Transfection by Polyethyleneimine-Coated Magnetic Nanoparticles: Fine-Tuning the Condition for Electrophysiological Experiments

被引:8
|
作者
Svoboda, Ondrej [1 ,2 ]
Fohlerova, Zdenka [2 ,3 ,4 ]
Baiazitova, Larisa [1 ]
Mlynek, Petr [5 ]
Samouylov, Konstantin [6 ]
Provaznik, Ivo [1 ]
Hubalek, Jaromir [2 ,3 ,4 ]
机构
[1] Brno Univ Technol, Fac Elect Engn & Commun, Dept Biomed Engn, Tech 12, Brno 61600, Czech Republic
[2] Brno Univ Technol, Cent European Inst Technol, Purkynova 123, Brno 61200, Czech Republic
[3] Brno Univ Technol, Fac Elect Engn & Commun, Dept Microelect, Tech 10, Brno 61600, Czech Republic
[4] Brno Univ Technol, Fac Elect Engn & Commun, Dept Microelect, Ctr 6,Tech 3058 10, Brno 61600, Czech Republic
[5] Brno Univ Technol, Fac Elect Engn & Commun, Dept Telecommun, Tech 10, Brno 61600, Czech Republic
[6] RUDN Univ, Peoples Friendship Univ Russia, 6 Miklukho Maklaya St, Moscow 117198, Russia
关键词
Polyethylenelmine; Magnetic Nanoparticles; Transfection; Patch Clamp; Cytotoxicity; ASAP1; CELL;
D O I
10.1166/jbn.2018.2602
中图分类号
TB3 [工程材料学];
学科分类号
0805 ; 080502 ;
摘要
A non-viral tool for the delivery of nucleic acids termed magnetofection was recently developed as a promising transgenic technique with high transfection efficiency for gene delivery into mammalian cells. Despite the fact that transfection efficiency was the objective in the past, the post-transfection cell morphology and the essential gigaseal formation between cells and patch clamp glass electrodes have not been studied in detail. The cell viability and fluorescent response of Accelerated Sensor of Action Potentials (ASAP1) were studied in somatic HEK293 cells with respect to preserving physiological cell behavior and morphology. The DNA vector (pcDNA3.1/Puro-CAG-ASAP1) was intracellularly delivered by DNA/polyethyleneimine/magnetic nanoparticles and the transfection protocols varied in complex formations were optimized with respect to transfection rate, cytotoxicity of modified nanoparticles and essential gigaseal formation needed for patch clamp technique. A patch clamp study of transfected cells was carried out 72 hours post-transfection. Our results showed the best complex formation in order DNA/magnetic nanoparticle/polyethyleneimine that provides 51.82% transfection efficiency, 83.45% of patch clamp applicable cells, and 90.15% of gigasealed patch clamp applicable cells. A significant difference in fluorescent response of transfected cells was not found compared to control. Thus, these observations suggested that a large amount of the cells were able to create a gigaseal with a glass electrode 72 hours from transfection despite the lower transfection efficiencies.
引用
收藏
页码:1505 / 1514
页数:10
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