Literature DB >> 10757018

Accurate estimation of transduction efficiency necessitates a multiplex real-time PCR.

D Klein1, B Bugl, W H Günzburg, B Salmons.   

Abstract

Transduction efficiency can be easily monitored during pre-clinical trials by inclusion of marker genes. However, the use of such marker genes should be avoided in the final clinical gene therapy application since their products are often immunogenic, making it difficult to monitor transduction, especially if the vector is applied in vivo. In these cases PCR-based methods like the real-time PCR might provide a powerful tool to estimate biodistribution. To investigate the accuracy of this method, we have developed and tested a real-time PCR assay for the quantification of the enhanced green fluorescent protein (EGFP) gene and compared the results with transduction efficiencies estimated by FACS analysis. Although our real-time PCR assay itself was characterized by a high precision over a wide dynamic range of quantification, significant differences in the transduction efficiency compared with FACS data were initially observed. Accurate determination could only be achieved using an optimized multiplex real-time PCR assay, which allows the simultaneous calculation of cell number and EGFP copy number in the same tube. In view of future needs for methods allowing precise and accurate analysis of biodistribution in gene therapy trials, our data highlight the necessity critically to check both parameters in the implemented assay.

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Year:  2000        PMID: 10757018     DOI: 10.1038/sj.gt.3301112

Source DB:  PubMed          Journal:  Gene Ther        ISSN: 0969-7128            Impact factor:   5.250


  19 in total

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3.  Multiple modifications allow high-titer production of retroviral vectors carrying heterologous regulatory elements.

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Journal:  J Virol       Date:  2004-02       Impact factor: 5.103

4.  Flexibility of the adenovirus fiber is required for efficient receptor interaction.

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5.  Correct capsid assembly mediated by a conserved YXXLGL motif in prototype foamy virus Gag is essential for infectivity and reverse transcription of the viral genome.

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Authors:  Lindsay A Pfeffer; Becky K Brisson; Hanqin Lei; Elisabeth R Barton
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8.  MHC mismatch results in neural progenitor cell rejection following spinal cord transplantation in a model of viral-induced demyelination.

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9.  Effects of viral strain, transgene position, and target cell type on replication kinetics, genomic stability, and transgene expression of replication-competent murine leukemia virus-based vectors.

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10.  Influence of vector design and host cell on the mechanism of recombination and emergence of mutant subpopulations of replicating retroviral vectors.

Authors:  Matthias Paar; Dieter Klein; Brian Salmons; Walter H Günzburg; Matthias Renner; Daniel Portsmouth
Journal:  BMC Mol Biol       Date:  2009-02-09       Impact factor: 2.946

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