首页> 外文期刊>Molecular therapy: the journal of the American Society of Gene Therapy >Development of a transposon-based approach for identifying novel transgene insertion sites within the replicating adenovirus.
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Development of a transposon-based approach for identifying novel transgene insertion sites within the replicating adenovirus.

机译:基于转座子的方法的开发,用于鉴定复制腺病毒内的新型转基因插入位点。

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摘要

Therapeutic gene delivery from an oncolytic adenovirus (Ad) is one approach to enhancing the potency of Ad-based virotherapies for cancer. To identify therapeutic transgene insertion sites compatible with the replicating virus, a methodology that broadly scans the viral genome is needed. To address this we modified a transposon (Tn7)-based in vitro transposition system to take advantage of its nonprejudiced scanning ability to identify insertion sites compatible with viral replication. Using this system with a plasmid containing an E3-deleted Ad5, we identified several unique sites for promoter-based expression cassette insertions within the Ad genome. The transposon-based expression cassette is bounded by PmeI restriction endonuclease sites unique to the transposon, making expression cassette substitutions easy to perform. Additional expression cassettes containing different promoters and reporter genes were substituted into two of the newly identified transgene insertion sites. The results suggest that the ease and orientation of expression cassette substitution depend on both the insertion site location and the promoter and gene of the replacement expression cassette. These studies establish the transposon-based system as an efficient approach to scanning the Ad genome and identifying insertion sites compatible with viral replication and represents a powerful tool for the development of armed therapeutic viruses for cancer.
机译:从溶瘤腺病毒(Ad)的治疗性基因传递是一种增强基于Ad的病毒疗法对癌症的效力的方法。为了鉴定与复制病毒相容的治疗性转基因插入位点,需要一种广泛扫描病毒基因组的方法。为了解决这个问题,我们修改了基于转座子(Tn7)的体外转座系统,以利用其不受偏见的扫描能力来识别与病毒复制兼容的插入位点。使用该系统与含有E3缺失的Ad5的质粒,我们确定了Ad基因组内基于启动子的表达盒插入的几个独特位点。基于转座子的表达盒由转座子特有的PmeI限制性核酸内切酶位点限制,使表达盒替换更容易进行。将含有不同启动子和报道基因的其他表达盒替换为两个新近鉴定的转基因插入位点。结果表明表达盒替换的容易性和方向取决于插入位点位置以及替换表达盒的启动子和基因。这些研究建立了基于转座子的系统,作为扫描Ad基因组和识别与病毒复制兼容的插入位点的有效方法,并且代表了开发用于癌症的武装治疗性病毒的强大工具。

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