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Establishment of a melanogenesis regulation assay system using a fluorescent protein reporter combined with the promoters for the melanogenesis-related genes in human melanoma cells

机译:使用荧光蛋白报告基因与人黑色素瘤细胞中与黑色素生成相关基因的启动子结合的黑色素生成调节测定系统的建立

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There are two established depigmenting agent assays currently in use. However, these methods are unreliable and time-consuming. Therefore, it will be valuable to establish a better assay system for depigmenting agent analysis. In this study, we established a melanogenesis regulation assay system using a fluorescent protein reporter combined with the promoters for the microphthalmia-associated transcription factor (MITF), tyrosinase (Tyr) and dopachrome tautomerase (Dct) genes in MeWo human melanoma cells. We used several melanogenesis regulators, including theophylline, hesperetin, arbutin and rottlerin, to confirm the function of this assay system. The established MeWo/pMITF-EGFP, MeWo/pTyr-EGFP and MeWo/pDct-EGFP stable cells integrated the pMITF-EGFP, pTyr-EGFP and pDct-EGFP plasmids into their genomic DNA. These stably transfected cells were used to examine alterations in the expression of the MITF, Tyr and Dct genes. All of the tested compounds, including theophylline, hesperetin, arbutin and rottlerin, could be analyzed in the stable cells, producing reliable results. Therefore, we believe that this melanogenesis regulation assay system can be used as a rapid and reliable assay system to analyze the regulation of melanogenesis by many known or unknown compounds. (C) 2014 Elsevier Inc. All rights reserved.
机译:目前有两种已建立的脱色剂测定法。但是,这些方法不可靠且耗时。因此,建立更好的色素脱色剂分析系统将是很有价值的。在这项研究中,我们建立了一个黑色素生成调节测定系统,该系统使用荧光蛋白报道分子与MeWo人黑色素瘤细胞中与小眼症相关转录因子(MITF),酪氨酸酶(Tyr)和多巴色素互变异构酶(Dct)基因的启动子结合。我们使用了多种黑色素生成调节剂,包括茶碱,橙皮素,熊果苷和rottlerin,以确认该测定系统的功能。已建立的MeWo / pMITF-EGFP,MeWo / pTyr-EGFP和MeWo / pDct-EGFP稳定细胞将pMITF-EGFP,pTyr-EGFP和pDct-EGFP质粒整合到其基因组DNA中。这些稳定转染的细胞用于检查MITF,Tyr和Dct基因表达的变化。所有测试的化合物,包括茶碱,橙皮素,熊果苷和rottlerin,都可以在稳定的细胞中进行分析,从而获得可靠的结果。因此,我们相信该黑色素生成调节测定系统可以用作快速可靠的测定系统,以分析许多已知或未知化合物对黑色素生成的调节。 (C)2014 Elsevier Inc.保留所有权利。

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