Group I aptazymes as genetic regulatory switches

被引：78

作者：

Thompson K.M. ^{[2
]}

Syrett H.A. ^{[1
]}

Knudsen S.M. ^{[1
]}

Ellington A.D. ^{[1
]}

机构：

[1] Department of Chemistry/Biochemistry, Inst. for Cellular/Molecular Biology, University of Texas at Austin, Austin

[2] Archemix Corp., Cambridge, MA 02139

来源：

BMC Biotechnology | / 2卷 / 1期

关键词：

Theophylline; Hammerhead Ribozyme; Splice Reaction; Splice Activity; Ribozyme Activity;

D O I：

10.1186/1472-6750-2-21

中图分类号：

学科分类号：

摘要：

Background: Allosteric ribozymes (aptazymes) that have extraordinary activation parameters have been generated in vitro by design and selection. For example, hammerhead and ligase ribozymes that are activated by small organic effectors and protein effectors have been selected from random sequence pools appended to extant ribozymes. Many ribozymes, especially self-splicing introns, are known control gene regulation or viral replication in vivo. We attempted to generate Group I self-splicing introns that were activated by a small organic effector, theophylline, and to show that such Group I aptazymes could mediate theophylline-dependent splicing in vivo. Results: By appending aptamers to the Group I self-splicing intron, we have generated a Group I aptazyme whose in vivo splicing is controlled by exogenously added small molecules. Substantial differences in gene regulation could be observed with compounds that differed by as little as a single methyl group. The effector-specificity of the Group I aptazyme could be rationally engineered for new effector molecules. Conclusion: Group I aptazymes may find applications as genetic regulatory switches for generating conditional knockouts at the level of mRNA or for developing economically viable gene therapies. © 2002 Thompson et al; licensee BioMed Central Ltd.

引用

页数：12

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