Department of Cell Biology, Faculty of Biochemistry, Biophysics and Biotechnology, Jagiellonian University, Gronostajowa 7, 30-387, Cracow, Poland.
Cell Mol Biol Lett. 2013 Mar;18(1):102-19. doi: 10.2478/s11658-012-0042-3. Epub 2012 Dec 27.
Experiments on reversible and irreversible cell electroporation were carried out with an experimental setup based on a standard apparatus for horizontal electrophoresis, a syringe pump with regulated cell suspension flow velocity and a dcEF power supply. Cells in suspension flowing through an orifice in a barrier inserted into the electrophoresis apparatus were exposed to defined localized dcEFs in the range of 0-1000 V/cm for a selected duration in the range 10-1000 ms. This method permitted the determination of the viability of irreversibly electroperforated cells. It also showed that the uptake by reversibly electroperforated cells of fluorescent dyes (calcein, carboxyfluorescein, Alexa Fluor 488 Phalloidin), which otherwise do not penetrate cell membranes, was dependent upon the dcEF strength and duration in any given single electrical field exposure. The method yields reproducible results, makes it easy to load large volumes of cell suspensions with membrane non-penetrating substances, and permits the elimination of irreversibly electroporated cells of diameter greater than desired. The results concur with and elaborate on those in earlier reports on cell electroporation in commercially available electroporators. They proved once more that the observed cell perforation does not depend upon the thermal effects of the electric current upon cells. In addition, the method eliminates many of the limitations of commercial electroporators and disposable electroporation chambers. It permits the optimization of conditions in which reversible and irreversible electroporation are separated. Over 90% of reversibly electroporated cells remain viable after one short (less than 400 ms) exposure to the localized dcEF. Experiments were conducted with the AT-2 cancer prostate cell line, human skin fibroblasts and human red blood cells, but they could be run with suspensions of any cell type. It is postulated that the described method could be useful for many purposes in biotechnology and biomedicine and could help optimize conditions for in vivo use of both reversible and irreversible electroporation.
进行了可逆和不可逆细胞电穿孔的实验,实验装置基于标准的水平电泳仪、带有调节细胞悬浮流速的注射器泵和直流电场电源。悬浮在通过插入电泳仪的障碍物中的孔中的细胞在选定的持续时间(10-1000ms 范围内)内,暴露于 0-1000V/cm 范围内的限定局部直流电场中。该方法允许确定不可逆电穿孔细胞的活力。它还表明,可逆电穿孔细胞对荧光染料(钙黄绿素、羧基荧光素、Alexa Fluor 488 鬼笔环肽)的摄取取决于在任何给定的单次电场暴露中直流电场强度和持续时间。该方法产生可重复的结果,易于用膜不可穿透的物质加载大量细胞悬浮液,并允许消除直径大于所需的不可逆电穿孔细胞。该结果与商业可用电穿孔仪中的细胞电穿孔的早期报告中的结果一致并加以详细说明。它们再次证明观察到的细胞穿孔不取决于电流对细胞的热效应。此外,该方法消除了商业电穿孔仪和一次性电穿孔室的许多限制。它允许优化可逆和不可逆电穿孔分离的条件。在短时间(小于 400ms)暴露于局部直流电场后,超过 90%的可逆电穿孔细胞保持活力。使用 AT-2 前列腺癌细胞系、人皮肤成纤维细胞和人红细胞进行了实验,但也可以对任何细胞类型的悬浮液进行实验。据推测,所描述的方法可能对生物技术和生物医学的许多目的有用,并有助于优化体内使用可逆和不可逆电穿孔的条件。