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天然及合成维甲酸诱导人早幼粒细胞白血病HL-60细胞分化及细胞毒性的基因表达分析

Gene expression analysis of human promyelocytic leukemia HL-60 cell differentiation and cytotoxicity induced by natural and synthetic retinoids.

作者信息

Wang Jin, Fong Chi-Chun, Tzang Chi-Hung, Xiao Peigen, Han Rui, Yang Mengsu

出版信息

Life Sci. 2009 Apr 24;84(17-18):576-83.

PMID:26324987
Abstract

AIMS

This study analyzed gene expression profiles of human promyelocytic leukemia HL-60 cells treated with natural and synthetic retinoids (ATRA, RII and R9158), in an attempt to investigate the structure-function relationship of the retinoids in inducing cell differentiation and cytotoxicity.

MAIN METHODS

Flow cytometry was used to determine cell cycle changes in HL-60 cells following treatment (1.0 μM) with natural and synthetic retinoids (ATRA, RII and R9158), and cDNA microarrays were used to monitor the gene expression profiles of HL-60 cells treated with the various retinoids.

KEY FINDINGS

Consistent with retinoid-induced cell differentiation, treatment with these three retinoids correlated with an increase in the percentage of cells arrested in the G1/G0 phase of the cell cycle. Microarray analysis showed upregulation of known differentiation genes, adhesion molecules, and the oxidase activation pathway following retinoid treatment. Differential expression of several genes was observed in HL-60 cells treated with the three retinoids. For example, tissue remodeling protein genes, ubiquitin genes, and signal transduction genes were highly expressed in ATRA- and R9158-treated HL-60 cells, but remained unchanged in HL-60 cells treated with RII.

SIGNIFICANCE

The above findings suggest that the differentiation of HL-60 cells induced by the three retinoids occurs through similar pathways, and that there exists a structure-function relationship regarding retinoids and the induction of cell differentiation and cytotoxicity.

摘要

目的

本研究分析了用天然和合成类视黄醇(全反式维甲酸、RII和R9158)处理的人早幼粒细胞白血病HL-60细胞的基因表达谱,试图研究类视黄醇在诱导细胞分化和细胞毒性方面的构效关系。

主要方法

采用流式细胞术测定HL-60细胞在用天然和合成类视黄醇(全反式维甲酸、RII和R9158,1.0 μM)处理后的细胞周期变化,并用cDNA微阵列监测用各种类视黄醇处理的HL-60细胞的基因表达谱。

主要发现

与类视黄醇诱导的细胞分化一致,用这三种类视黄醇处理与细胞周期G1/G0期停滞细胞百分比的增加相关。微阵列分析显示,类视黄醇处理后已知的分化基因、粘附分子和氧化酶激活途径上调。在用三种类视黄醇处理的HL-60细胞中观察到几个基因的差异表达。例如,组织重塑蛋白基因、泛素基因和信号转导基因在全反式维甲酸和R9158处理的HL-60细胞中高表达,但在用RII处理的HL-60细胞中保持不变。

意义

上述发现表明,三种类视黄醇诱导的HL-60细胞分化通过相似途径发生,并且类视黄醇与细胞分化和细胞毒性的诱导之间存在构效关系。

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