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Dynamic imaging of protease activity with fluorescently quenched activity-based probes

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TLDR
The design and synthesis of a selective, cell-permeable qABP is reported, used to monitor real-time protease activity in live human cells with fluorescence microscopy techniques as well as standard biochemical methods.
Abstract
Protease activity is tightly regulated in both normal and disease conditions. However, it is often difficult to monitor the dynamic nature of this regulation in the context of a live cell or whole organism. To address this limitation, we developed a series of quenched activity-based probes (qABPs) that become fluorescent upon activity-dependent covalent modification of a protease target. These reagents freely penetrate cells and allow direct imaging of protease activity in living cells. Targeted proteases are directly identified and monitored biochemically by virtue of the resulting covalent tag, thereby allowing unambiguous assignment of protease activities observed in imaging studies. We report here the design and synthesis of a selective, cell-permeable qABP for the study of papain-family cysteine proteases. This probe is used to monitor real-time protease activity in live human cells with fluorescence microscopy techniques as well as standard biochemical methods.

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Citations
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Targeting proteases: successes, failures and future prospects.

TL;DR: The status of human protease research and prospects for future protease-targeted drugs are reviewed, with reference to some key examples where protease drugs have succeeded or failed.
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Cysteine cathepsins: From structure, function and regulation to new frontiers

TL;DR: The view of cysteine cathepsins as lysosomal proteases is changing as there is now clear evidence of their localization in other cellular compartments, and some of the remarkable advances that have taken place in the past decade are presented.
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Extracellular matrix dynamics in development and regenerative medicine.

TL;DR: Stem cell self-renewal and differentiation is influenced by the 3D environment within the stem cell niche, and the intimate dynamic relationship between cells and the ECM must be understood to ensure appropriate cell behavior.
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Fluorescence imaging in vivo: recent advances.

TL;DR: In vivo fluorescence imaging uses a sensitive camera to detect fluorescence emission from fluorophores in whole-body living small animals and the list of NIR probes continues to grow with the recent addition of fluorescent organic, inorganic and biological nanoparticles.
References
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Morphogenesis and oncogenesis of MCF-10A mammary epithelial acini grown in three-dimensional basement membrane cultures

TL;DR: A collection of protocols to culture MCF-10A cells, to establish stable pools expressing a gene of interest via retroviral infection, as well as to grow and analyzeMCF- 10A cells in three-dimensional basement membrane culture are provided.
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Activity-based protein profiling: The serine hydrolases

TL;DR: The chemical synthesis and utility of an active-site directed probe for visualizing dynamics in the expression and function of an entire enzyme family, the serine hydrolases, is described and it is shown that FP-biotin labels these proteins in an activity-dependent manner that can be followed kinetically.
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Irreversible inhibitors of serine, cysteine, and threonine proteases.

TL;DR: This paper presents a meta-review of the literature on Vinyl Sulfones, Michael Acceptors, and Heterocyclic Inhibitors dating back to the 1970s, which revealed a wide diversity of opinions about the properties of these substances and their role in the human immune system.
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Human and mouse proteases: a comparative genomic approach

TL;DR: The availability of the human and mouse genome sequences has allowed the identification and comparison of their respective degradomes — the complete repertoire of proteases that are produced by these organisms.
Journal ArticleDOI

Building epithelial architecture: insights from three-dimensional culture models

TL;DR: It is proposed that the morphogenetic behaviour of epithelial cells is guided by two distinct elements: an intrinsic differentiation programme that drives formation of a lumen-enclosing monolayer, and a growth factor-induced, transient de-differentiation that allows this monolayers to be remodelled.
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