生命科学研究
生命科學研究
생명과학연구
LIFE SCIENCE RESEARCH
2009年
6期
496-500
,共5页
张明香%符州%田代印%王莉佳%刘恩梅%戴继宏%罗征秀
張明香%符州%田代印%王莉佳%劉恩梅%戴繼宏%囉徵秀
장명향%부주%전대인%왕리가%류은매%대계굉%라정수
协同激活分子CBP%诱饵表达质粒%诱饵蛋白
協同激活分子CBP%誘餌錶達質粒%誘餌蛋白
협동격활분자CBP%유이표체질립%유이단백
co-activator CBP%bait expression plasmid%bait protein
构建协同激活分子CBP(CREB(cAMP response element binding)binding protein)的诱饵表这质拉pGSKT7-CBP并检测其蛋白表达、毒性和自激活作用.PcR扩增小鼠CBP的基因编码序列(CDS(coding sequence)序列)并克隆入诱饵表达载体pGBKT7中,通过酶切和测序鉴定后,把构建好的诱饵表达质粒pGBKT7-CBP转化到酵母AH109细胞中,Western blot检测诱饵蛋白表达情况,同时检测诱饵蛋白的毒性和自激活作用.结果成功扩增了小鼠CBP基因的CDS序列,并成功克隆到酵母诱饵表达载体pGBKT7中,测序结果正确.诱饵表达质粒成功转化到酵母AH109细胞中,Western blot分析结果证实酵母细胞高表达诱饵蛋白CBP,但诱饵蛋白有自激活作用.提示pGBKT7-CBP不能用于酵母双杂交或三杂交系统检测CBP与其他蛋白质或小分子的相互作用,对其他研究CBP生物学功能试验的方法选取具有一定的借鉴意义.
構建協同激活分子CBP(CREB(cAMP response element binding)binding protein)的誘餌錶這質拉pGSKT7-CBP併檢測其蛋白錶達、毒性和自激活作用.PcR擴增小鼠CBP的基因編碼序列(CDS(coding sequence)序列)併剋隆入誘餌錶達載體pGBKT7中,通過酶切和測序鑒定後,把構建好的誘餌錶達質粒pGBKT7-CBP轉化到酵母AH109細胞中,Western blot檢測誘餌蛋白錶達情況,同時檢測誘餌蛋白的毒性和自激活作用.結果成功擴增瞭小鼠CBP基因的CDS序列,併成功剋隆到酵母誘餌錶達載體pGBKT7中,測序結果正確.誘餌錶達質粒成功轉化到酵母AH109細胞中,Western blot分析結果證實酵母細胞高錶達誘餌蛋白CBP,但誘餌蛋白有自激活作用.提示pGBKT7-CBP不能用于酵母雙雜交或三雜交繫統檢測CBP與其他蛋白質或小分子的相互作用,對其他研究CBP生物學功能試驗的方法選取具有一定的藉鑒意義.
구건협동격활분자CBP(CREB(cAMP response element binding)binding protein)적유이표저질랍pGSKT7-CBP병검측기단백표체、독성화자격활작용.PcR확증소서CBP적기인편마서렬(CDS(coding sequence)서렬)병극륭입유이표체재체pGBKT7중,통과매절화측서감정후,파구건호적유이표체질립pGBKT7-CBP전화도효모AH109세포중,Western blot검측유이단백표체정황,동시검측유이단백적독성화자격활작용.결과성공확증료소서CBP기인적CDS서렬,병성공극륭도효모유이표체재체pGBKT7중,측서결과정학.유이표체질립성공전화도효모AH109세포중,Western blot분석결과증실효모세포고표체유이단백CBP,단유이단백유자격활작용.제시pGBKT7-CBP불능용우효모쌍잡교혹삼잡교계통검측CBP여기타단백질혹소분자적상호작용,대기타연구CBP생물학공능시험적방법선취구유일정적차감의의.
To construct the bait expression plasmid pGBKT7-CBP(CREB(cAMP response element binding)binding protein)of co-activator CBP and detect its protein expression,toxicity and self-activation,the CDS (coding sequence)sequence of mouse CBP was amplified by PCR,and then was cloned into pGBKT7.After being verified by cutting and sequencing,it was transformed into yeast cells AH109 and the expression of the bait protein was analyzed by Western blot.Toxicity and self-activation of the bait protein were detected.It Was demonstrated that the CDS sequence of motlse CBP Was amplified and cloned into pGBKT7 successfully,the bait expression plasmid Waa transformed into yeast cells AH109 successfully and was verified self-activated,the expression of the bait protein was confirmed by Western blot.This indicate that the full-length CDS sequence of CBP couldn't be used as bait in yeast two or three hybrid system,and is of important significance for other study related to the interaction of CBP with other proteins and small moleculars.
