中华耳科学杂志
中華耳科學雜誌
중화이과학잡지
CHINESE JOURNAL OF OTOLOGY
2013年
1期
112-117
,共6页
孙毓晗*%侯昭晖*%肖玉丽
孫毓晗*%侯昭暉*%肖玉麗
손육함*%후소휘*%초옥려
Smad4%慢病毒
Smad4%慢病毒
Smad4%만병독
Smad4%Lentivirus
目的构建含有小鼠Smad4基因和增强型绿色荧光蛋白基因(EGFP)的慢病毒病毒表达载体,为今后应用该重组慢病毒介导的内耳基因导入和相关的聋病基因治疗奠定实验基础.方法利用基因重组、限制性内切酶酶切及基因测序的方法,构建并鉴定pLenti6.3-Smad4-IRES2-EGFP真核表达质粒;利用脂质体介导转染的方法,将pLenti6.3-Smad4-IRES2-EGFP转染导入293T细胞,荧光显微镜下观察EGFP基因表达情况,利用实时荧光PCR的方法检测小鼠Smad4基因mRNA水平的表达情况.结果经PCR鉴定和基因测序证实了小鼠Smad4基因序列与基因bank中的序列相一致.pLenti6.3-Smad4-IRES2-EGFP质粒转入293T细胞后,荧光显微镜下可见有绿色荧光蛋白表达.293T细胞经慢病毒感染后,其小鼠Smad4基因mRNA表达量增加了66427倍.病毒滴度经测定为2.5×108TU/ml.结论成功地构建了含有小鼠Smad4基因的慢病毒表达载体,并能在293T细胞中表达.
目的構建含有小鼠Smad4基因和增彊型綠色熒光蛋白基因(EGFP)的慢病毒病毒錶達載體,為今後應用該重組慢病毒介導的內耳基因導入和相關的聾病基因治療奠定實驗基礎.方法利用基因重組、限製性內切酶酶切及基因測序的方法,構建併鑒定pLenti6.3-Smad4-IRES2-EGFP真覈錶達質粒;利用脂質體介導轉染的方法,將pLenti6.3-Smad4-IRES2-EGFP轉染導入293T細胞,熒光顯微鏡下觀察EGFP基因錶達情況,利用實時熒光PCR的方法檢測小鼠Smad4基因mRNA水平的錶達情況.結果經PCR鑒定和基因測序證實瞭小鼠Smad4基因序列與基因bank中的序列相一緻.pLenti6.3-Smad4-IRES2-EGFP質粒轉入293T細胞後,熒光顯微鏡下可見有綠色熒光蛋白錶達.293T細胞經慢病毒感染後,其小鼠Smad4基因mRNA錶達量增加瞭66427倍.病毒滴度經測定為2.5×108TU/ml.結論成功地構建瞭含有小鼠Smad4基因的慢病毒錶達載體,併能在293T細胞中錶達.
목적구건함유소서Smad4기인화증강형록색형광단백기인(EGFP)적만병독병독표체재체,위금후응용해중조만병독개도적내이기인도입화상관적롱병기인치료전정실험기출.방법이용기인중조、한제성내절매매절급기인측서적방법,구건병감정pLenti6.3-Smad4-IRES2-EGFP진핵표체질립;이용지질체개도전염적방법,장pLenti6.3-Smad4-IRES2-EGFP전염도입293T세포,형광현미경하관찰EGFP기인표체정황,이용실시형광PCR적방법검측소서Smad4기인mRNA수평적표체정황.결과경PCR감정화기인측서증실료소서Smad4기인서렬여기인bank중적서렬상일치.pLenti6.3-Smad4-IRES2-EGFP질립전입293T세포후,형광현미경하가견유록색형광단백표체.293T세포경만병독감염후,기소서Smad4기인mRNA표체량증가료66427배.병독적도경측정위2.5×108TU/ml.결론성공지구건료함유소서Smad4기인적만병독표체재체,병능재293T세포중표체.
Objective To construct a lentivirus expression vector containing the mouse smad4 gene and EGFP gene for possible application in recombinant lentivirus-mediated inner ear gene transfer and gene therapy for deafness. Methods The eukaryotic expression plasmid pLenti6.3-Smad4-IRES2-EGFP was constructed and identified by gene recombination, restriction enzyme digestion and gene sequencing methods. The 293T cells were transfected with the pLen?ti6.3-Smad4-IRES2-EGFP plasmid by the lipofectamine-mediated transfection method EGFP gene expression was exam?ined under a fluorescence microscope. Mouse Smad4 mRNA expression was detected by real-time PCR. Results The PCR and sequencing analysis confirmed that the mouse smad4 gene sequence was consistent with the reference in the gene bank. After 293T cells were transfected with the pLenti6.3-Smad4-IRES2-EGFP plasmid, the green fluorescent protein was visi?ble. After 293T cells were infected with lentivirus, Smad4 gene mRNA expression increased by 66,427 times, reaching to a titer of 2.5 ×108TU/ml. Conclusions The recombinant lentivirus expression vector for mouse smad4 gene can be constructed with successful vector expression in 293T cells.
