Blöcher D
Int J Radiat Biol Relat Stud Phys Chem Med. 1982 Sep;42(3):317-28. doi: 10.1080/09553008214551231.
DNA double strand breaks (dsb) were determined in Ehrlich ascites tumour cells at doses down to 5 Gy. The method is based on the separation of DNA from other components by heating in a solution of pronase and detergents held in wide-mouth syringes, which were also used to facilitate the application of the released high molecular weight DNA to sucrose gradients. Purified DNA was sedimented in neutral sucrose gradients at low speed to reduce speed artifacts. The sedimentation profiles were analysed using a computer program and the number of dsb was determined by simulation of random breaks in the mass distribution of the control sample and by comparison of this simulated profile with that of the irradiated one. The number of dsb formed was proportional to X-ray dose in the range of 5 to 2000 Gy. The induction per dose was found to be nmr-1 D-1 = (11.7 +/- 2) x 10(-12) Gy-1.
在剂量低至5戈瑞的情况下,对艾氏腹水瘤细胞中的DNA双链断裂(dsb)进行了测定。该方法基于通过在装有链霉蛋白酶和去污剂的溶液中加热,将DNA与其他成分分离,加热过程在广口注射器中进行,这些注射器还用于便于将释放的高分子量DNA应用于蔗糖梯度。纯化后的DNA在中性蔗糖梯度中低速沉降,以减少速度假象。使用计算机程序分析沉降图谱,并通过模拟对照样品质量分布中的随机断裂以及将该模拟图谱与辐照样品的图谱进行比较来确定dsb的数量。在5至2000戈瑞的范围内,形成的dsb数量与X射线剂量成正比。发现每剂量的诱导率为nmr-1 D-1 =(11.7±2)×10(-12)Gy-1。
