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Fluorogenic Chemical Probes for Wash-free Imaging of Cell Membrane Damage in Ferroptosis, Necrosis, and Axon Injury

化学 体内 细胞 DNA损伤 膜透性 荧光显微镜 细胞膜 生物物理学 细胞生物学 生物化学 荧光 DNA 量子力学 生物技术 生物 物理
作者
Philipp Mauker,Daniela Beckmann,Annabel Kitowski,Constanze Heise,Chantal Wientjens,Andrew J. Davidson,Simone Wanderoy,Gabin Fabre,Angelika B. Harbauer,Will Wood,Christoph Wilhelm,Julia Thorn‐Seshold,Thomas Misgeld,Martin Kerschensteiner,Oliver Thorn‐Seshold
出处
期刊:Journal of the American Chemical Society [American Chemical Society]
被引量:19
标识
DOI:10.1021/jacs.3c07662
摘要

Selectively labeling cells with damaged membranes is needed not only for identifying dead cells in culture, but also for imaging membrane barrier dysfunction in pathologies in vivo. Most membrane permeability stains are permanently colored or fluorescent dyes that need washing to remove their non-uptaken extracellular background and reach good image contrast. Others are DNA-binding environment-dependent fluorophores, which lack design modularity, have potential toxicity, and can only detect permeabilization of cell volumes containing a nucleus (i.e., cannot delineate damaged volumes in vivo nor image non-nucleated cell types or compartments). Here, we develop modular fluorogenic probes that reveal the whole cytosolic volume of damaged cells, with near-zero background fluorescence so that no washing is needed. We identify a specific disulfonated fluorogenic probe type that only enters cells with damaged membranes, then is enzymatically activated and marks them. The esterase probe MDG1 is a reliable tool to reveal live cells that have been permeabilized by biological, biochemical, or physical membrane damage, and it can be used in multicolor microscopy. We confirm the modularity of this approach by also adapting it for improved hydrolytic stability, as the redox probe MDG2. We conclude by showing the unique performance of MDG probes in revealing axonal membrane damage (which DNA fluorogens cannot achieve) and in discriminating damage on a cell-by-cell basis in embryos in vivo. The MDG design thus provides powerful modular tools for wash-free in vivo imaging of membrane damage, and indicates how designs may be adapted for selective delivery of drug cargoes to these damaged cells: offering an outlook from selective diagnosis toward therapy of membrane-compromised cells in disease.
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