Abstract
Electroporation is an electro-physical, non-viral approach to perform DNA, RNA, and protein transfections of cells. Upon application of an electric field, the cell membrane is compromised, allowing the delivery of exogenous materials into cells. Cell viability and electro-transfection efficiency (eTE) are dependent on various experimental factors, including pulse waveform, vector concentration, cell type/density, and electroporation buffer properties. In this work, the effects of buffer composition on cell viability and eTE were systematically explored for plasmid DNA encoding green fluorescent protein following electroporation of 3T3 fibroblasts. A HEPES-based buffer was used in conjunction with various salts and sugars to modulate conductivity and osmolality, respectively. Pulse applications were chosen to maintain constant applied electrical energy (J) or total charge flux (C/m2). The energy of the pulse application primarily dictated cell viability, with Mg2+-based buffers expanding the reversible electroporation range. The enhancement of viability with Mg2+-based buffers led to the hypothesis that this enhancement is due to ATPase activation via re-establishing ionic homeostasis. We show preliminary evidence for this mechanism by demonstrating that the enhanced viability is eliminated by introducing lidocaine, an ATPase inhibitor. However, Mg2+ also hinders eTE compared to K+-based buffers. Collectively, the results demonstrate that the rational selection of pulsing conditions and buffer compositions are critical for the design of electroporation protocols to maximize viability and eTE.
Highlights
Electroporation is an electro-physical, non-viral approach to perform DNA, RNA, and protein transfections of cells
Electroporation outcomes are typically defined as the resulting cell viability, defined as the percentage of living cells following electroporation compared to a non-electroporated control, and electro-transfection efficiency, defined as the percentage of cells receiving or expressing the delivered vector
Electroporation buffers generally fall into several categories of composition – saline-based, phosphate-based, HEPES-based, or cell-culture-media based – with conductivity tailored by the salt added and osmolality adjusted with an osmotic agent, often sugar or an inert protein[13,14,15]
Summary
Electroporation is an electro-physical, non-viral approach to perform DNA, RNA, and protein transfections of cells. Electroporation outcomes are typically defined as the resulting cell viability, defined as the percentage of living cells following electroporation compared to a non-electroporated control, and electro-transfection efficiency (eTE), defined as the percentage of cells receiving or expressing the delivered vector These outcomes are dependent on a variety of experimental parameters including: electric pulse strength and duration, number of electric pulses applied, cell type, cell density, pDNA concentration, buffer conductivity, and buffer composition[8,9,10,11,12]. Does such a large number of experimental variables increase the complexity of protocol optimization, it has www.nature.com/scientificreports led to a vast landscape of published work, making it difficult to draw conclusions among them. These early studies motivated us to explore how buffer composition can affect electroporation outcomes
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