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采用空气中微束质子激发 X 射线荧光法对人食管鳞癌细胞系顺铂敏感性的定量分析。

Quantitative analysis of cisplatin sensitivity of human esophageal squamous cancer cell lines using in-air micro-PIXE.

机构信息

Department of General Surgical Science, Gunma University, Maebashi, Japan.

出版信息

Cancer Sci. 2010 Jun;101(6):1487-92. doi: 10.1111/j.1349-7006.2010.01542.x. Epub 2010 Jan 25.

Abstract

Cisplatin is a key chemotherapeutic agent for the treatment of esophageal cancer. We examined the intracellular localization of cisplatin in esophageal cancer cell lines and determined their sensitivity to cisplatin using in-air micro-PIXE (particle induced X-ray emission). Two human esophageal squamous cell carcinoma (ESCC) cell lines, TE-2 and TE-13, were examined for their response to cisplatin using MTT assay, flow cytometry, and DNA fragmentation assays. Real-time reverse transcription-polymerase chain reaction was also used to evaluate the mRNA expression of multidrug resistance protein 2 (MRP2) in both cell lines. Platinum localizations of intracellular and intranuclear were measured using in-air micro-PIXE. TE-2 cells were more sensitive to cisplatin than TE-13 cells (IC(50): 37.5 mum and 56.3 mum, respectively). Flow cytometry analysis confirmed that more TE-2 than TE-13 cells were in the sub-G1 phase. DNA fragmentation assay was analyzed to confirm the MTT assay and flow cytometry results. The expression of MRP2 mRNA in TE-13 cells was stronger than in TE-2 cells. In-air micro-PIXE showed that TE-2 cells had higher intracellular cisplatin concentrations than TE-13 cells and the ratio of intranuclear to intracellular cisplatin in individual cells was not significantly different. We observed the intracellular and intranuclear localization of cisplatin using in-air micro-PIXE. The results of this study suggest that in-air micro-PIXE could be a useful quantitative method for evaluating the cisplatin sensitivity of individual cells. Finally, we speculate that MRP2 in the cell membrane may play an important role in regulating the cisplatin sensitivity of ESCC cells.

摘要

顺铂是治疗食管癌的一种重要化疗药物。我们研究了顺铂在食管癌细胞系中的细胞内定位,并使用空气中微束质子诱导 X 射线发射(micro-PIXE)技术测定了它们对顺铂的敏感性。使用 MTT 检测法、流式细胞术和 DNA 片段化检测法,我们检测了两种人食管鳞状细胞癌(ESCC)细胞系 TE-2 和 TE-13 对顺铂的反应。还使用实时逆转录聚合酶链反应(real-time RT-PCR)评估了这两种细胞系中多药耐药蛋白 2(MRP2)的 mRNA 表达。使用空气中微束质子诱导 X 射线发射技术测定了细胞内和核内铂的定位。TE-2 细胞比 TE-13 细胞对顺铂更敏感(IC50:分别为 37.5 µm 和 56.3 µm)。流式细胞术分析证实,TE-2 细胞比 TE-13 细胞更多地处于亚 G1 期。DNA 片段化检测用于证实 MTT 检测法和流式细胞术的结果。TE-13 细胞中 MRP2 mRNA 的表达强于 TE-2 细胞。空气中微束质子诱导 X 射线发射显示,TE-2 细胞的细胞内顺铂浓度高于 TE-13 细胞,单个细胞核内与细胞内顺铂的比值无显著差异。我们使用空气中微束质子诱导 X 射线发射观察了顺铂的细胞内和核内定位。本研究结果表明,空气中微束质子诱导 X 射线发射可能是评估单个细胞顺铂敏感性的一种有用的定量方法。最后,我们推测细胞膜上的 MRP2 可能在调节 ESCC 细胞对顺铂的敏感性方面发挥重要作用。

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