The selectable marker neo gene down-regulates gene expression from retroviral vectors containing an internal ribosome entry site

Byun, Ji Won; Jm, Kim; Robbins, P. D.; S, Kim

doi:10.1038/sj.gt.3300762

Cited by 14 publications

(7 citation statements)

References 10 publications

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“…31,32 On the other hand, sequences other than those present in the LTR can influence viral transcription. 33 Indeed, the pBH vectors contain sequence elements, such as the hygromycin resistance gene and a prokaryotic origin of DNA replication, 12 that may contribute to the negative reciprocal interactions that results in poor or absent gp91-gene expression.…”

Section: Discussionmentioning

confidence: 99%

Variegation of retroviral vector gene expression in myeloid cells

et al. 2000

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We have comparatively evaluated the efficiency of a series of retroviral vectors transducing the gp91-phox gene, whose defects are responsible for impaired production of superoxide anion (O 2 − ) by phagocytic cells and lead to the X-linked form of chronic granulomatous disease (X-CGD). These vectors included four constructs based on the MoMuLV backbone and expressing gp91-phox from the viral long terminal repeat (LTR) or from internal promoters, and one construct based on the myelotropic FMEV vector. Expression of the therapeutic gene from the MoMuLV LTR was unsatisfactory after transduction of the PLB985 X-CGD knockout cell line and of primary CD34+ hematopoietic progenitors from X-CGD patients. The presence of either constitutive or inducible internal promoters did not result in important improvements in the efficiency of O 2 − production and lowered the titers of the viral preparations. In contrast, sustained levels of superoxide generation were obtained upon transduction with the FMEV vector. To analyze the efficiency of trans-

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Section: Discussionmentioning

confidence: 99%

Variegation of retroviral vector gene expression in myeloid cells

et al. 2000

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“…Numerous other mechanisms that could play a contributory role to our observed loss of gene expression have also been reported. For example, expression of the neomycin resistance gene has been linked to problems with gene expression 41–43. Although we cannot directly exclude any of these mechanisms as contributory, our results suggest either (1) a problem directly associated with the SRα promoter's ability to maintain gene expression in vivo on murine T cells or (2) a problem indirectly related to the SRα promoter gene position in the specific retroviral construct used in these studies.…”

Section: Discussionmentioning

confidence: 79%

Loss of T cell-mediated antitumor immunity after construct-specific downregulation of retrovirally encoded T-cell receptor expression in vivo

et al. 2008

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Adoptive T-cell therapy is clinically efficacious in the treatment of select cancers. However, it is often difficult to obtain adequate numbers of tumor-specific T cells for therapy. One method for overcoming this limitation is to generate tumor-specific T cells by retrovirally mediated T-cell-receptor (TCR) gene transfer. However, despite instances of therapeutic success, major obstacles remain, including attaining the survival of retrovirally modified T cells in vivo as well as inducing long-term and multi-gene retroviral expression. Using a murine model of adoptively transferred retrovirally modified CD8 þ T cells, where antitumor immunity was dependent on sustained, multigene expression, we found that in vitro assays are poor indicators of in vivo efficacy. Despite persisting for over 9 months in a nonlymphopenic environment, genetically modified T cells exhibited discordant retrovirally mediated gene expression in vivo not readily evident from initial in vitro assays. In particular, one of the two TCR subunit genes necessary for antigen specificity was selectively lost in vivo. As this discordant gene expression was associated with the loss of antitumor immunity, consideration of these findings may provide guidance in the design, evaluation and application of retroviral vectors for use in the treatment of cancer and other human disease.

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“…Again, MT‐IDS gave the highest level of IDS activity, on average 2‐ and 4‐fold higher levels than MIN‐IDS and two other vectors, respectively (Figure 3B). These results suggested that even the same LTR could give varying results when placed under different genomic environments, consistent with our previously published data 24.…”

Section: Resultsmentioning

confidence: 90%

Construction of a high efficiency retroviral vector for gene therapy of Hunter's syndrome

Hong

Kim

et al. 2002

The Journal of Gene Medicine

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Minimum-sized retroviral vector that contains no selective marker as well as a viral coding sequences could drive a high level of gene expression, be produced efficiently from the producer line, and enter hematopoietic cells at a high frequency. Our data suggest the great potential for using MT-based vector(s) in a gene therapy trial for Hunter's syndrome utilizing human CD34+ stem cells as target cells.

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The selectable marker neo gene down-regulates gene expression from retroviral vectors containing an internal ribosome entry site

Cited by 14 publications

References 10 publications

Variegation of retroviral vector gene expression in myeloid cells

Variegation of retroviral vector gene expression in myeloid cells

Loss of T cell-mediated antitumor immunity after construct-specific downregulation of retrovirally encoded T-cell receptor expression in vivo

Construction of a high efficiency retroviral vector for gene therapy of Hunter's syndrome

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