醫(yī)學(xué)論文范文:編碼大鼠Nogo受體mRNA的shRNA重組腺病毒載體的構(gòu)建和鑒定
【摘要】 目的: 構(gòu)建Nogo受體(NgR)特異性shRNA重組腺病毒載體,為應(yīng)用基因沉默技術(shù)從轉(zhuǎn)錄后水平進行缺血性腦損傷的基因治療研究奠定基礎(chǔ). 方法: 將前期構(gòu)建的大鼠Nogo受體mRNA的shRNA特異性真核表達載體pGenesil1shRNA的表達啟動子U6連同shRNA亞克隆至穿梭質(zhì)粒pAdTrack,酶切及DNA測序鑒定后, 將含NgR基因的重組穿梭質(zhì)粒pAdTrackU6shRNA經(jīng)PmeI線性化后轉(zhuǎn)化入pAdEasy1感受態(tài)細(xì)菌. 將pAdU6shRNA質(zhì)粒經(jīng)PacI線性化后轉(zhuǎn)染293細(xì)胞,包裝重組腺病毒AdenoU6shRNA,并進行PCR鑒定、PCR產(chǎn)物測序及病毒滴度測定. 結(jié)果: 結(jié)果證實pAdTrackU6shRNA及pAdU6shRNA質(zhì)粒構(gòu)建正確,收獲病毒后的PCR及DNA測序結(jié)果證明AdenoU6shRNA包被成功. 結(jié)論: 成功構(gòu)建了大鼠Nogo受體mRNA的shRNA重組腺病毒載體AdenoU6shRNA,將為應(yīng)用基因沉默技術(shù)研究NgR在缺血性腦損傷后神經(jīng)再生中的作用奠定基礎(chǔ).
【關(guān)鍵詞】 Nogo受體;RNA干擾;腺病毒
Construction and identification of recombinant adenovirus expressing the shRNA of rat Nogo66 receptor
ZHANG QinLi1, QIN XinYue1, YIN Cheng1, PENG Yan2
1Department of Neurology, First Affiliated Hospital, 2Department of Histology and Embryology, Chongqing Medical University, Chongqing 400016, China醫(yī).學(xué).全.在.線f1411.cn
【Abstract】 AIM: To construct the recombinant adenovirus vector of shRNA targeted to the rat Nogo66 receptor gene for the therapy of ischemic brain injury in posttranscriptional regulation. METHODS: The used pGenesil1shRNA was construsted and identified in previous experiment. The U6 and shRNA of pGenesil1shRNA were subcloned to pAdTrack. The product pAdTrackU6shRNA was linearized by Pme I to mediate homologous recombination with pAdEasy1 in pAdEasy1 host bacteria. The positive clone was identified by enzyme digestion, PCR analysis and DNA sequence analysis. After linearized by Pac I, the recombinant adenovirus DNA pAdU6shRNA was transfected into 293 cells for packaging and amplification of AdenoU6shRNA. AdenoU6shRNA was further identified by PCR analysis and DNA sequence analysis. RESULTS: PCR analysis, enzyme digestion and DNA sequence analysis proved the pAdTrackU6shRNA and the pAdU6shRNA had been successfully constructed. After being packaged in 293 cells, the recombinant adenovirus AdenoU6shRNA was identified by PCR analysis and DNA sequence analysis. CONCLUSION: We have successfully constructed recombinant adenovirus AdenoU6shRNA targeted against the rat Nogo66 receptor gene. It will be helpful to use RNAi in the research of the role of NgR in neural regeneration after cerebral ischemic injury.
【Keywords】 Nogo66 receptor; RNAi; adenoviruses
0引言
缺血性腦損傷后中樞神經(jīng)的再生是神經(jīng)康復(fù)難以逾越的障礙,近來研究發(fā)現(xiàn),中樞神經(jīng)再生困難的原因是CNS三種軸突再生抑制蛋白的存在,它們是NogoA,MAG和OMgp,與共同的受體NgR結(jié)合,激活下游信號及GTPase Rho系統(tǒng),導(dǎo)致軸突生長錐崩潰[1]. 因此,NgR成為理想的治療靶. RNA干擾(RNAi)是由雙鏈RNA介導(dǎo)的、在轉(zhuǎn)錄后mRNA水平關(guān)閉相應(yīng)基因表達過程-將與靶基因同源的21~23 bp的雙鏈RNA導(dǎo)入細(xì)胞,它在細(xì)胞中可與靶基因mRNA結(jié)合,并迅速將其降解,從而抑制該基因的表達的過程[2].而成功地進行RNAi的關(guān)鍵在于使siRNA導(dǎo)入細(xì)胞,我們利用前期實驗已構(gòu)建的NgR shRNA真核表達載體,進一步構(gòu)建腺病毒表達載體,通過病毒載體導(dǎo)入NgR siRNA沉默NgR基因,從而達到拮抗NgR基因的效應(yīng),促進神經(jīng)再生.