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Design of a ribozyme targeting human telomerase reverse transcriptase and cloning of it’s gene

机译:靶向人类端粒酶逆转录酶的核酶的设计及其基因的克隆

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摘要

AIM: To design a hammerhead ribozyme targeting human telomerase reverse transcriptase (hTERT) and clone it’s gene for future use in the study of tumor gene therapy.METHODS: Using the software RNAstructure, the secondary structure of hTERT mRNA was predicted and the cleavage site of ribozyme was selected. A hammerhead ribozyme targeting this site was designed and bimolecular fold between the ribozyme and hTERT was predicted. The DNA encoding the ribozyme was synthesized and cloned into pGEMEX-1 and the sequence of the ribozyme gene was confirmed by DNA sequencing.RESULTS: Triplet GUC at 1742 of hTERT mRNA was chosen as the cleavage site of the ribozyme. The designed ribozyme was comprised of 22 nt catalytic core and 17 nt flanking sequence. Computer-aided prediction suggested that the ribozyme and hTERT mRNA could cofold into a proper conformation. Endonuclease restriction and DNA sequencing confirmed the correct insertion of the ribozyme gene into the vector pGEMEX-1.CONCLUSION: This fundamental work of successful designing and cloning of an anti-hTERT hammerhead ribozyme has paved the way for further study of inhibiting tumor cell growth by cleaving hTERT mRNA with ribozyme.
机译:目的:设计针对人端粒酶逆转录酶(hTERT)的锤头状核酶,克隆其基因,以供将来在肿瘤基因治疗研究中使用。方法:利用RNA结构软件,预测hTERT mRNA的二级结构并确定其切割位点。选择了核酶。设计了靶向该位点的锤头状核酶,并预测了核酶和hTERT之间的双分子折叠。合成了编码核酶的DNA并将其克隆到pGEMEX-1中,并通过DNA测序证实了核酶基因的序列。结果:选择hTERT mRNA 1742的三重态GUC作为核酶的切割位点。设计的核酶由22nt的催化核心和17nt的侧翼序列组成。计算机辅助预测表明,核酶和hTERT mRNA可以共折叠成适当的构象。核酸内切酶的限制和DNA测序证实核酶基因正确插入到载体pGEMEX-1中。结论:这项成功设计和克隆抗hTERT锤头状核酶的基础工作为进一步研究抑制肿瘤细胞生长铺平了道路。用核酶裂解hTERT mRNA。

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