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使用病毒粒子DNA作为构建突变型和重组疱疹病毒的克隆载体。

Use of virion DNA as a cloning vector for the construction of mutant and recombinant herpesviruses.

作者信息

Duboise S M, Guo J, Desrosiers R C, Jung J U

机构信息

Department of Microbiology and Molecular Genetics, New England Regional Primate Research Center, Harvard Medical School, Southborough, MA 01772-9102, USA.

出版信息

Proc Natl Acad Sci U S A. 1996 Oct 15;93(21):11389-94. doi: 10.1073/pnas.93.21.11389.

DOI:10.1073/pnas.93.21.11389
PMID:8876145
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC38067/
Abstract

We have developed improved procedures for the isolation of deletion mutant, point mutant, and recombinant herpesvirus saimiri. These procedures take advantage of the absence of NotI and AscI restriction enzyme sites within the viral genome and use reporter genes for the identification of recombinant viruses. Genes for secreted engineered alkaline phosphatase and green fluorescent protein were placed under simian virus 40 early promoter control and flanked by NotI and AscI restriction sites. When permissive cells were cotransfected with herpesvirus saimiri virion DNA and one of the engineered reporter genes cloned within herpesvirus saimiri sequences, recombinant viruses were readily identified and purified on the basis of expression of the reporter gene. Digestion of recombinant virion DNA with NotI or AscI was used to delete the reporter gene from the recombinant herpesvirus saimiri. Replacement of the reporter gene can be achieved by NotI or AscI digestion of virion DNA and ligation with a terminally matched fragment or, alternatively, by homologous recombination in cotransfected cells. Any gene can, in theory, be cloned directly into the virion DNA when flanked by the appropriate NotI or AscI sites. These procedures should be widely applicable in their general form to most or all herpesviruses that replicate permissively in cultured cells.

摘要

我们已经开发出改进的程序来分离缺失突变体、点突变体和重组猴疱疹病毒。这些程序利用了病毒基因组中不存在NotI和AscI限制性酶切位点这一特性,并使用报告基因来鉴定重组病毒。将分泌型工程碱性磷酸酶和绿色荧光蛋白的基因置于猴病毒40早期启动子的控制之下,并在两侧加上NotI和AscI限制性位点。当允许性细胞与猴疱疹病毒病毒粒子DNA以及克隆在猴疱疹病毒序列中的一个工程报告基因共转染时,基于报告基因的表达很容易鉴定和纯化重组病毒。用NotI或AscI消化重组病毒粒子DNA可从重组猴疱疹病毒中删除报告基因。报告基因的替换可以通过用NotI或AscI消化病毒粒子DNA并与末端匹配的片段连接来实现,或者通过在共转染细胞中的同源重组来实现。理论上,任何基因在两侧加上合适的NotI或AscI位点时都可以直接克隆到病毒粒子DNA中。这些程序的一般形式应广泛适用于在培养细胞中允许性复制的大多数或所有疱疹病毒。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/da03/38067/d6d3ca3f9d24/pnas01525-0118-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/da03/38067/d6d3ca3f9d24/pnas01525-0118-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/da03/38067/d6d3ca3f9d24/pnas01525-0118-a.jpg

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Herpesvirus saimiri.赛米利疱疹病毒
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Viral vectors for gene transfer: a review of their use in the treatment of human diseases.用于基因转移的病毒载体:其在人类疾病治疗中的应用综述

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