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胶原固定化的细胞外 FRET 报告分子用于可视化活细胞分泌的蛋白酶活性。

Collagen-Immobilized Extracellular FRET Reporter for Visualizing Protease Activity Secreted by Living Cells.

机构信息

Department of Life Science, BK21 Plus Bio-Defense Research Team, Hanyang University, Seoul 04763, Republic of Korea.

Department of Bioengineering, BK21 Plus Future Biopharmaceutical Human Resources Training and Research Team, Hanyang University, Seoul 04763, Republic of Korea.

出版信息

ACS Sens. 2020 Mar 27;5(3):655-664. doi: 10.1021/acssensors.9b01456. Epub 2020 Feb 21.

Abstract

Despite the diverse roles of cell-secreted proteases in the extracellular matrix (ECM), classical methods to analyze protease activity have not been explored at the cell culture site. Here, we report a stable, matrix-sticky, and protease-sensitive extracellular reporter that comprises a collagen-binding protein and a Förster resonance energy transfer (FRET) coupler of an enhanced green fluorescent protein and a small dye molecule. The extracellular FRET reporter via split intein-mediated protein trans-splicing is able to adhere to collagen matrices, leading to fluorescence changes by matrix metalloproteinase-2 (MMP2) activity during living cell culture without impeding cell viability. When a proMMP2 mutant (Y581A) with altered protease secretion and activity was transfected into cancer cells, the reporter revealed a dramatic reduction in MMP2 activity in both two- and three-dimensional culture systems, compared with cells transfected with wild-type proMMP2. Our reporter is immediately amenable to monitor protease activity in diverse ECM-resident cells as well as to study protease-related extracellular signaling and tissue remodeling.

摘要

尽管细胞分泌的蛋白酶在细胞外基质 (ECM) 中发挥着多种作用,但经典的蛋白酶活性分析方法尚未在细胞培养部位得到探索。在这里,我们报告了一种稳定的、基质粘性的、蛋白酶敏感的细胞外报告器,它由胶原结合蛋白和荧光蛋白和小染料分子的Förster 共振能量转移 (FRET) 偶联物组成。通过分裂 intein 介导的蛋白质转剪接的细胞外 FRET 报告器能够附着到胶原基质上,在活细胞培养过程中,通过基质金属蛋白酶-2(MMP2)的活性导致荧光变化,而不影响细胞活力。当具有改变的蛋白酶分泌和活性的 proMMP2 突变体 (Y581A) 转染到癌细胞中时,与转染野生型 proMMP2 的细胞相比,报告器显示出在二维和三维培养系统中 MMP2 活性的显著降低。我们的报告器可以立即用于监测多种 ECM 驻留细胞中的蛋白酶活性,以及研究与蛋白酶相关的细胞外信号和组织重塑。

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