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自切割核酶介导的人横纹肌肉瘤细胞中β淀粉样前体蛋白(βAPP)的减少

Self-cleaving-ribozyme-mediated reduction of betaAPP in human rhabdomyosarcoma cells.

作者信息

Dolzhanskaya N, Conti J, Schwenk V, Merz G, Denman R B

机构信息

Department of Molecular Biology, New York State Institute for Basic Research in Developmental Disabilities, Staten Island 10314, USA.

出版信息

Arch Biochem Biophys. 2001 Mar 15;387(2):223-32. doi: 10.1006/abbi.2000.2262.

DOI:10.1006/abbi.2000.2262
PMID:11370845
Abstract

A self-cleaving hammerhead ribozyme targeted to codon 47 in beta-amyloid precursor protein (betaAPP) mRNA was cloned as a eucaryotic transcription cassette into the 3' UTR of enhanced green fluorescence protein (EGFP) mRNA, producing a C-terminal fusion mRNA. CMV promotor-driven vectors bearing this construct or a mutationally inactive ribozyme construct were transiently transfected into human embryonic rhabdomyosarcoma (A-204) cells and their effects studied. Ribozyme self-cleavage in vivo was demonstrated by Northern blotting and the site of self-cleavage was delineated using site-specific deoxyoligonucleotide probes and primer extension arrest. Using this ribozyme reporter we demonstrated that ribozyme expression correlated with lower betaAPP levels in the transfected cells. Control studies with the inactive ribozyme construct showed that both ribozyme cleavage and antisense mechanisms combined to produce the observed effect. Furthermore, production of truncated EGFP mRNA via ribozyme self-cleavage reduced EGFP-reporter expression compared to full-length EGFP control mRNAs, indicating that truncation affects the translatability of the reporter. This occurred because of a slight decrease in the stability of the fusion mRNA. The results of these studies suggest that self-cleaving ribozyme vectors may be an effective means of delivering and visualizing the expression of small active ribozymes in vivo.

摘要

将一个靶向β-淀粉样前体蛋白(βAPP)mRNA密码子47的自切割锤头状核酶作为真核转录盒克隆到增强型绿色荧光蛋白(EGFP)mRNA的3'非翻译区,产生一个C末端融合mRNA。将携带该构建体或突变失活核酶构建体的巨细胞病毒启动子驱动载体瞬时转染到人胚胎横纹肌肉瘤(A - 204)细胞中,并研究其作用。通过Northern印迹法证明了核酶在体内的自切割,并使用位点特异性脱氧寡核苷酸探针和引物延伸终止法确定了自切割位点。使用这种核酶报告基因,我们证明了核酶表达与转染细胞中较低的βAPP水平相关。对失活核酶构建体的对照研究表明,核酶切割和反义机制共同作用产生了观察到的效果。此外,与全长EGFP对照mRNA相比,通过核酶自切割产生的截短EGFP mRNA降低了EGFP报告基因的表达,表明截短影响了报告基因的可翻译性。这是由于融合mRNA的稳定性略有下降所致。这些研究结果表明,自切割核酶载体可能是在体内递送和可视化小活性核酶表达的有效手段。

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