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首页> 外文期刊>Toxicology mechanisms and methods >Proteomic Analysis to Identify the Cellular Responses Induced by Hydroquinone in Human Embryonic Lung Fibroblasts
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Proteomic Analysis to Identify the Cellular Responses Induced by Hydroquinone in Human Embryonic Lung Fibroblasts

机译:蛋白质组学分析,以确定对苯二酚诱导人胚肺成纤维细胞的细胞反应。

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摘要

Hydroquinone (HQ), a major metabolite of benzene, is used widely as a reagent in photographic developers, as an antioxidant in the manufacture of rubber, as a polymerization inhibitor for acrylic and vinyl acetate monomers, and in cosmetic products as a skin-lightening agent. But the mechanism of its effect on human cells is far from clear. In the present work, we studied the cellular response induced by HQ using proteomic approaches. Human embryonic lung fibroblasts (HLFs) were treated with 100 muM HQ for 24 h. This dose of HQ was found in assays to significantly decrease cell viability. After treatment, two-dimensional electrophoresis was performed using the Amersham Bioscience 2DE system following the manufacturer's instructions. Proteins were visualized by staining with colloidal coomassie blue. Fifteen protein spots showed significant changes after HQ treatment. Eleven protein spots were identified by peptide mass fingerprinting using MALDI-TOF or by peptide sequence tagging using MALDI-TOF-TOF. Among them are transaldolase, growth factor receptor-bound protein 2, mutant beta-actin, 7-actin, Lasp-1, TAR DNA-binding protein, and a protein similar to neural precursor cell-expressed protein. These include proteins involved in oxidative stress, cellular signaling, RNA splicing, and cytoskeleton reconstruction. Most of their involvements in the cellular responses to HQ have not been reported. Therefore,our findings may offer new insights into the mechanisms of HQ cytotoxicity and these proteins may serve as new biomarkers for detecting exposure of human populations to HQ. It is suggested that proteomic approaches may provide new strategies to evaluate the toxicity of xenobiotics.
机译:对苯二酚(HQ)是苯的主要代谢产物,已广泛用作照相显影剂中的试剂,橡胶生产中的抗氧化剂,丙烯酸和乙酸乙烯酯单体的阻聚剂以及化妆品中的亮肤剂。代理商。但是,其对人体细胞的作用机理尚不清楚。在目前的工作中,我们研究了使用蛋白质组学方法由HQ诱导的细胞反应。将人胚胎肺成纤维细胞(HLF)用100μMHQ处理24小时。在测定中发现此剂量的HQ可显着降低细胞活力。处理后,使用Amersham Bioscience 2DE系统按照制造商的说明进行二维电泳。通过用胶体考马斯蓝染色使蛋白质可视化。 HQ处理后有15个蛋白质斑点显示出显着变化。通过使用MALDI-TOF的肽质量指纹识别或通过使用MALDI-TOF-TOF的肽序列标记识别了11个蛋白斑点。其中有转醛缩酶,生长因子受体结合蛋白2,突变体β-肌动蛋白,7-肌动蛋白,Lasp-1,TAR DNA结合蛋白和类似于神经前体细胞表达蛋白的蛋白。这些包括涉及氧化应激,细胞信号转导,RNA剪接和细胞骨架重建的蛋白质。他们的大多数参与对总部的细胞反应尚未报道。因此,我们的发现可能会提供有关HQ细胞毒性机制的新见解,并且这些蛋白质可能会成为检测人群暴露于HQ的新生物标记。有人认为,蛋白质组学方法可能为评估异种生物的毒性提供新的策略。

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