经济动物学报
經濟動物學報
경제동물학보
JOURNAL OF ECONOMIC ANIMAL
2012年
1期
26-30
,共5页
张志崇%王春生%张秋婷%朴善花%苗向阳%安铁洙
張誌崇%王春生%張鞦婷%樸善花%苗嚮暘%安鐵洙
장지숭%왕춘생%장추정%박선화%묘향양%안철수
中国林蛙%抗菌肽%绵羊成纤维细胞%瞬时表达
中國林蛙%抗菌肽%綿羊成纖維細胞%瞬時錶達
중국림와%항균태%면양성섬유세포%순시표체
Rana chensinensis%antimicrobial peptide%sheep fibroblast cell%transient expression activityanalysis
为了建立大量获取中国林蛙抗菌肽的方法,根据GenBank中的中国林蛙皮肤抗菌肽Temporin-1CEa基因的mRNA序列(EU624139)设计一对特异性引物,以提取的中国林蛙皮肤总RNA反转录出的cDNA为模板,将扩增的编码序列与pEASY-T3克隆载体连接获得Tem-T3;利用酶切、连接等分子生物学手段,将GFP基因连入Tem-T3克隆载体,再经酶切获得Tem-GFP片段,并插入真核表达载体pcDNA3.1,最终得到Tem-GFP-pcD-NA3.1重组质粒;利用脂质体转染法将该质粒转入绵羊成纤维细胞,48 h后可在荧光倒置显微镜下观察到GFP的绿色荧光表达;qPCR数据分析显示,与对照组相比,转染Tem-GFP-pcDNA3.1的绵羊成纤维细胞中融合蛋白Tem-GFP的表达量可提高约300倍。本研究为构建Temporin-1CEa基因山羊乳腺特异表达载体提供依据。
為瞭建立大量穫取中國林蛙抗菌肽的方法,根據GenBank中的中國林蛙皮膚抗菌肽Temporin-1CEa基因的mRNA序列(EU624139)設計一對特異性引物,以提取的中國林蛙皮膚總RNA反轉錄齣的cDNA為模闆,將擴增的編碼序列與pEASY-T3剋隆載體連接穫得Tem-T3;利用酶切、連接等分子生物學手段,將GFP基因連入Tem-T3剋隆載體,再經酶切穫得Tem-GFP片段,併插入真覈錶達載體pcDNA3.1,最終得到Tem-GFP-pcD-NA3.1重組質粒;利用脂質體轉染法將該質粒轉入綿羊成纖維細胞,48 h後可在熒光倒置顯微鏡下觀察到GFP的綠色熒光錶達;qPCR數據分析顯示,與對照組相比,轉染Tem-GFP-pcDNA3.1的綿羊成纖維細胞中融閤蛋白Tem-GFP的錶達量可提高約300倍。本研究為構建Temporin-1CEa基因山羊乳腺特異錶達載體提供依據。
위료건립대량획취중국림와항균태적방법,근거GenBank중적중국림와피부항균태Temporin-1CEa기인적mRNA서렬(EU624139)설계일대특이성인물,이제취적중국림와피부총RNA반전록출적cDNA위모판,장확증적편마서렬여pEASY-T3극륭재체련접획득Tem-T3;이용매절、련접등분자생물학수단,장GFP기인련입Tem-T3극륭재체,재경매절획득Tem-GFP편단,병삽입진핵표체재체pcDNA3.1,최종득도Tem-GFP-pcD-NA3.1중조질립;이용지질체전염법장해질립전입면양성섬유세포,48 h후가재형광도치현미경하관찰도GFP적록색형광표체;qPCR수거분석현시,여대조조상비,전염Tem-GFP-pcDNA3.1적면양성섬유세포중융합단백Tem-GFP적표체량가제고약300배。본연구위구건Temporin-1CEa기인산양유선특이표체재체제공의거。
In order to establish a method to get a large number of antimicrobial peptides from Rana chensinensis,a series of experiments were conducted as follows.According to Chinese frog skin antimicrobial peptides Temporin-1CEa gene mRNA sequence(EU624139) in GenBank,a pair of specific primers were designed and cDNA was obtained from Chinese forest frog skin RNA by reverse transcription.Temporin-1CEa gene coding sequence was amplified using the cDNA,and linked with pEASY-T3 cloning vector.The GFP gene was inserted into the recombinant plasmid Tem-T3 by molecular methods.The Tem-GFP fragment was linked with eukaryotic expression vector pcDNA3.1,and Tem-GFP-pcDNA3.1 recombinant plasmid was achieved finally.Using of lipid infection method,the plasmids were transfected into sheep fibroblast cells,the green fluorescence was observed under a fluorescence microscope after 48 h.qPCR data showed that Tem-GFP fusion protein expression level of transfected Tem-GFP-pcDNA3.1 sheep fibroblasts increased about 300 folds than that of the control group.This study supplied the technical basis for developing mammary gland bioreactor of expressing Temporin-1CEa gene.