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Optoporation and genetic manipulation of cells using femtosecond laser pulses

机译:飞秒激光脉冲对细胞的对抗和遗传操作

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Femtosecond laser optoporation is a powerful technique to introduce membrane-impermeable molecules, such as DNA plasmids, into targeted cells in culture, yet only a narrow range of laser regimes have been explored. In addition, the dynamics of the laser-produced membrane pores and the effect of pore behavior on cell viability and transfection efficiency remain poorly elucidated. We studied optoporation in cultured cells using tightly focused femtosecond laser pulses in two irradiation regimes: millions of low-energy pulses and two higher-energy pulses. We quantified the pore radius and resealing time as a function of incident laser energy and determined cell viability and transfection efficiency for both irradiation regimes. These data showed that pore size was the governing factor in cell viability, independently of the laser irradiation regime. For viable cells, larger pores resealed more quickly than smaller pores, ruling out a passive resealing mechanism. Based on the pore size and resealing time, we predict that few DNA plasmids enter the cell via diffusion, suggesting an alternative mechanism for cell transfection. Indeed, we observed fluorescently labeled DNA plasmid adhering to the irradiated patch of the cell membrane, suggesting that plasmids may enter the cell by adhering to the membrane and then being translocated.
机译:飞秒激光对位技术是一种将不可渗透膜的分子(例如DNA质粒)引入培养的目标细胞的强大技术,但仅研究了狭窄的激光范围。另外,仍未充分阐明激光产生的膜孔的动力学以及孔行为对细胞活力和转染效率的影响。我们使用紧密聚焦的飞秒激光脉冲在两种照射方式下研究了培养细胞的对映作用:数百万个低能脉冲和两个高能脉冲。我们量化孔径半径和重新密封时间作为入射激光能量的函数,并确定两种照射方案的细胞活力和转染效率。这些数据表明,孔径是细胞活力的决定因素,与激光照射方式无关。对于活细胞,较大的孔比较小的孔重新密封的速度更快,从而排除了被动重新密封的机制。根据孔径和重新密封的时间,我们预测几乎没有DNA质粒通过扩散进入细胞,这提示了细胞转染的另一种机制。确实,我们观察到荧光标记的DNA质粒粘附在细胞膜的辐射斑片上,这表明质粒可以通过粘附在细胞膜上然后进入细胞而进入细胞。

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