1998
DOI: 10.1038/sj.gt.3300700
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High efficiency gene transfer to the central nervous system of rodents and primates using herpes virus vectors lacking functional ICP27 and ICP34.5

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Cited by 50 publications
(41 citation statements)
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“…[7][8][9] Common marmosets are bred in designated Primate Research Facilities within the United States and as such these animals are readily available at most biomedical research centers, thus facilitating experimental planning and potentially accelerating transitions into important clinical trials.…”
Section: Introductionmentioning
confidence: 99%
“…[7][8][9] Common marmosets are bred in designated Primate Research Facilities within the United States and as such these animals are readily available at most biomedical research centers, thus facilitating experimental planning and potentially accelerating transitions into important clinical trials.…”
Section: Introductionmentioning
confidence: 99%
“…The newly synthesised viral particles are released from the infected cells by lysis. Since many of the HSV proteins are nonessential for viral replication, they can be removed and replaced with the target therapeutic genes [68,105].…”
Section: Non-integrating Viral Vectorsmentioning
confidence: 99%
“…Each virus was plaque purified following homologous recombination of the respective plasmids into ICP27-deleted virus DNA. 11 The photomicrographs in Figure 2 clearly demonstrate that in B130/2 cells infected with the 17+pR19 IRES virus (Figure 2a and b) where the deletion of ICP27 is complemented, both reporter genes are expressed to a high level. However, it is also clear that the expression of both the transgene upstream and downstream of the EMCV IRES is decreased in comparison to B130/2 cells infected with the single transgene-expressing 17+pR19 lacZ and 17+pR19 GFP viruses (Figure 2c and d).…”
Section: Figure 2 Reporter Gene Expression In B130/2 Cells Infected Wmentioning
confidence: 99%
“…10,11 Therefore, the vectors used for this study were also deleted for ICP27. Transgene expression was driven by the human cytomegalovirus immediate-early (CMV IE) promoter and the promoter/transgene cassette was inserted by homologous recombination into the 2 kb LAT sequence in the HSV-1 genome (strain 17+).…”
Section: Figure 1 Schematic Representation Of the 17+pr19-based Hsv-1mentioning
confidence: 99%