Caetano-Pinto Pedro, Jamalpoor Amer, Ham Janneke, Goumenou Anastasia, Mommersteeg Monique, Pijnenburg Dirk, Ruijtenbeek Rob, Sanchez-Romero Natalia, van Zelst Bertrand, Heil Sandra G, Jansen Jitske, Wilmer Martijn J, van Herpen Carla M L, Masereeuw Rosalinde
Division of Pharmacology, Utrecht Institute for Pharmaceutical Sciences, Faculty of Science, Utrecht University , 3584 CG Utrecht, The Netherlands.
Department of Oncology, Radboud University Medical Center , 6525 GA Nijmegen, The Netherlands.
Mol Pharm. 2017 Jun 5;14(6):2147-2157. doi: 10.1021/acs.molpharmaceut.7b00308. Epub 2017 May 24.
The combination of methotrexate with epidermal growth factor receptor (EGFR) recombinant antibody, cetuximab, is currently being investigated in treatment of head and neck carcinoma. As methotrexate is cleared by renal excretion, we studied the effect of cetuximab on renal methotrexate handling. We used human conditionally immortalized proximal tubule epithelial cells overexpressing either organic anion transporter 1 or 3 (ciPTEC-OAT1/ciPTEC-OAT3) to examine OAT1 and OAT3, and the efflux pumps breast cancer resistance protein (BCRP), multidrug resistance protein 4 (MRP4), and P-glycoprotein (P-gp) in methotrexate handling upon EGF or cetuximab treatment. Protein kinase microarrays and knowledge-based pathway analysis were used to predict EGFR-mediated transporter regulation. Cytotoxic effects of methotrexate were evaluated using the dimethylthiazol bromide (MTT) viability assay. Methotrexate inhibited OAT-mediated fluorescein uptake and decreased efflux of Hoechst33342 and glutathione-methylfluorescein (GS-MF), which suggested involvement of OAT1/3, BCRP, and MRP4 in transepithelial transport, respectively. Cetuximab reversed the EGF-increased expression of OAT1 and BCRP as well as their membrane expressions and transport activities, while MRP4 and P-gp were increased. Pathway analysis predicted cetuximab-induced modulation of PKC and PI3K pathways downstream EGFR/ERBB2/PLCg. Pharmacological inhibition of ERK decreased expression of OAT1 and BCRP, while P-gp and MRP4 were increased. AKT inhibition reduced all transporters. Exposure to methotrexate for 24 h led to a decreased viability, an effect that was reversed by cetuximab. In conclusion, cetuximab downregulates OAT1 and BCRP while upregulating P-gp and MRP4 through an EGFR-mediated regulation of PI3K-AKT and MAPKK-ERK pathways. Consequently, cetuximab attenuates methotrexate-induced cytotoxicity, which opens possibilities for further research into nephroprotective comedication therapies.
甲氨蝶呤与表皮生长因子受体(EGFR)重组抗体西妥昔单抗联合用药目前正处于治疗头颈癌的研究阶段。由于甲氨蝶呤通过肾脏排泄清除,我们研究了西妥昔单抗对肾脏处理甲氨蝶呤的影响。我们使用过表达有机阴离子转运体1或3的人条件永生化近端肾小管上皮细胞(ciPTEC - OAT1/ciPTEC - OAT3)来检测OAT1和OAT3,以及在表皮生长因子(EGF)或西妥昔单抗处理后甲氨蝶呤处理过程中的外排泵乳腺癌耐药蛋白(BCRP)、多药耐药蛋白4(MRP4)和P - 糖蛋白(P - gp)。使用蛋白激酶微阵列和基于知识的通路分析来预测EGFR介导的转运体调控。使用二甲基噻唑溴化物(MTT)活力测定法评估甲氨蝶呤的细胞毒性作用。甲氨蝶呤抑制OAT介导的荧光素摄取,并减少Hoechst33342和谷胱甘肽 - 甲基荧光素(GS - MF)的外排,这分别表明OAT1/3、BCRP和MRP4参与了跨上皮转运。西妥昔单抗逆转了EGF诱导的OAT-1和BCRP的表达增加以及它们的膜表达和转运活性,而MRP4和P - gp则增加。通路分析预测西妥昔单抗诱导EGFR/ERBB2/PLCg下游的PKC和PI3K通路的调节。ERK的药理抑制降低了OAT1和BCRP的表达,而P - gp和MRP4增加。AKT抑制降低了所有转运体。暴露于甲氨蝶呤24小时导致活力下降,这种作用被西妥昔单抗逆转。总之,西妥昔单抗通过EGFR介导的PI3K - AKT和MAPKK - ERK通路调节下调OAT1和BCRP,同时上调P - gp和MRP4。因此,西妥昔单抗减弱了甲氨蝶呤诱导的细胞毒性,这为进一步研究肾保护联合用药疗法开辟了可能性。
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