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一种用于构建在早期区域1和3中有插入或缺失的腺病毒载体的高效且灵活的系统。

An efficient and flexible system for construction of adenovirus vectors with insertions or deletions in early regions 1 and 3.

作者信息

Bett A J, Haddara W, Prevec L, Graham F L

机构信息

Department of Biology, McMaster University, Hamilton, ON, Canada.

出版信息

Proc Natl Acad Sci U S A. 1994 Sep 13;91(19):8802-6. doi: 10.1073/pnas.91.19.8802.

Abstract

Human adenoviruses (Ads) are attracting considerable attention because of their potential utility for gene transfer and gene therapy, for development of live viral vectored vaccines, and for protein expression in mammalian cells. Engineering Ad vectors for these applications requires a variety of reagents in the form of Ads and bacterial plasmids containing viral DNA sequences and requires different strategies for construction of vectors for different purposes. To simplify Ad vector construction and develop a procedure with maximum flexibility, efficiency, and cloning capacity, we have developed a vector system based on use of Ad5 DNA sequences cloned in bacterial plasmids. Expanded deletions in early region 1 (3180 bp) and early region 3 (2690 or 3132 bp) can be combined in a single vector that should have a capacity for inserts of up to 8.3 kb, enough to accommodate the majority of cDNAs encoding proteins with regulatory elements. Genes can be inserted into either early region 1 or 3 or both and mutations or deletions can be readily introduced elsewhere in the viral genome. To illustrate the flexibility of the system, we have introduced a wild-type early region 3 into the vectors, and to illustrate the high capacity for inserts, we have isolated a vector with two genes totaling 7.8 kb.

摘要

人腺病毒(Ads)因其在基因转移和基因治疗、活病毒载体疫苗开发以及哺乳动物细胞中蛋白质表达方面的潜在用途而备受关注。为这些应用设计腺病毒载体需要多种试剂,包括腺病毒形式的试剂以及含有病毒DNA序列的细菌质粒,并且针对不同目的构建载体需要不同的策略。为了简化腺病毒载体构建并开发一种具有最大灵活性、效率和克隆能力的方法,我们开发了一种基于使用克隆在细菌质粒中的Ad5 DNA序列的载体系统。早期区域1(3180 bp)和早期区域3(2690或3132 bp)中的扩展缺失可以组合在一个单一载体中,该载体应该具有容纳高达8.3 kb插入片段的能力,足以容纳大多数带有调控元件的编码蛋白质的cDNA。基因可以插入早期区域1或3或两者,并且突变或缺失可以很容易地引入病毒基因组的其他位置。为了说明该系统的灵活性,我们已将野生型早期区域3引入载体中,并且为了说明其高插入片段容纳能力,我们已分离出一个含有两个总计7.8 kb基因的载体。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/be6a/44694/841a66e46a93/pnas01141-0084-a.jpg

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