生物技术通报
生物技術通報
생물기술통보
BIOTECHNOLOGY BULLETIN
2009年
11期
83-88
,共6页
黄思超%杜军%邱胜红%徐俊%傅刘鹏%马锦珊%蔡绍晖
黃思超%杜軍%邱勝紅%徐俊%傅劉鵬%馬錦珊%蔡紹暉
황사초%두군%구성홍%서준%부류붕%마금산%채소휘
IκBα缺失突变体%载体构建NF-κB
IκBα缺失突變體%載體構建NF-κB
IκBα결실돌변체%재체구건NF-κB
IκBα%Deletion mutant%Vector construction%NF-κB
旨在构建缺失N端前36个氨基酸的IκBα突变体真核表达载体,并对其表达及生物学活性进行检测.从人源子宫颈癌细胞HeLa中提取总RNA,利用RT-PCR的方法获得IκBα缺失突变体的cDNA,将其克隆至真核表达载体pcDNA3.1/myc-His A中,构建重组载体pcDNA3.1-IκBαΔN.通过PCR方法、NcoⅠ酶切以及核酸测序分析对其进行鉴定;采用Western Blot检测IκBα缺失突变体蛋白在HeLa细胞中的表达.将pcDNA3.1-IκBαΔN和pNF-κB-Luc共转染 HeLa细胞,经TNF-α诱导后,利用萤光素酶报告系统来检测重组载体对NF-αB的抑制活性.结果表明,经PCR方法、NcoⅠ酶切鉴定及核酸测序分析后,证实成功构建了重组载体pcDNA3.1-IκBαΔN;IκBα缺失突变体蛋白在HeLa细胞中高效表达,并对NF-κB有显著的抑制活性(P<0.01).因此,真核表达载体pcDNA3.1-IκBαΔN构建成功,为一步研究NF-κB信号传导通路及其相关疾病提供有效的分子工具.
旨在構建缺失N耑前36箇氨基痠的IκBα突變體真覈錶達載體,併對其錶達及生物學活性進行檢測.從人源子宮頸癌細胞HeLa中提取總RNA,利用RT-PCR的方法穫得IκBα缺失突變體的cDNA,將其剋隆至真覈錶達載體pcDNA3.1/myc-His A中,構建重組載體pcDNA3.1-IκBαΔN.通過PCR方法、NcoⅠ酶切以及覈痠測序分析對其進行鑒定;採用Western Blot檢測IκBα缺失突變體蛋白在HeLa細胞中的錶達.將pcDNA3.1-IκBαΔN和pNF-κB-Luc共轉染 HeLa細胞,經TNF-α誘導後,利用螢光素酶報告繫統來檢測重組載體對NF-αB的抑製活性.結果錶明,經PCR方法、NcoⅠ酶切鑒定及覈痠測序分析後,證實成功構建瞭重組載體pcDNA3.1-IκBαΔN;IκBα缺失突變體蛋白在HeLa細胞中高效錶達,併對NF-κB有顯著的抑製活性(P<0.01).因此,真覈錶達載體pcDNA3.1-IκBαΔN構建成功,為一步研究NF-κB信號傳導通路及其相關疾病提供有效的分子工具.
지재구건결실N단전36개안기산적IκBα돌변체진핵표체재체,병대기표체급생물학활성진행검측.종인원자궁경암세포HeLa중제취총RNA,이용RT-PCR적방법획득IκBα결실돌변체적cDNA,장기극륭지진핵표체재체pcDNA3.1/myc-His A중,구건중조재체pcDNA3.1-IκBαΔN.통과PCR방법、NcoⅠ매절이급핵산측서분석대기진행감정;채용Western Blot검측IκBα결실돌변체단백재HeLa세포중적표체.장pcDNA3.1-IκBαΔN화pNF-κB-Luc공전염 HeLa세포,경TNF-α유도후,이용형광소매보고계통래검측중조재체대NF-αB적억제활성.결과표명,경PCR방법、NcoⅠ매절감정급핵산측서분석후,증실성공구건료중조재체pcDNA3.1-IκBαΔN;IκBα결실돌변체단백재HeLa세포중고효표체,병대NF-κB유현저적억제활성(P<0.01).인차,진핵표체재체pcDNA3.1-IκBαΔN구건성공,위일보연구NF-κB신호전도통로급기상관질병제공유효적분자공구.
It was to construct a eukaryotic expression vector of IκBα mutant deleted N-terminal aminos from 1 to 36, and to i-dentify its expression and bioactivity. Total RNA was extracted from human cervical cancer HeLa cells, and cDNA of IκBα deletion mutant was obtained by RT-PCR method. The mutant gene was cloned into the eukaryotic expression plasm id pcDNA3. 1/ myc-His (A) to construct the recombinant vector pcDNA3. 1-IκBα△N. PCR method,Nco I digestion and DNA sequencing analysis were -employed to identify the recombinant vector. The expression of IκBα deletion mutant was detected by Western Blot. HeLa cells were co-transfected with pcDNA3. 1-IκBα△N and pNF-κB-Luc. Then,after the induction of TNF-α,its inhibitory effect on NF-κB was tested by Luciferase Assay System. Result indicated that the recombinant vector pcDNA3. 1 -IκBα△N was confirmed by PCR method, Nco I digestion and DNA sequencing analysis. The IκBα△N gene was expressed in HeLa cells and the deletion mutant protein had displayed obvious inhibitory effect on NF-κB (P <0.01 ). Therefore,the pcDNA3. 1-IκBα△N,a eukaryotic expression vector of IκBα deletion mutant,was constructed successfully. It provides a potent molecular tool for further study of NF-kB signal transduction pathway and related diseases.
