Dixit M, Yang J L, Poirier M C, Price J O, Andrews P A, Arteaga C L
Department of Medicine, Vanderbilt University School of Medicine, Nashville, TN 37232-5536, USA.
J Natl Cancer Inst. 1997 Mar 5;89(5):365-73. doi: 10.1093/jnci/89.5.365.
Epidermal growth factor receptor (EGF-R) perturbation by receptor ligand(s), e.g., epidermal growth factor (EGF) and transforming growth factor-alpha (TGF-alpha), or receptor-specific antibodies accentuates cisplatin-induced toxicity in tumor cells. This sensitization occurs only in tumor cells with high expression of EGF-R but not in those with low expression of EGF-R.
Therefore, we have studied the role of EGF-R expression on cisplatin-mediated cytotoxicity.
MDA-468 human breast cancer cells were stably transfected with a p-chloramphenicol acetyl transferase (pact[p]-CAT) vector containing a 4.1-kilobase full-length antisense EGF-R complementary DNA. EGF-R content was assessed by 125I-EGF binding and EGF-R immunoblot assays. Cisplatin sensitivity was evaluated by (a) colony-forming assay in vitro, (b) xenograft growth in nude mice, (c) cell cycle distribution of propidium iodide-labeled DNA, (d) DNA fragmentation in agarose gels, and (e) terminal deoxynucleotidyl transferase (Tdt) fluorescence in situ. Cisplatin uptake was measured by atomic absorption spectroscopy, and the levels of drug-DNA intrastrand adducts were determined by a dissociation-enhanced fluoroimmunoassay that utilizes an antibody against cisplatin-modified DNA.
Selected clones (MDA-468/AS-EGFR) exhibited more than 90% loss of both 125I-EGF binding and receptor content determined by western blot analysis, whereas clones transfected with the vector alone (MDA-468/p-CAT) had EGF-R levels similar to those of the parent cells. By use of a colony-forming assay, the 1-hour IC50 (i.e., the concentration of drug required for 1 hour to achieve 50% cell kill) for cisplatin was 2 microM or less for parental and vector-transfected clones (n = 4), whereas it was 25 microM or more for all MDA-468/AS-EGFR clones (n = 3). MDA-468/p-CAT clones exhibited internucleosomal DNA fragmentation, enhanced Tdt-end labeling in situ, and G2 arrest 48 hours after a 1-hour incubation with 3-30 microM cisplatin. Under these conditions, apoptosis and G2 arrest were undetectable in all MDA-468/AS-EGFR clones. An MDA-468 subline selected after long-term treatment with a TGF-alpha-Pseudomonas exotoxin A fusion protein 40 lacked EGF binding and also exhibited cisplatin resistance (1-hour IC50: > 30 microM) compared with parental cells. This EGF-R-dependent difference in cisplatin response was confirmed in a nude mouse xenograft model by use of high- and low-EGF-R-expressing cell clones. Total intracellular drug accumulation after a 1-hour cisplatin exposure, as measured by atomic absorption spectroscopy, was identical in both groups of cells. Intrastrand drug-DNA adducts, however, were statistically higher in high EGF-R expressors than in low-EGF-R-expressing clones.
These data indicate that a critical level of EGF-R signaling, which is amplified in some common human cancers, is necessary for cisplatin-mediated apoptosis in tumor cells and suggest an inhibitory effect of this pathway on the repair of cisplatin-damaged DNA.
受体配体(如表皮生长因子(EGF)和转化生长因子-α(TGF-α))或受体特异性抗体对表皮生长因子受体(EGF-R)的干扰会增强顺铂对肿瘤细胞的毒性。这种致敏作用仅发生在EGF-R高表达的肿瘤细胞中,而在EGF-R低表达的肿瘤细胞中则不会发生。
因此,我们研究了EGF-R表达在顺铂介导的细胞毒性中的作用。
用含有4.1千碱基全长反义EGF-R互补DNA的对氯苯甲酰转移酶(pact[p]-CAT)载体稳定转染MDA-468人乳腺癌细胞。通过¹²⁵I-EGF结合和EGF-R免疫印迹分析评估EGF-R含量。通过以下方法评估顺铂敏感性:(a)体外集落形成试验;(b)裸鼠异种移植瘤生长情况;(c)碘化丙啶标记DNA的细胞周期分布;(d)琼脂糖凝胶中的DNA片段化;(e)末端脱氧核苷酸转移酶(Tdt)荧光原位检测。通过原子吸收光谱法测量顺铂摄取量,并通过利用抗顺铂修饰DNA抗体的解离增强荧光免疫测定法测定药物-DNA链内加合物的水平。
通过蛋白质免疫印迹分析,所选克隆(MDA-468/AS-EGFR)的¹²⁵I-EGF结合和受体含量均损失超过90%,而仅用载体转染的克隆(MDA-468/p-CAT)的EGF-R水平与亲本细胞相似。通过集落形成试验,亲本细胞和载体转染的克隆(n = 4)的顺铂1小时半数抑制浓度(IC50,即1小时内达到50%细胞杀伤所需的药物浓度)为2μM或更低,而所有MDA-468/AS-EGFR克隆(n = 3)的该浓度为25μM或更高。MDA-468/p-CAT克隆在与3 - 30μM顺铂孵育1小时后48小时出现核小体间DNA片段化、原位Tdt末端标记增强和G2期阻滞。在这些条件下,所有MDA-468/AS-EGFR克隆均未检测到凋亡和G2期阻滞。用TGF-α-绿脓杆菌外毒素A融合蛋白40长期处理后选择的MDA-468亚系缺乏EGF结合,与亲本细胞相比也表现出顺铂抗性(1小时IC50:> 30μM)。通过使用高表达和低表达EGF-R的细胞克隆,在裸鼠异种移植模型中证实了这种顺铂反应中EGF-R依赖性差异。通过原子吸收光谱法测量,两组细胞在顺铂暴露1小时后的细胞内总药物积累量相同。然而,链内药物-DNA加合物在高EGF-R表达者中在统计学上高于低EGF-R表达克隆。
这些数据表明,在某些常见人类癌症中扩增的EGF-R信号传导的关键水平对于顺铂介导的肿瘤细胞凋亡是必要的,并提示该途径对顺铂损伤DNA修复具有抑制作用。
