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Fowl pox virus double-gene expression carrier (PG7.5N)

An expression vector and fowl pox virus technology, applied in gene therapy, genetic engineering, plant gene improvement, etc., can solve the problems of cumbersome operation, few restriction sites, and reduced expression of the second gene, etc., to increase the number , Improve expression efficiency, reduce the effect of vector length

Inactive Publication Date: 2008-07-16
SOUTH CHINA AGRI UNIV
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0003] At present, the existing fowlpox virus vectors are not perfect, such as the vector is too large, the length of the foreign gene that can be carried is limited, there are not many available restriction sites, and the operation is cumbersome
Moreover, most of the double-gene expression vectors are expressed in cis, which has a certain reduction in the expression of the second gene.

Method used

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  • Fowl pox virus double-gene expression carrier (PG7.5N)
  • Fowl pox virus double-gene expression carrier (PG7.5N)

Examples

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Embodiment 1

[0031] This embodiment will take the expression vector shown in SEQ ID NO.1 as an example to describe its construction method and application in detail.

[0032] 1. Materials

[0033] Live fowlpox vaccine (I) was purchased from Qianyuanhao Nanjing Biopharmaceutical Factory. pGEM4z was purchased from Huamei Bioengineering Co., Ltd. 6-well cell culture plate, DMEM, Opti-MEM and Lipofatamine2000 were purchased from Invitrogen. X-gal, low melting point agarose, T4 polynucleotide kinase, PrimeSTAR TM HS DNA polymerase and DNA LigationKit (Mighty Mix) were purchased from Takara. Gel Extraction Kit and Plasmid miniKit (200) were purchased from Omega. JM109 competent cells were purchased from Takara. The primers used were the same as in the specification.

[0034] 2. Construction method

[0035] 2.1 Shuttle plasmid construction method

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Abstract

The invention provides a fowlpox virus double-gene expression vector, which has a nucleotide sequence that is shown by SEQ ID NO.1. The invention includes a promoter P7.5, an LacZ gene, multiple cloning sites which are located on the LacZ gene, a rare restriction enzyme cutting site Not1, homologous arms F11L1 and F11L2 of the fowlpox virus, an Amp <R> resistance marker gene and an origin of replication (ori). The double-gene expression vector constructed by the invention can reduce the length of the vector to the maximum extent, thus a larger exogenous gene can be contained; the number of available restriction enzyme cutting sites is increased so as to facilitate the cloning of different exogenous genes; the promoter at an insertion site Not1 is not limited and the promoter which is matched with the exogenous gene can be freely chosen so as to improve expression efficiency; furthermore, the invention adopts a reverse expression method so as to improve the expression efficiency of the exogenous gene.

Description

technical field [0001] The invention belongs to the field of biotechnology, and in particular relates to a fowlpox virus double-gene expression vector, its construction method and application. Background technique [0002] Poxviridae is a large group of obligate viruses with a diameter of 300-400nm and a lipid-protein shell surrounding a complex core structure. This structure contains a linear nearly 20kb double-stranded DNA molecule, encoding multiple subunits, and DNA-dependent The RNA polymerase, transcription factor, cap structure and methylase, poly A polymerase, are all packaged in the viral core and translated into mRNAs. Fowlpox Virus (FPV) belongs to the genus Fowlpoxvirus of the family Poxviridae. The virion core contains double-strand linear DNA, G+C=35%, and the genome is about 300kb long. Under natural conditions, it can only infect poultry, but it can produce abortive infection on mammalian cells, does not produce infectious virus particles, but can express a...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12N15/863A61K48/00A61K31/7088
Inventor 廖明江经伟孔令辰郁宏伟任涛
Owner SOUTH CHINA AGRI UNIV
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