Lin Mao-Fang, Qian Xi-Jun
Department of Hematology, The First Affiliated Hospital, Medical College of Zhejiang University, Hangzhou 310003, China.
Zhongguo Shi Yan Xue Ye Xue Za Zhi. 2006 Jun;14(3):471-6.
This study was purposed to investigate whether aminopeptidase inhibitor, bestatin, can potentiate all-trans retinoic acid (ATRA)-inducing differentiation in NB4 cells, and to explore its mechanism. The NB4 cells were exposed to either bestatin and ATRA alone or in combination, the morphological changes of NB4 cells were observed by optical microscopy, the CD11b expression was measured by flow cytometry, the function of defferentiation cells was analyzed by nitroblue-tetrazolium (NBT) reduction assay, the mRNA expressions of c-myc and c-EBPepsilon in NB4 cells were detected by RT-PCR, the c-Myc protein expression was determined by Western blot. The results showed that treatment with bestatin alone induced no significant changes in morphology, NBT reduction activity and CD11b expression in NB4 cells. NB4 cells incubated with 10 nmol/L ATRA plus 100 microg/ml bestatin showed more morphologic feature of metamyelocyte and band neutrophil than ATRA alone treated cells. 100 microg/ml bestatin enhanced the NBT reduction activity in NB4 cells induced by various concentrations of ATRA (10, 20, 40 nmol/L). The effects of various concentrations of ATRA in combination with 100 microg/ml bestatin were statistically different from the effect of ATRA alone (P < 0.01). From 48 to 96 hours, 100 microg/ml bestatin time-dependently increased NBT reduction in NB4 cells induced by 10 nmol/L ATRA (P < 0.01). 10 nmol/L ATRA plus 100 microg/ml bestatin for 72 hours prominently elevated CD11b expression in NB4 cells as compared with ATRA alone treated NB4 cells (P < 0.01). There was a substantial decrease in c-myc mRNA levels when 100 microg/ml bestatin was added to 10 nmol/L ATRA (P < 0.05). Various concentrations (50, 75, 100 microg/ml) of bestatin combined with 10 nmol/L ATRA down-regulated the expression of c-Myc protein, which was negatively correlated with the NBT reduction activity of NB4 cells induced by 10 nmol/L ATRA alone or plus bestatin at various concentrations (r = -0.940, P = 0.017). However, 100 microg/ml bestatin plus 10 nmol/L ATRA could not induce any significant changes in the levels of c-EBPepsilon mRNA as compared with ATRA alone treated NB4 cells. It is concluded that an aminopeptidase inhibitor bestatin can potentiate ATRA-inducing differentiation of NB4 cells, possibly by down-regulating c-myc expression in synergy with ATRA.
本研究旨在探讨氨肽酶抑制剂苯丁抑制素是否能增强全反式维甲酸(ATRA)诱导NB4细胞分化的作用,并探讨其作用机制。将NB4细胞分别单独或联合暴露于苯丁抑制素和ATRA中,通过光学显微镜观察NB4细胞的形态变化,采用流式细胞术检测CD11b表达,通过硝基蓝四氮唑(NBT)还原试验分析分化细胞的功能,用逆转录聚合酶链反应(RT-PCR)检测NB4细胞中c-myc和c-EBPε的mRNA表达,用蛋白质免疫印迹法检测c-Myc蛋白表达。结果显示,单独用苯丁抑制素处理对NB4细胞的形态、NBT还原活性及CD11b表达无明显影响。与单独用ATRA处理的细胞相比,用10 nmol/L ATRA加100 μg/ml苯丁抑制素孵育的NB4细胞表现出更多中幼粒细胞和带状中性粒细胞的形态特征。100 μg/ml苯丁抑制素增强了不同浓度(10、20、40 nmol/L)ATRA诱导的NB4细胞的NBT还原活性。不同浓度的ATRA与100 μg/ml苯丁抑制素联合作用的效果与单独用ATRA的效果相比差异有统计学意义(P<0.01)。在48至96小时内,100 μg/ml苯丁抑制素能使10 nmol/L ATRA诱导的NB4细胞的NBT还原呈时间依赖性增加(P<0.01)。与单独用ATRA处理的NB4细胞相比,10 nmol/L ATRA加100 μg/ml苯丁抑制素作用72小时可显著提高NB4细胞中CD11b的表达(P<0.01)。当100 μg/ml苯丁抑制素加入10 nmol/L ATRA中时,c-myc mRNA水平显著降低(P<0.05)。不同浓度(50、75、100 μg/ml)的苯丁抑制素与10 nmol/L ATRA联合可下调c-Myc蛋白表达,这与单独用10 nmol/L ATRA或加不同浓度苯丁抑制素诱导的NB4细胞的NBT还原活性呈负相关(r=-0.940,P=0.017)。然而,与单独用ATRA处理的NB4细胞相比,100 μg/ml苯丁抑制素加10 nmol/L ATRA对c-EBPε mRNA水平无明显影响。结论是氨肽酶抑制剂苯丁抑制素可增强ATRA诱导的NB4细胞分化,可能是通过与ATRA协同下调c-myc表达来实现的。
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