首页> 外文期刊>Journal of chromatography, B. Analytical technologies in the biomedical and life sciences >Characterization of proteinase activation dynamics by capillary electrophoresis conjugating with fluorescent protein-based probe
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Characterization of proteinase activation dynamics by capillary electrophoresis conjugating with fluorescent protein-based probe

机译:毛细管电泳与基于荧光蛋白的探针偶联,表征蛋白酶激活动力学

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In this paper, a novel strategy was reported to characterize dynamics of proteinase activation based on capillary electrophoresis (CE), using caspase-2 as the model system. A fusion protein conjugating an amino acid sequence VDVAD with two fluorescent proteins enhanced cyan fluorescence protein (ECFP) and red fluorescence protein (DsRed), ECFP-VDVAD-DsRed, was specially designed and expressed in HeLa cells as the substrate of proteinase caspase-2. In this substrate, the sequence VDVAD could be specifically recognized and cleaved by caspase-2 as soon as its activation was initiated with treatment of a certain dose of cisplatin to HeLa cells, which led to a break of the substrate into two fragments. Analyses of the cell lysates using CE in a time course of the apoptosis illustrated the dynamics of caspase-2 activation. It showed that the employment of fusion fluorescent protein greatly facilitated both CE separation and identification of the analytes. This result from cell colony by CE was compared with that from single cell achieved by optical imaging. (c) 2006 Elsevier B.V. All rights reserved.
机译:在本文中,报道了一种新的策略,以caspase-2为模型系统,基于毛细管电泳(CE)表征蛋白酶激活的动力学。特别设计了融合氨基酸序列VDVAD和两种荧光蛋白的融合蛋白,增强了蓝绿色荧光蛋白(ECFP)和红色荧光蛋白(DsRed)ECFP-VDVAD-DsRed,并在HeLa细胞中表达为蛋白酶caspase-2的底物。 。在此底物中,只要用一定剂量的顺铂处理HeLa细胞就可以激活caspase-2,序列就可以被caspase-2特异性识别并切割,从而导致底物分解为两个片段。在凋亡的时间过程中使用CE对细胞裂解物进行的分析说明了caspase-2激活的动力学。结果表明,融合荧光蛋白的使用极大地促进了CE的分离和分析物的鉴定。将CE的细胞集落结果与光学成像获得的单细胞结果进行了比较。 (c)2006 Elsevier B.V.保留所有权利。

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