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Immunogenicity and safety of defective vaccinia virus lister: comparison with modified vaccinia virus Ankara.缺陷型痘苗病毒李斯特株的免疫原性和安全性:与改良痘苗病毒安卡拉株的比较。
J Virol. 2002 Aug;76(15):7713-23. doi: 10.1128/jvi.76.15.7713-7723.2002.
2
Retroviral vectors produced in the cytoplasmic vaccinia virus system transduce intron-containing genes.在细胞质痘苗病毒系统中产生的逆转录病毒载体可转导含内含子的基因。
J Virol. 2002 Feb;76(3):1236-43. doi: 10.1128/jvi.76.3.1236-1243.2002.
3
Lentiviral vectors: excellent tools for experimental gene transfer and promising candidates for gene therapy.慢病毒载体:用于实验性基因转移的优秀工具及基因治疗的有前景候选者。
J Gene Med. 2000 Sep-Oct;2(5):308-16. doi: 10.1002/1521-2254(200009/10)2:5<308::AID-JGM131>3.0.CO;2-3.
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Stable gene transfer to the nervous system using a non-primate lentiviral vector.使用非灵长类慢病毒载体将基因稳定转移至神经系统。
Gene Ther. 1999 Nov;6(11):1808-18. doi: 10.1038/sj.gt.3301023.
5
Poxviral/retroviral chimeric vectors allow cytoplasmic production of transducing defective retroviral particles.痘病毒/逆转录病毒嵌合载体可在细胞质中产生具有转导能力的缺陷型逆转录病毒颗粒。
Virology. 1999 Jan 5;253(1):107-14. doi: 10.1006/viro.1998.9496.
6
Transient marker stabilisation: a general procedure to construct marker-free recombinant vaccinia virus.瞬时标记稳定化:构建无标记重组痘苗病毒的通用方法。
Arch Virol. 1998;143(3):467-74. doi: 10.1007/s007050050303.
7
Packaging of intron-containing genes into retrovirus vectors by alphavirus vectors.通过甲病毒载体将含内含子的基因包装到逆转录病毒载体中。
Proc Natl Acad Sci U S A. 1998 Mar 31;95(7):3650-4. doi: 10.1073/pnas.95.7.3650.
8
Apoptosis induced by a postbinding step of vaccinia virus entry into Chinese hamster ovary cells.痘苗病毒进入中国仓鼠卵巢细胞的结合后步骤所诱导的细胞凋亡。
Virology. 1998 Mar 1;242(1):138-49. doi: 10.1006/viro.1997.8985.
9
Rapid identification of viable retrovirus-transduced cells using the green fluorescent protein as a marker.以绿色荧光蛋白为标记物快速鉴定有活力的逆转录病毒转导细胞。
Gene Ther. 1997 Nov;4(11):1256-60. doi: 10.1038/sj.gt.3300519.
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Compact, synthetic, vaccinia virus early/late promoter for protein expression.用于蛋白质表达的紧凑型合成痘苗病毒早期/晚期启动子。
Biotechniques. 1997 Dec;23(6):1094-7. doi: 10.2144/97236st07.

通过用单一杂交痘苗病毒感染产生具有转导能力的逆转录病毒载体。

Generation of transduction-competent retroviral vectors by infection with a single hybrid vaccinia virus.

作者信息

Konetschny Christian, Holzer Georg W, Urban Carsten, Hämmerle Thomas, Mayrhofer Josef, Falkner Falko G

机构信息

Baxter Vaccine AG, Biomedical Research Center, A-2304 Orth/Donau, Austria.

出版信息

J Virol. 2003 Jun;77(12):7017-25. doi: 10.1128/jvi.77.12.7017-7025.2003.

DOI:10.1128/jvi.77.12.7017-7025.2003
PMID:12768020
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC156191/
Abstract

Recombinant vaccinia viruses that express defective retroviral vectors upon a single infection event in normal host cells were constructed. The gag-pol and envelope genes and a retroviral vector unit were inserted as vaccinia virus promoter-controlled transcription units at three separate loci. The triple recombinant virus was used to infect such diverse cell types as monkey and rabbit kidney, human lung, and primary chicken cells, resulting in the production of transduction-competent defective retroviral vectors. Infection of Chinese hamster ovary cells, which are nonpermissive for vaccinia virus replication, also resulted in production of retroviral vectors and secondary permanent transduction of the host cells. Since vaccinia virus supports the expression of cytotoxic proteins, the vesicular stomatitis virus G glycoprotein could be chosen as the envelope allowing a broad host range of transduction. Functionality of particles was monitored by expression of the green fluorescent protein in transduced 3T3 cell clones. This is the first description of a single chimeric virus encoding and releasing functional retroviral vectors, providing proof of principle of the new concept. No replication-competent retrovirus was detectable by sensitive reverse transcriptase assays. Since vaccinia virus has a broad host range, is extremely robust, and can be obtained at high titers and safe nonreplicating vaccinia virus strains are available, the hybrid system may open new perspectives for gene delivery.

摘要

构建了在正常宿主细胞单次感染事件后表达缺陷型逆转录病毒载体的重组痘苗病毒。将gag-pol和包膜基因以及逆转录病毒载体单元作为痘苗病毒启动子控制的转录单元插入到三个不同的位点。该三重重组病毒用于感染多种细胞类型,如猴肾和兔肾细胞、人肺细胞和原代鸡细胞,从而产生具有转导能力的缺陷型逆转录病毒载体。感染对痘苗病毒复制不敏感的中国仓鼠卵巢细胞,也会产生逆转录病毒载体并对宿主细胞进行二次永久转导。由于痘苗病毒支持细胞毒性蛋白的表达,因此可以选择水泡性口炎病毒G糖蛋白作为包膜,从而实现广泛的宿主转导范围。通过在转导的3T3细胞克隆中表达绿色荧光蛋白来监测颗粒的功能。这是对一种编码并释放功能性逆转录病毒载体的单一嵌合病毒的首次描述,为这一新概念提供了原理证明。通过灵敏的逆转录酶检测未检测到有复制能力 的逆转录病毒。由于痘苗病毒具有广泛的宿主范围,极其稳定,并且可以获得高滴度,而且有安全的非复制型痘苗病毒株可用,因此该杂交系统可能为基因递送开辟新的前景。