黑龙江八一农垦大学学报
黑龍江八一農墾大學學報
흑룡강팔일농은대학학보
JOURNAL OF HEILONGJIANG AUGUST FIRST LAND RECLAMATION UNIVERSITY
2011年
6期
31-35
,共5页
郭丽%杨焕民%于志国%计红%符亚原
郭麗%楊煥民%于誌國%計紅%符亞原
곽려%양환민%우지국%계홍%부아원
籽鹅%催乳素基因%克隆%表达%Western%blot
籽鵝%催乳素基因%剋隆%錶達%Western%blot
자아%최유소기인%극륭%표체%Western%blot
zi goose%prolactin%cloning%prokaryotic expression%western blot
运用RT-PCR方法,获得籽鹅脑垂体催乳素(Prolactin,PRL)基因编码区序列cDNA,克隆到pMD18-T载体上。DNA序列分析表明,PRL cDNA全长690 bp,编码230个氨基酸残基,与皖西白鹅的碱基同源性达99.57%,氨基酸同源性达99.56%。将所得序列与表达载体pET-32 a(+)构建表达质粒pET-32 a(+)-PRL。该质粒的DH5α转化菌经终浓度为1 mmoL.L-1的IPTG在37℃环境下诱导5 h可表达PRL基因融合蛋白,表达量约占菌体总蛋白的29.63%。用纯化的融合蛋白和凝血酶酶切后的单体蛋白主动免疫小白鼠,经Western blot检测,所制抗体清晰地检测到PRL基因表达蛋白的特异带,由此证明PRL基因的融合蛋白和凝血酶酶切后的单体蛋白均有较好的免疫原性。
運用RT-PCR方法,穫得籽鵝腦垂體催乳素(Prolactin,PRL)基因編碼區序列cDNA,剋隆到pMD18-T載體上。DNA序列分析錶明,PRL cDNA全長690 bp,編碼230箇氨基痠殘基,與皖西白鵝的堿基同源性達99.57%,氨基痠同源性達99.56%。將所得序列與錶達載體pET-32 a(+)構建錶達質粒pET-32 a(+)-PRL。該質粒的DH5α轉化菌經終濃度為1 mmoL.L-1的IPTG在37℃環境下誘導5 h可錶達PRL基因融閤蛋白,錶達量約佔菌體總蛋白的29.63%。用純化的融閤蛋白和凝血酶酶切後的單體蛋白主動免疫小白鼠,經Western blot檢測,所製抗體清晰地檢測到PRL基因錶達蛋白的特異帶,由此證明PRL基因的融閤蛋白和凝血酶酶切後的單體蛋白均有較好的免疫原性。
운용RT-PCR방법,획득자아뇌수체최유소(Prolactin,PRL)기인편마구서렬cDNA,극륭도pMD18-T재체상。DNA서렬분석표명,PRL cDNA전장690 bp,편마230개안기산잔기,여환서백아적감기동원성체99.57%,안기산동원성체99.56%。장소득서렬여표체재체pET-32 a(+)구건표체질립pET-32 a(+)-PRL。해질립적DH5α전화균경종농도위1 mmoL.L-1적IPTG재37℃배경하유도5 h가표체PRL기인융합단백,표체량약점균체총단백적29.63%。용순화적융합단백화응혈매매절후적단체단백주동면역소백서,경Western blot검측,소제항체청석지검측도PRL기인표체단백적특이대,유차증명PRL기인적융합단백화응혈매매절후적단체단백균유교호적면역원성。
The mature segment gene of prolactin(PRL) in Zi Goose was amplified from pituitary by RT-PCR and then cloned into the pMD18-T vector.Sequencing analysis showed that the cDNA has a length of 690 bp and encodes a protein composed of 230 amino acid residues,which differs from the published PRL cDNA sequence.There was a homology of 99.57% in base and 99.56% in amino acid residues with that of Wanxi White Goose,respectively.A prokaryotic expression vector,pET-32 a(+),was used to construct the recombinant plasmid pET-32 a(+)-PRL to produce protein.Having been induced by IPTG,the host cell carrying the recombinant plasmid expressed the recombinant PRL.The optimal condition for expression was 1 mmoL·L-1 IPTG at 37 ℃.Based on this condition,the expression dose rose to the highest level by 5 hours of induction,accounting for 29.63% of the total bacterial protein.Purified fused proteins and digested PRL monomers by thrombin were injected into Kuming mouse to perform active immunity,the results showed that the fused proteins of PRL could be tested clearly by westernblot,and both of fused proteins and monomers have efficient immunogenicity.