首页> 外文期刊>Journal of biomolecular screening: The official journal of the Society for Biomolecular Screening >Evaluation of different glutathione S-transferase-tagged protein captures for screening E6/E6AP interaction inhibitors using AlphaScreen (R)
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Evaluation of different glutathione S-transferase-tagged protein captures for screening E6/E6AP interaction inhibitors using AlphaScreen (R)

机译:使用AlphaScreen(R)评估不同的谷胱甘肽S-转移酶标签的蛋白质捕获以筛选E6 / E6AP相互作用抑制剂

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摘要

Human papillomavirus (HPV) infection is responsible for the development of cervical cancer and its premalignant lesions in women. The virus-encoded oncogene E6 is a promising target for an anti-HPV drug therapy. The authors describe the development of a homogenous screening assay for inhibitors of the E6 interaction with its cellular target, the E6-associated protein (E6AP), based on AlphaScreen (R) technology. The E6 protein was expressed and purified as glutathione S-transferase (GST) fusion protein, and the binding to a biotinylated E6AP peptide was monitored using GST-detecting Acceptor beads coated either with anti-GST antibody or glutathione. After optimization of the assay conditions, a commercial library of 3000 compounds was screened for inhibitors. Active compounds were retested and counterscreened for E6/E6AP specificity using biotinylated GST as a control protein. The results obtained with both types of GST-detecting reagents correlated very well and demonstrated the great potential of the newly developed glutathione-coated Acceptor beads as a detection reagent for GST fusion proteins.
机译:人乳头瘤病毒(HPV)感染是导致妇女宫颈癌及其癌变前病变的原因。病毒编码的癌基因E6是抗HPV药物治疗的有希望的靶标。作者描述了基于AlphaScreen(R)技术的E6与细胞靶标E6相关蛋白(E6AP)相互作用抑制剂的同质筛选试验的开发。 E6蛋白被表达并纯化为谷胱甘肽S-转移酶(GST)融合蛋白,并使用涂有抗GST抗体或谷胱甘肽的GST检测受体珠来监测与生物素化E6AP肽的结合。优化测定条件后,筛选了3000种化合物的商业文库中的抑制剂。重新测试活性化合物,并使用生物素化的GST作为对照蛋白对E6 / E6AP特异性进行反筛选。两种类型的GST检测试剂获得的结果都具有很好的相关性,并证明了新开发的谷胱甘肽涂层受体珠作为GST融合蛋白检测试剂的巨大潜力。

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