癌变·畸变·突变
癌變·畸變·突變
암변·기변·돌변
CARCINOGENSES,TERATOGENSIS AND MUTAGENESIS
2014年
3期
204-208,212
,共6页
谢杏%柯跃斌%刘庆成%刘建军%毛侃琅%徐新云%夏菠%杨淋清
謝杏%柯躍斌%劉慶成%劉建軍%毛侃瑯%徐新雲%夏菠%楊淋清
사행%가약빈%류경성%류건군%모간랑%서신운%하파%양림청
hsa-miR-148a-3p%DNA甲基转移酶1%16HBE细胞%慢病毒
hsa-miR-148a-3p%DNA甲基轉移酶1%16HBE細胞%慢病毒
hsa-miR-148a-3p%DNA갑기전이매1%16HBE세포%만병독
hsa-miR-148a-3p%DNMT1%16HBE cells%lentivirus
目的:建立稳定的hsa-miR-148a-3p低表达人支气管上皮细胞株(16HBE)。方法:根据miRBase中提供的序列信息设计hsa-miR-148a-3p tough decoy RNA(TuD RNA),并将其连接到慢病毒载体pLKO.1-puro上。将重组慢病毒载体转染至293FT细胞并包装为慢病毒后,收集病毒上清,感染正常16HBE细胞。用嘌呤霉素筛选出has-miR-148a-3p低表达的16HBE细胞株,通过荧光定量PCR对其进行鉴定,然后对筛选出的细胞分别采用荧光定量PCR和Western blot检测DNA甲基转移酶1(DNMT1) mRNA和蛋白的表达水平。结果:测序结果表明含hsa-miR-148a-3p TuD RNA的重组慢病毒载体构建成功;荧光定量PCR检测显示has-miR-148a-3p低表达的16HBE细胞株has-miR-148a-3p的表达量比正常16HBE细胞低44%(P<0.01),其作用靶基因DNMT1的mRNA和蛋白表达水平分别为正常细胞的3.4倍和2.0倍(P均<0.01)。结论:成功建立hsa-miR-148a-3p低表达的16HBE细胞,hsa-miR-148a-3p的低表达能提高DNMT1 mRNA和蛋白的表达水平。
目的:建立穩定的hsa-miR-148a-3p低錶達人支氣管上皮細胞株(16HBE)。方法:根據miRBase中提供的序列信息設計hsa-miR-148a-3p tough decoy RNA(TuD RNA),併將其連接到慢病毒載體pLKO.1-puro上。將重組慢病毒載體轉染至293FT細胞併包裝為慢病毒後,收集病毒上清,感染正常16HBE細胞。用嘌呤黴素篩選齣has-miR-148a-3p低錶達的16HBE細胞株,通過熒光定量PCR對其進行鑒定,然後對篩選齣的細胞分彆採用熒光定量PCR和Western blot檢測DNA甲基轉移酶1(DNMT1) mRNA和蛋白的錶達水平。結果:測序結果錶明含hsa-miR-148a-3p TuD RNA的重組慢病毒載體構建成功;熒光定量PCR檢測顯示has-miR-148a-3p低錶達的16HBE細胞株has-miR-148a-3p的錶達量比正常16HBE細胞低44%(P<0.01),其作用靶基因DNMT1的mRNA和蛋白錶達水平分彆為正常細胞的3.4倍和2.0倍(P均<0.01)。結論:成功建立hsa-miR-148a-3p低錶達的16HBE細胞,hsa-miR-148a-3p的低錶達能提高DNMT1 mRNA和蛋白的錶達水平。
목적:건립은정적hsa-miR-148a-3p저표체인지기관상피세포주(16HBE)。방법:근거miRBase중제공적서렬신식설계hsa-miR-148a-3p tough decoy RNA(TuD RNA),병장기련접도만병독재체pLKO.1-puro상。장중조만병독재체전염지293FT세포병포장위만병독후,수집병독상청,감염정상16HBE세포。용표령매소사선출has-miR-148a-3p저표체적16HBE세포주,통과형광정량PCR대기진행감정,연후대사선출적세포분별채용형광정량PCR화Western blot검측DNA갑기전이매1(DNMT1) mRNA화단백적표체수평。결과:측서결과표명함hsa-miR-148a-3p TuD RNA적중조만병독재체구건성공;형광정량PCR검측현시has-miR-148a-3p저표체적16HBE세포주has-miR-148a-3p적표체량비정상16HBE세포저44%(P<0.01),기작용파기인DNMT1적mRNA화단백표체수평분별위정상세포적3.4배화2.0배(P균<0.01)。결론:성공건립hsa-miR-148a-3p저표체적16HBE세포,hsa-miR-148a-3p적저표체능제고DNMT1 mRNA화단백적표체수평。
OBJECTIVE: To construct a 16HBE cell line with low expression of hsa-miR-148a-3p. METHODS:A pair of TuD RNA sequences of hsa-miR-148a-3p was designed according to information provided in miRBase, which was ligated to lentiviral vector pLKO.1-puro afterwards. The recombinant vector was transfected into 293FT cells for lentivirus packaging. The viruses were collected and used to infect normal 16HBE cells. The target cells were selected with Puromycin and was identified by quantitative PCR. The mRNA expression and the protein expression level of DNMT1 were then tested. RESULTS:Sequencing results indicated the successful construction of recombinant lentiviral vector with hsa-miR-148a-3p TuD RNA,quantitative PCR showed that the expression level of hsa-miR-148a-3p in the target cells was 44%lower than that of normal 16HBE cells(P<0.01),whereas a 3.4-fold increase of the mRNA expression level and a two-fold increase of protein expression level of DNMT1 were observed in the cell line(P<0.01). CONCLUSION:Low expression of hsa-miR-148a-3p of 16HBE cell line was successfully constructed,and inhibition of hsa-miR-148a-3p could lead to higher expression and higher protein levels of DNMT1.
