4.7 Article

Mechanisms of in vivo DNA electrotransfer:: Respective contributions of cell electropermeabilization and DNA electrophoresis

Journal

MOLECULAR THERAPY
Volume 5, Issue 2, Pages 133-140

Publisher

CELL PRESS
DOI: 10.1006/mthe.2002.0526

Keywords

gene therapy; electrogenetherapy; DNA electrotransfer; electropermeabilization; electroporation; electric pulses; nonviral gene therapy; muscle; naked DNA; plasmid DNA

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Efficient cell electrotransfection can be achieved using combinations of high-voltage (HV; 800 V/cm, 100 mus) and low-voltage (LV; 80 V/cm, 100 ms) pulses. We have developed equipment allowing the generation of various HV and LV combinations with precise control of the lag between the HV and LV pulses. We injected luciferase-encoding DNA in skeletal muscle, before or after pulse delivery, and measured luciferase expression after various pulse combinations. In parallel, we determined permeabilization levels using uptake of Cr-51-labeled EDTA. High voltage alone resulted in a high level of muscle permeabilization for 300 seconds, but very low DNA transfer. Combinations of one HV pulse followed by one or four LV pulses did not prolong the high permeabilization level, but resulted in a large increase in DNA transfer for lags up to 100 seconds in the case of one HV + one LV and up to 3000 seconds in the case of one HV + four LV. DNA expression also reached similar levels when we injected the DNA between the HV and LV pulses. We conclude that the role of the HV pulse is limited to muscle cell permeabilization and that the LV pulses have a direct effect on DNA. In vivo DNA electrotransfer is thus a multistep process that includes DNA distribution, muscle permeabilization, and DNA electrophoresis.

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