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甲氨蝶呤处理的急性早幼粒细胞白血病细胞的表达蛋白质组学

Expression proteomics of acute promyelocytic leukaemia cells treated with methotrexate.

作者信息

Agarwal Nitin Kumar, Mueller Gerhard Anton, Mueller Claudia, Streich Jan-Henrick, Asif Abdul Rahman, Dihazi Hassan

机构信息

Department of Nephrology and Rheumatology, Center of Internal Medicine, Georg-August University Göttingen, D-37075, Göttingen, Germany.

出版信息

Biochim Biophys Acta. 2010 Apr;1804(4):918-28. doi: 10.1016/j.bbapap.2010.01.002. Epub 2010 Jan 22.

DOI:10.1016/j.bbapap.2010.01.002
PMID:20097313
Abstract

Methotrexate was first introduced as a cytotoxic agent that inhibits nucleotide biosynthesis in various cancer disorders; its molecular mechanism remains elusive. To understand the molecular mechanism by which methotrexate induces apoptosis, we analyzed the resulting intracellular protein changes in methotrexate-treated acute promyelocytic leukaemia (HL-60) cells by cysteine-labeled differential in-gel electrophoresis (CL-DIGE) combined with mass spectrometry. Initial CL-DIGE analysis revealed that 24 proteins were differentially expressed (p<0.05) in the HL-60 cell proteome after treatment with 2.5microM methotrexate for 72h. We found that three structural alpha4, alpha5, alpha7 proteasome subunits, a non-catalytic beta3 and two 26S regulatory proteasome subunits were down-regulated in methotrexate-treated HL-60 cells. Western blot analyses further showed that the inhibition of proteasome subunits is accompanied by suppression of NF-kappaB subunits and promotes the accumulation of ubiquitinated proteins. Furthermore, methotrexate activated unfolded protein response by inducing the expression of endoplasmic reticulum-resident proteins such as calreticulin, protein disulphide isomerase A3 and A4, and 78kDa glucose regulated protein in a time-dependent manner. Altogether, our findings demonstrated that targeting NF-kappaB, structural and regulatory proteasome subunits with methotrexate may provide new insight into understanding methotrexate-induced apoptotic activities in HL-60 cells.

摘要

甲氨蝶呤最初作为一种细胞毒性药物被引入,用于抑制各种癌症疾病中的核苷酸生物合成;其分子机制仍不清楚。为了了解甲氨蝶呤诱导细胞凋亡的分子机制,我们通过半胱氨酸标记差异凝胶电泳(CL-DIGE)结合质谱分析了甲氨蝶呤处理的急性早幼粒细胞白血病(HL-60)细胞中产生的细胞内蛋白质变化。最初的CL-DIGE分析显示,用2.5微摩尔甲氨蝶呤处理72小时后,HL-60细胞蛋白质组中有24种蛋白质表达差异(p<0.05)。我们发现,在甲氨蝶呤处理的HL-60细胞中,三种结构α4、α5、α7蛋白酶体亚基、一种非催化性β3和两种26S调节蛋白酶体亚基表达下调。蛋白质印迹分析进一步表明,蛋白酶体亚基的抑制伴随着NF-κB亚基的抑制,并促进泛素化蛋白的积累。此外,甲氨蝶呤通过时间依赖性诱导内质网驻留蛋白如钙网蛋白、蛋白二硫键异构酶A3和A4以及78kDa葡萄糖调节蛋白的表达来激活未折叠蛋白反应。总之,我们的研究结果表明,用甲氨蝶呤靶向NF-κB、结构和调节蛋白酶体亚基可能为理解甲氨蝶呤在HL-60细胞中诱导的凋亡活性提供新的见解。

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