首页> 美国卫生研究院文献>Nucleic Acids Research >Enhancement of ribozyme catalytic activity by a contiguous oligodeoxynucleotide (facilitator) and by 2-O-methylation.
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Enhancement of ribozyme catalytic activity by a contiguous oligodeoxynucleotide (facilitator) and by 2-O-methylation.

机译:连续的寡脱氧核苷酸(促进剂)和2-O-甲基化可增强核酶的催化活性。

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摘要

RNA catalysts (ribozymes) designed to cleave sequences unique to viral RNA's might be developed as therapeutics. For this purpose, they would require high catalytic efficiency and resistance to nucleases. Reported here are two approaches that can be used in combination to improve these properties. First, catalytic efficiency can be improved by oligonucleotides (facilitators) that bind to the substrate contiguously with the 3'-end of the ribozyme. Second, 2'-O-methylation of flanking sequences of the ribozyme increases catalytic activity as well as resistance to nucleases. In combination with a facilitator oligodeoxynucleotide, the cleavage rate was increased 20 fold over that of the unmodified ribozyme.
机译:设计用于切割病毒RNA特有序列的RNA催化剂(核酶)可能被开发为治疗剂。为此,它们将需要高的催化效率和对核酸酶的抗性。这里报告了两种可以组合使用以改善这些特性的方法。首先,可以通过寡核苷酸(促进剂)提高催化效率,该寡核苷酸与核酶的3'末端连续结合在底物上。第二,核酶侧翼序列的2'-O-甲基化增加了催化活性以及对核酸酶的抗性。与促进剂寡聚脱氧核苷酸组合,切割速率比未修饰的核酶提高了20倍。

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