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Nonreplicating vaccinia vector efficiently expresses recombinant genes.

机译:非复制型痘苗病毒载体有效表达重组基因。

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摘要

Modified vaccinia Ankara (MVA), a highly attenuated vaccinia virus strain that has been safety tested in humans, was evaluated for use as an expression vector. MVA has multiple genomic deletions and is severely host cell restricted: it grows well in avian cells but is unable to multiply in human and most other mammalian cells tested. Nevertheless, we found that replication of viral DNA appeared normal and that both early and late viral proteins were synthesized in human cells. Proteolytic processing of viral structural proteins was inhibited, however, and only immature virus particles were detected by electron microscopy. We constructed an insertion plasmid with the Escherichia coli lacZ gene under the control of the vaccinia virus late promoter P11, flanked by sequences of MVA DNA, to allow homologous recombination at the site of a naturally occurring 3500-base-pair deletion within the MVA genome. MVA recombinants were isolated and propagated in permissive avian cells and shown to express the enzyme beta-galactosidase upon infection of nonpermissive human cells. The amount of enzyme made was similar to that produced by a recombinant of vaccinia virus strain Western Reserve, which also had the lacZ gene under control of the P11 promoter, but multiplied to high titers. Since recombinant gene expression is unimpaired in nonpermissive human cells, MVA may serve as a highly efficient and exceptionally safe vector.
机译:修饰的牛痘安卡拉(MVA)是一种高度减毒的牛痘病毒株,已在人类中进行安全性测试,被评估用作表达载体。 MVA具有多个基因组缺失,并且受到宿主细胞的严格限制:它在禽类细胞中生长良好,但在人类和大多数其他哺乳动物细胞中无法繁殖。尽管如此,我们发现病毒DNA的复制似乎是正常的,早期和晚期病毒蛋白都是在人细胞中合成的。病毒结构蛋白的蛋白水解过程受到抑制,但是,通过电子显微镜只能检测到未成熟的病毒颗粒。我们在牛痘病毒后期启动子P11的控制下构建了带有大肠杆菌lacZ基因的插入质粒,其两侧为MVA DNA序列,以允许在MVA基因组内自然发生的3500个碱基对缺失的位点进行同源重组。分离出MVA重组体并在允许的禽类细胞中繁殖,并显示出在感染非允许的人类细胞后表达β-半乳糖苷酶。产生的酶的量类似于牛痘病毒株Western Reserve的重组酶产生的酶,该株也具有lacZ基因在P11启动子的控制下,但滴度高。由于重组基因在非人类细胞中的表达不受损害,因此MVA可以用作高效且异常安全的载体。

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  • 作者

    Sutter, G; Moss, B;

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  • 年度 1992
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  • 正文语种 en
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