Nadin Silvina Beatriz, Vargas-Roig Laura M, Drago Gisela, Ibarra Jorge, Ciocca Daniel R
Oncology Laboratory, Institute of Experimental Medicine and Biology of Cuyo, Regional Center for Scientific and Technological Research, C.C.855, C.P. 5500 Mendoza, Argentina.
Cancer Lett. 2006 Jul 28;239(1):84-97. doi: 10.1016/j.canlet.2005.07.025. Epub 2005 Sep 6.
Drug resistance is considered the main impediment to successful cancer chemotherapy. The quest for a method useful to predict individual responses to chemotherapy prior to treatment is highly desired. This study was designed to determine the individual influences of doxorubicin and cisplatin on the degree of DNA damage, DNA repair and hMSH2 and the hMLH1 protein expression in peripheral blood lymphocytes (PBL) and their correlations with the clinical response. PBL were obtained from 25 cancer patients (pre- and post-chemotherapy) and from 10 healthy persons, cultured and exposed to doxorubicin or cisplatin. Cells were collected at T0 (immediately after drug treatment) and 24h after damage (T24). The alkaline comet assay was employed to assess the DNA damage and repair function, and immunocytochemistry to study hMLH1 and hMSH2 expression. Clinical response was evaluated after three cycles of chemotherapy. Pre-chemotherapy PBL from cancer patients showed significantly higher levels of basal DNA damage than healthy persons, with appreciable interindividual variations between them. The in vivo administration of antineoplasic drugs was accompanied by significant DNA damage, and an increased in the number of apoptotic cells. Cancer patients with complete response showed a high number of apoptotic cells. The DNA migration increased at T0 and at T24 in cisplatin-treated patients, reflecting a decreased rate of cisplatin adducts repair than that observed in healthy individuals. The ability to repair DNA lesions in doxorubicin-damaged cells was very similar between healthy individuals and cancer patients. Cisplatin-treated patients that died by the disease showed lower DNA migration than the mean value. The expression of hMLH1 and hMSH2 was practically identical between healthy individuals and cancer patients. Nevertheless, chemotherapy induced a depletion mostly of hMLH1. In 83% of cisplatin-treated patients with CR the hMLH1 and hMSH2 expression at T24 was higher than the mean. In this pilot study the alkaline comet assay offered information about the amount of DNA damage and the DNA repair status in PBL from individual patients and this seems useful in predicting the response to chemotherapy.
耐药性被认为是癌症化疗成功的主要障碍。人们迫切希望找到一种方法,能够在治疗前预测个体对化疗的反应。本研究旨在确定阿霉素和顺铂对外周血淋巴细胞(PBL)中DNA损伤程度、DNA修复以及hMSH2和hMLH1蛋白表达的个体影响,及其与临床反应的相关性。PBL取自25例癌症患者(化疗前后)和10名健康人,进行培养并暴露于阿霉素或顺铂。在T0(药物治疗后立即)和损伤后24小时(T24)收集细胞。采用碱性彗星试验评估DNA损伤和修复功能,并用免疫细胞化学研究hMLH1和hMSH2表达。化疗三个周期后评估临床反应。癌症患者化疗前的PBL显示出比健康人更高的基础DNA损伤水平,且个体间存在明显差异。体内给予抗肿瘤药物伴随着显著的DNA损伤和凋亡细胞数量增加。完全缓解的癌症患者显示出大量凋亡细胞。顺铂治疗患者在T0和T24时DNA迁移增加,这反映出顺铂加合物的修复率低于健康个体。健康个体和癌症患者中,阿霉素损伤细胞修复DNA损伤的能力非常相似。死于该疾病的顺铂治疗患者显示出低于平均值的DNA迁移。健康个体和癌症患者中hMLH1和hMSH2的表达几乎相同。然而,化疗主要导致hMLH1减少。在83%的完全缓解的顺铂治疗患者中,T24时hMLH1和hMSH2的表达高于平均值。在这项初步研究中,碱性彗星试验提供了关于个体患者PBL中DNA损伤量和DNA修复状态的信息,这似乎有助于预测化疗反应。
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