Safe and efficient novel approach for non-invasive gene electrotransfer to skin

被引:0
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作者
Lise Pasquet
Sophie Chabot
Elisabeth Bellard
Bostjan Markelc
Marie-Pierre Rols
Jean-Paul Reynes
Gérard Tiraby
Franck Couillaud
Justin Teissie
Muriel Golzio
机构
[1] Université de Toulouse,Institut de Pharmacologie et de Biologie Structurale
[2] CNRS,undefined
[3] UPS,undefined
[4] BP 64182,undefined
[5] 205 Route de Narbonne,undefined
[6] Invivogen Cayla SAS,undefined
[7] 5 rue Jean Rodier,undefined
[8] Zone industrielle de Montaudran,undefined
[9] Laboratoire d’Imagerie Moléculaire et Thérapies innovantes en Oncologie (IMOTION) EA 7435,undefined
[10] Université de Bordeaux,undefined
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关键词
Gene Electrotransfer (GET); Protein tdTomato; Electrode Contact; tdTomato Expression; Treated Skin Surface;
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学科分类号
摘要
Gene transfer into cells or tissue by application of electric pulses (i.e. gene electrotransfer (GET)) is a non-viral gene delivery method that is becoming increasingly attractive for clinical applications. In order to make GET progress to wide clinical usage its efficacy needs to be improved and the safety of the method has to be confirmed. Therefore, the aim of our study was to increase GET efficacy in skin, by optimizing electric pulse parameters and the design of electrodes. We evaluated the safety of our novel approach by assaying the thermal stress effect of GET conditions and the biodistribution of a cytokine expressing plasmid. Transfection efficacy of different pulse parameters was determined using two reporter genes encoding for the green fluorescent protein (GFP) and the tdTomato fluorescent protein, respectively. GET was performed using non-invasive contact electrodes immediately after intradermal injection of plasmid DNA into mouse skin. Fluorescence imaging of transfected skin showed that a sophistication in the pulse parameters could be selected to get greater transfection efficacy in comparison to the standard ones. Delivery of electric pulses only mildly induced expression of the heat shock protein Hsp70 in a luminescent reporting transgenic mouse model, demonstrating that there were no drastic stress effects. The plasmid was not detected in other organs and was found only at the site of treatment for a limited period of time. In conclusion, we set up a novel approach for GET combining new electric field parameters with high voltage short pulses and medium voltage long pulses using contact electrodes, to obtain a high expression of both fluorescent reporter and therapeutic genes while showing full safety in living animals.
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