浙江临床医学
浙江臨床醫學
절강림상의학
ZHEJIANG CLINICAL MEDICAL JOURNAL
2014年
12期
1866-1868
,共3页
细菌%同源重组%重组腺病毒质粒
細菌%同源重組%重組腺病毒質粒
세균%동원중조%중조선병독질립
homlogous recombination%Recombinant adenovirus plasmid%TCF21
目的:利用大肠杆菌BJ5183细菌内同源重组法构建重组腺病毒pAd-TCF21载体。方法设计TCF21cDNA 扩增引物,从真核表达载体pCMV-SPORT6.1-TCF21中扩增TCF21的DNA序列,与腺病毒穿梭质粒pAdTrack-CMV进行连接,构成穿梭质粒pAdTrack-TCF21;然后再用经PmeI酶线性化的pAdTrack-TCF21转化含pAdeasy-1的超感受态AdBJ5183,采用细菌内同源重组法构建腺病毒质粒pAd-TCF21;筛选同源重组质粒阳性克隆,提取pAd-TCF21质粒经PacI酶切鉴定和PCR鉴定。结果线性化的pAdTrack-TCF21转化含pAdeasy-1的超感受态AdBJ5183,12~20h后获得了40%阳性重组质粒克隆,经酶切获得>23kb的大片段和3.0 kb的特征性片段,PCR反应扩增出了540bp的片段,证明重组腺病毒质粒中已成功插入目的基因TCF21。结论细菌内同源重组法成功构建了含TCF21基因的重组腺病毒质粒,为下一步腺病毒介导的TCF21转染A549细胞的研究打下基础。
目的:利用大腸桿菌BJ5183細菌內同源重組法構建重組腺病毒pAd-TCF21載體。方法設計TCF21cDNA 擴增引物,從真覈錶達載體pCMV-SPORT6.1-TCF21中擴增TCF21的DNA序列,與腺病毒穿梭質粒pAdTrack-CMV進行連接,構成穿梭質粒pAdTrack-TCF21;然後再用經PmeI酶線性化的pAdTrack-TCF21轉化含pAdeasy-1的超感受態AdBJ5183,採用細菌內同源重組法構建腺病毒質粒pAd-TCF21;篩選同源重組質粒暘性剋隆,提取pAd-TCF21質粒經PacI酶切鑒定和PCR鑒定。結果線性化的pAdTrack-TCF21轉化含pAdeasy-1的超感受態AdBJ5183,12~20h後穫得瞭40%暘性重組質粒剋隆,經酶切穫得>23kb的大片段和3.0 kb的特徵性片段,PCR反應擴增齣瞭540bp的片段,證明重組腺病毒質粒中已成功插入目的基因TCF21。結論細菌內同源重組法成功構建瞭含TCF21基因的重組腺病毒質粒,為下一步腺病毒介導的TCF21轉染A549細胞的研究打下基礎。
목적:이용대장간균BJ5183세균내동원중조법구건중조선병독pAd-TCF21재체。방법설계TCF21cDNA 확증인물,종진핵표체재체pCMV-SPORT6.1-TCF21중확증TCF21적DNA서렬,여선병독천사질립pAdTrack-CMV진행련접,구성천사질립pAdTrack-TCF21;연후재용경PmeI매선성화적pAdTrack-TCF21전화함pAdeasy-1적초감수태AdBJ5183,채용세균내동원중조법구건선병독질립pAd-TCF21;사선동원중조질립양성극륭,제취pAd-TCF21질립경PacI매절감정화PCR감정。결과선성화적pAdTrack-TCF21전화함pAdeasy-1적초감수태AdBJ5183,12~20h후획득료40%양성중조질립극륭,경매절획득>23kb적대편단화3.0 kb적특정성편단,PCR반응확증출료540bp적편단,증명중조선병독질립중이성공삽입목적기인TCF21。결론세균내동원중조법성공구건료함TCF21기인적중조선병독질립,위하일보선병독개도적TCF21전염A549세포적연구타하기출。
ObjectiveTo construct recombinant adenovirus plasmids by using a method of homologous recombination in bacteria with TCF21 as target gene .Method The TCF21cDNA primers were designed,the DNA sequence of TCF21 was amplified from eukaryotic vector pCMV-SPORT6.1-TCF21 and ligated into the adenovirus shuttle plasmid pAdTrack-CMV,the shuttle plasmid named pAdTrack-TCF21 was constructed. Then the pAdTrack-TCF21 was linealized with PmeI and transformed into ultracompletent BJ5183 containing pAdeasy-l,then recombinant advenovirus plasmid pAd-TCF21 was constructed by homologous recombination in bacteria.Positive clone of homologous recombination was selected,pAd-TCF21 was extracted and identified by PacI digestion and PCR.ResultsThe linealized pAdTrack-TCF21 was transformed into ultracompletent BJ5183 containing pAdeasy-1.There were over 40% positive recombinant plasmid.There were two bands:3kb and larger than 23 kb when pAd-TCF21 was digested with PacI.A 540bp TCF21 cDNA fragment was amplified by PCR.The target gene tcf21 was successfully cloned into adenovirus genomie DNA plasmid by digesting with PacI and the PCR technique .ConclusionThe recombinant adenoviral plasmid containing TCF21 was successfully constructed with homologous recombination in bacteria.This study provides a basis for the next research of the transfection of A549 cells by adenovirus-mediated TCF21.
