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显著提高从 cDNA 质粒中拯救狂犬病病毒的效率。

Significantly improved rescue of rabies virus from cDNA plasmids.

机构信息

Max von Pettenkofer-Institute & Gene Center, Ludwig-Maximilians-University Munich, Feodor-Lynen-Strasse 25, Munich, Germany.

出版信息

Eur J Cell Biol. 2012 Jan;91(1):10-6. doi: 10.1016/j.ejcb.2011.01.008. Epub 2011 Mar 12.

DOI:10.1016/j.ejcb.2011.01.008
PMID:21397981
Abstract

The rescue of recombinant rabies virus (RV) from cloned cDNA is an inefficient process because it relies on the de novo formation within cells of functional ribonucleoprotein (RNP) complexes from plasmid-expressed viral-like antigenome RNAs and three helper proteins. In the standard RV reverse genetics systems, bacteriophage T7 RNA polymerase drives the transcription of virus antigenome-like RNAs containing three nonviral G residues at the 5'-end and a correct 3'-end generated by the autocatalytic activity of an 85 nucleotides long hepatitis delta virus antigenomic "core" ribozyme (HDVagrz). Here, we show that employing optimized ribozyme sequences significantly improves RV rescue. Substitution of the "core" HDVagrz by a ribozyme with an enhanced cleavage activity resulted in an approximately 10-fold higher number of rescue events and faster initiation of an infectious cycle. The alternative use of a hammerhead ribozyme for the generation of an exact 5'-end similarly enhanced rescue efficiency. Notably, RV cDNA clones containing the combination of optimized 3'- and 5'-ribozymes were rescued at an at least 100-fold increase. In addition to virus rescue, reporter gene expression from transfected minigenome cDNAs was significantly enhanced by the novel ribozymes. The improved RV reverse genetics system greatly facilitates recovery of strongly attenuated viruses and vectors for biomedical applications.

摘要

从克隆 cDNA 中拯救重组狂犬病病毒 (RV) 是一个效率低下的过程,因为它依赖于细胞内从头形成功能性核糖核蛋白 (RNP) 复合物,这些复合物由质粒表达的病毒样抗原基因组 RNA 和三种辅助蛋白组成。在标准的 RV 反向遗传学系统中,噬菌体 T7 RNA 聚合酶驱动病毒抗原基因组样 RNA 的转录,这些 RNA 在 5' 端含有三个非病毒 G 残基,并且通过长度为 85 个核苷酸的自身催化活性的乙型肝炎 delta 病毒抗原基因组“核心”核酶 (HDVagrz) 生成正确的 3' 端。在这里,我们表明,采用优化的核酶序列可显著提高 RV 的拯救效率。用具有增强切割活性的核酶替代“核心”HDVagrz 可导致拯救事件的数量增加约 10 倍,并且感染周期的起始更快。替代使用锤头核酶来产生精确的 5' 端也同样提高了拯救效率。值得注意的是,含有优化的 3' 和 5' 核酶组合的 RV cDNA 克隆的拯救效率至少提高了 100 倍。除了病毒拯救之外,新型核酶还显著增强了转染的小基因文库 cDNA 中的报告基因表达。改进的 RV 反向遗传学系统极大地促进了用于生物医学应用的强减毒病毒和载体的恢复。

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