Boye E, Köhnlein W, Skarstad K
Nucleic Acids Res. 1984 Nov 12;12(21):8281-91. doi: 10.1093/nar/12.21.8281.
DNA strand breaks induced by Neocarzinostatin in Escherichia coli cells have been characterized. Radioactively labeled phage lambda DNA was introduced into lysogenic host bacteria allowing the phage DNA to circularize into superhelical molecules. After drug treatment DNA single- and double-strand breaks were measured independently after neutral sucrose gradient sedimentation. The presence of alkali-labile lesions was measured in parallel in alkaline sucrose gradients. The cell envelope provided an efficient protection towards the drug, since no strand breaks were detected unless the cells were made permeable with toluene or with hypotonic Tris buffer. In permeable cells, no double strand breaks could be detected, even at high NCS concentration (100 micrograms/ml). Induction of single-strand breaks leveled off after 15 min at 20 degrees C in the presence of 2 mM mercaptoethanol. Exposure to 0.3N NaOH doubled the number of strand breaks. No enzymatic repair of the breaks could be observed.
新制癌菌素在大肠杆菌细胞中诱导产生的DNA链断裂已得到表征。将放射性标记的噬菌体λDNA引入溶原性宿主细菌中,使噬菌体DNA环化形成超螺旋分子。药物处理后,通过中性蔗糖梯度沉降分别测量DNA单链和双链断裂情况。同时在碱性蔗糖梯度中测量碱不稳定损伤的存在情况。细胞膜对药物提供了有效的保护,因为除非用甲苯或低渗Tris缓冲液使细胞通透,否则检测不到链断裂。在通透的细胞中,即使在高浓度新制癌菌素(100微克/毫升)下也检测不到双链断裂。在2毫摩尔巯基乙醇存在的情况下,20℃下15分钟后单链断裂的诱导趋于平稳。暴露于0.3N氢氧化钠会使链断裂的数量增加一倍。未观察到断裂的酶促修复。
