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An in vivo selection method to optimize trans-splicing ribozymes

机译:优化转拼核酶的体内选择方法

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摘要

Group I intron ribozymes can repair mutated mRNAs by replacing the 3′-terminal portion of the mRNA with their own 3′-exon. This trans-splicing reaction has the potential to treat genetic disorders and to selectively kill cancer cells or virus-infected cells. However, these ribozymes have not yet been used in therapy, partially due to a low in vivo trans-splicing efficiency. Previous strategies to improve the trans-splicing efficiencies focused on designing and testing individual ribozyme constructs. Here we describe a method that selects the most efficient ribozymes from millions of ribozyme variants. This method uses an in vivo rescue assay where the mRNA of an inactivated antibiotic resistance gene is repaired by trans-splicing group I intron ribozymes. Bacterial cells that express efficient trans-splicing ribozymes are able to grow on medium containing the antibiotic chloramphenicol. We randomized a 5′-terminal sequence of the Tetrahymena thermophila group I intron and screened a library with 9 × 106 ribozyme variants for the best trans-splicing activity. The resulting ribozymes showed increased trans-splicing efficiency and help the design of efficient trans-splicing ribozymes for different sequence contexts. This in vivo selection method can now be used to optimize any sequence in trans-splicing ribozymes.
机译:第一组内含子核酶可以通过用自身的3'外显子替换mRNA的3'末端部分来修复突变的mRNA。这种转拼反应具有治疗遗传疾病和选择性杀死癌细胞或病毒感染细胞的潜力。但是,这些核酶尚未用于治疗中,部分原因是体内转拼效率低。以前提高反拼效率的策略集中在设计和测试单个核酶构建体上。在这里,我们描述了一种从数百万个核酶变体中选择最有效的核酶的方法。该方法使用体内拯救试验,其中灭活的抗生素抗性基因的mRNA由反式剪接的I组内含子核酶修复。表达有效转拼核酶的细菌细胞能够在含有抗生素氯霉素的培养基上生长。我们随机化了嗜热四膜膜虫第1组内含子的5'-末端序列,并筛选了具有9×10 6 核酶变体的文库,以实现最佳的转拼活性。所得到的核酶显示出增加的反剪接效率,并有助于针对不同序列背景设计有效的反剪接核酶。现在可以使用这种体内选择方法来优化反式拼接核酶中的任何序列。

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