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Molecular mechanism of apoptosis and gene expressions in human lymphoma U937 cells treated with anisomycin.

机译:茴香霉素处理的人淋巴瘤U937细胞凋亡和基因表达的分子机制。

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Anisomycin is known as a potent apoptosis inducer by activating JNK/SAPK and inhibiting protein synthesis during translation. However, only few details are known about the mechanism of apoptosis induced by this compound. The present study was undertaken to further elucidate the molecular mechanism of apoptosis and the changes of gene expression elicited by anisomycin using DNA microarrays and computational gene-expression analysis tools in human lymphoma U937 cells. Anisomycin was found to induce apoptosis in time- and concentration-dependent manner as confirmed by phosphatidylserine externalization and DNA fragmentation analysis. Furthermore, anisomycin-treated cells also showed caspase-8 activation, mitochondrial membrane potential collapse, Bid activation, caspase-3 cleavage and cytochrome c release into the cytosol. In the gene-expression analysis, six gene clusters were detected. From clusters I and II, three significant genetic networks were identified. Interestingly, many bZIP family transcription factors were observed in the up-regulated genetic networks. Moreover, the expression of protein-synthesis-related genes, such as EIF4 family proteins and ribosomal proteins, were inhibited. This finding could explain the reason why anisomycin inhibits the protein synthesis at the translation steps. These results provide novel information for understanding the molecular mechanism of apoptosis induced by anisomycin.
机译:通过激活JNK / SAPK并抑制翻译过程中的蛋白质合成,茴香霉素被称为有效的凋亡诱导剂。然而,关于该化合物诱导的细胞凋亡的机制只有很少的细节。本研究的目的是进一步阐明使用DNA芯片和计算基因表达分析工具在人淋巴瘤U937细胞中凋亡和由茴香霉素引起的基因表达变化的分子机制。如磷脂酰丝氨酸外在化和DNA片段化分析所证实,发现茴香霉素以时间和浓度依赖性方式诱导凋亡。此外,经茴香霉素处理的细胞还显示caspase-8激活,线粒体膜电位崩溃,Bid激活,caspase-3裂解和细胞色素c释放到细胞质中。在基因表达分析中,检测到六个基因簇。从第一类和第二类中,确定了三个重要的遗传网络。有趣的是,在上调的遗传网络中观察到许多bZIP家族转录因子。此外,蛋白质合成相关基因,如EIF4家族蛋白和核糖体蛋白的表达受到抑制。这一发现可以解释茴香霉素在翻译步骤中抑制蛋白质合成的原因。这些结果为了解茴香霉素诱导的细胞凋亡的分子机制提供了新的信息。

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