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Peptide-Mediated Liposome Fusion as a Tool for the Detection of Matrix Metalloproteinases

机译:Peptide-Mediated脂质体融合的工具检测基质金属蛋白酶

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摘要

Biological cells continue to inspire the development of technologies toward rapid, sensitive, and selective detection of analytes. Membrane fusion is a key biological event in living cells that involves a highly selective recognition mechanism controlled by different functional proteins. Herein, liposome-liposome fusion mediated by coiled-coil forming peptides JR2EC and JR2KC to mimic biological membrane fusion is reported. The liposome fusion event is monitored through fluorescence generation and this mechanism forms the basis of a detection assay for matrix metalloproteinases (MMPs), which are key homeostatic proteases. Using this approach, a limit of detection of 0.35 |j,g mL-1 MMP-7 in biological samples is obtained, and this assay does not require washing, separation, or amplification steps. The developed tool could be extended for the detection of other proteolytic enzymes of the MMP family (diagnostic or prognostic markers) and has the potential for screening of peptide libraries against a target of interest.
机译:生物细胞继续激励技术的发展迅速,敏感,分析物的选择性检测。膜融合是一个关键的生物事件活细胞,包括一个高度选择性识别由不同的控制机制功能性蛋白质。融合由卷曲螺旋形成肽JR2EC和JR2KC模拟生物膜融合报道。通过荧光生成和监控这种机制的基础形式检测试验对基质金属蛋白酶(MMPs)关键是自我平衡的蛋白酶。方法检测极限0.35 | j, g mL-1MMP-7生物样品中获得,这试验不需要洗涤、分离或放大的步骤。延长其他蛋白水解的检测(诊断或酶的MMP的家庭预后标记)和潜力肽库筛选与目标感兴趣的。

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