Overcoming the Specific Toxicity of Large Plasmids Electrotransfer in Primary Cells In Vitro

Overview

Journal Mol Ther Nucleic Acids

Publisher Cell Press

Date 2016 Apr 26

PMID 27111417

Citations 49

Authors

Lea L Lesueur

Lluis M Mir

Franck M Andre

Affiliations

Soon will be listed here.

Abstract

Gene electrotransfer is a safe and efficient nonviral technique for the transfer of nucleic acids of all sizes. Using a small reporter plasmid (3.5 kbp), electrotransfer of more than 90% of the cells, with ~70% viability, can be routinely achieved even in primary cells like mesenchymal stem cells. However, under the same experimental conditions, electrotransfer of larger plasmids (from 6 to 16 kbp) results in very low viability and transfection efficacy. Here, we show that these strong decreases are directly linked to the physical size of the plasmid molecule. Moreover, large plasmids are toxic only when the cells are exposed to electrotransfer pulses. This specific toxicity of large plasmids during electrotransfer is not due to transgene expression and occurs within less than 45 minutes. Indeed, postpulses recovery times of up to 45 minutes are able to entirely abolish the specific toxicity of large plasmid electrotransfer, resulting in a survival and transfection efficacy identical to that of small plasmids. Finally, electrotransfer of small and large plasmids can reach 90-99% of transfection with 60-90% survival considering the findings here reported.

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