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Adenovirus Vector Designed for Expression of Toxic Proteins

机译:用于表达有毒蛋白质的腺病毒载体

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摘要

To construct recombinant adenoviruses expressing biologically active proteins may be impossible, or result in a significant reduction in virus yield, if the protein expressed has an inhibitory effect on virus replication or cellular growth. To overcome this problem, we previously designed adenovirus vectors expressing foreign proteins from inducible promoters. However, during our work with a replication-deficient virus expressing the ASF/SF2 splicing factor from a progesterone antagonist-inducible gene cassette, we discovered that ASF/SF2 was expressed at a significant level in the 293 producer cell line, even in the absence of inducer. 293 cells code for adenovirus E1A and E1B proteins and thus support the growth of E1-deficient adenoviruses. Here we show that this background ASF/SF2 expression results from a low level of E1A-mediated transactivation of the basal promoter driving transgene expression. To overcome the problem of leaky expression, we reconstructed a novel gene cassette that combines an inducible promoter and a Lac repressor protein-based block to reduce transcriptional elongation. We show that this novel vector system dramatically reduced background transgene expression and therefore should be useful for the rescue and propagation of high-titer stocks of recombinant adenoviruses expressing toxic proteins.
机译:如果表达的蛋白质对病毒复制或细胞生长具有抑制作用,则构建表达生物活性蛋白质的重组腺病毒可能是不可能的,或者导致病毒产量的显着降低。为了克服这个问题,我们以前设计了从诱导型启动子表达外源蛋白的腺病毒载体。但是,在我们研究一种从孕激素拮抗剂诱导型基因盒表达ASF / SF2剪接因子的复制缺陷型病毒的过程中,我们发现ASF / SF2在293生产细胞系中也有很高的表达水平,即使没有诱导剂。 293细胞编码腺病毒E1A和E1B蛋白,因此支持E1缺陷型腺病毒的生长。在这里,我们显示此背景ASF / SF2表达是由低水平的E1A介导的基础启动子驱动转基因表达的反式激活引起的。为了克服漏表达的问题,我们重建了一个新颖的基因盒,该盒结合了可诱导的启动子和基于Lac阻遏蛋白的块,以减少转录延伸。我们表明,这种新颖的载体系统大大减少了背景转基因表达,因此应可用于表达毒性蛋白的重组腺病毒的高滴度库存的抢救和繁殖。

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