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Study of mechanisms of electric field-induced DNA transfection. II. Transfection by low-amplitude low-frequency alternating electric fields.

机译:电场诱导的DNA转染机制的研究。二。通过低振幅低频交变电场进行转染。

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摘要

Electroporation for DNA transfection generally uses short intense electric pulses (direct current of kilovolts per centimeter, microseconds to milliseconds), or intense dc shifted radio-frequency oscillating fields. These methods, while remarkably effective, often cause death of certain cell populations. Previously it was shown that a completely reversible, high ionic permeation state of membranes could be induced by a low-frequency alternating electric field (ac) with a strength one-tenth, or less, of the critical breakdown voltage of the cell membrane (Teissie, J., and T. Y. Tsong. 1981. J. Physiol. (Paris). 77:1043-1053). We report the transfection of E. coli (JM105) by plasmid PUC18 DNA, which carries an ampicillin-resistance gene, using low-amplitude, low-frequency ac fields. E. coli transformants confer the ampicillin resistance and the efficiency of the transfection can be conveniently assayed by counting colonies in a selection medium containing ampicillin. For the range of ac fields employed (peak-to-peak amplitude 50-200 V/cm, frequency 0.1 Hz-1 MHz, duration 1-100 s), 100% of the E. coli survived the electric field treatment. Transfection efficiencies varied with field strength and frequency, and as high as 1 x 10(5)/micrograms DNA was obtained with a 200 V/cm square wave, 1 Hz ac field, 30 s exposure time, when the DNA/cell ratio was 50-75. Control samples gave a background transfection of much less than 10/micrograms DNA. With a square wave ac field, the transfection efficiency showed a frequency window: the optimal frequency was 1 Hz with a 200 V/cm field, and was approximately 0.1 Hz with a 50 V/cm field. Transfection efficiency varied with the waveform: square wave > sine wave > triangle wave. If the DNA was added after the ac field was turned off, transfection efficiency was reduced to the background level within 1 min. The field intensity used in this study was low and insufficient to cause electric breakdown of cell membranes. Thus, DNA transfection was not caused by electroporation of the cell membranes. Other possible mechanisms will be considered.
机译:用于DNA转染的电穿孔通常使用短而强烈的电脉冲(千伏每厘米的直流电,微秒至毫秒)或强烈的dc偏移射频振荡场。这些方法虽然非常有效,但通常会导致某些细胞群体死亡。以前的研究表明,强度为细胞膜临界击穿电压的十分之一或更低的低频交流电场(ac)可以诱导膜的完全可逆的高离子渗透状态。 ,J。和TY Tsong。1981. J. Physiol。(Paris)。77:1043-1053)。我们报告了质粒PUC18 DNA的大肠杆菌(JM105)转染,该质粒带有氨苄青霉素抗性基因,使用低振幅,低频交流场。大肠杆菌转化子赋予氨苄青霉素抗性,可以通过在含有氨苄青霉素的选择培养基中计数菌落来方便地测定转染效率。对于所使用的交流电场范围(峰到峰幅度50-200 V / cm,频率0.1 Hz-1 MHz,持续时间1-100 s),100%的大肠杆菌在电场处理中幸免。转染效率随场强和频率的变化而变化,当DNA /细胞比为200时,在200 V / cm方波,1 Hz交流场,30 s暴露时间下可获得高达1 x 10(5)/微克的DNA。 50-75。对照样品的背景转染远远少于10 /微克DNA。在方波交流电场下,转染效率显示出一个频率窗口:在200 V / cm电场下最佳频率为1 Hz,在50 V / cm电场下最佳频率为0.1 Hz。转染效率随波形变化:方波>正弦波>三角波。如果在关闭交流电场后添加了DNA,则转染效率会在1分钟内降至背景水平。在这项研究中使用的场强很低,不足以引起细胞膜的电击穿。因此,DNA转染不是由细胞膜的电穿孔引起的。将考虑其他可能的机制。

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