抗原單剋隆抗體的雜交瘤細胞株中提取總RNA,根據小鼠IgG恆定區序列設計特異性引物,通過5′RACE法擴增其輕鏈和重鏈的可變區基因,剋隆入pMD18-T載體,測序併分析其可變區序列。結果:3株抗人前列腺榦細胞抗原單剋隆抗體的重鏈可變區基因序列全長均為423 bp,編碼141箇氨基痠殘基;輕鏈可變區基因序列全長均為393 bp,編碼131箇氨基痠殘基;在GenBank中對氨基痠序列進行比對分析,均符閤小鼠IgG可變區基因的特徵;根據Kabat法則對3株抗體輕鏈和重鏈可變區氨基痠序列進行分析,確定瞭3箇抗原互補決定區、4箇框架區和前導肽。結論:通過5'RACE法得到瞭3株抗人前列腺榦細胞抗原單剋隆抗體輕鏈與重鏈可變區基因,為進一步研究抗體三維結構、人源化改造奠定瞭基礎。
목적:극륭병분석항인전렬선간세포항원단극륭항체경련화중련적가변구기인。방법:종분비항인전렬선간세포항원단극륭항체적잡교류세포주중제취총RNA,근거소서IgG항정구서렬설계특이성인물,통과5′RACE법확증기경련화중련적가변구기인,극륭입pMD18-T재체,측서병분석기가변구서렬。결과:3주항인전렬선간세포항원단극륭항체적중련가변구기인서렬전장균위423 bp,편마141개안기산잔기;경련가변구기인서렬전장균위393 bp,편마131개안기산잔기;재GenBank중대안기산서렬진행비대분석,균부합소서IgG가변구기인적특정;근거Kabat법칙대3주항체경련화중련가변구안기산서렬진행분석,학정료3개항원호보결정구、4개광가구화전도태。결론:통과5'RACE법득도료3주항인전렬선간세포항원단극륭항체경련여중련가변구기인,위진일보연구항체삼유결구、인원화개조전정료기출。
Objective: To clone and analyze the genes of light chain variable region(VL) and heavy chain vari-able region(VH) of monoclonal antibody(mAb) against human prostate stem cell antigen(PSCA). Methods: Total RNA was extracted from hybridoma cells which secrete mAb against human PSCA.Then VH and VL genes were amplified by 5'RACE with specific primers designed to match the high conservative nucleotide sequence of con-stant regions of mouse IgG. The PCR products were inserted into pMD18-T vector, followed by sequencing and analysis. Results: For each anti-PSCA mAb, VH gene contained 423 bp and encoded 141 amino acids, and the VL gene contained 393 bp and encoded 131 amino acids. They were homologous with the variable region of mouse IgG in GenBank. According to Kabat's rules, there were 4 framework regions, 3 complementarity determin-ing regions and a leader sequence in the VH and VL gene respectively.Conclusion: Acquisition of genes of the VH and VL of the anti-human PSCA mAbs will be a experimental basis for subsequent study of the mAb's 3D structure or humanization of antibody.
