Literature DB >> 31160463

Ratiometric two-photon microscopy reveals attomolar copper buffering in normal and Menkes mutant cells.

M Thomas Morgan1,2, Daisy Bourassa1,2, Shefali Harankhedkar1,2, Adam M McCallum1,2, Stephanie A Zlatic3, Jenifer S Calvo4, Gabriele Meloni4, Victor Faundez3, Christoph J Fahrni5,2.   

Abstract

Copper is controlled by a sophisticated network of transport and storage proteins within mammalian cells, yet its uptake and efflux occur with rapid kinetics. Present as Cu(I) within the reducing intracellular environment, the nature of this labile copper pool remains elusive. While glutathione is involved in copper homeostasis and has been assumed to buffer intracellular copper, we demonstrate with a ratiometric fluorescent indicator, crisp-17, that cytosolic Cu(I) levels are buffered to the vicinity of 1 aM, where negligible complexation by glutathione is expected. Enabled by our phosphine sulfide-stabilized phosphine (PSP) ligand design strategy, crisp-17 offers a Cu(I) dissociation constant of 8 aM, thus exceeding the binding affinities of previous synthetic Cu(I) probes by four to six orders of magnitude. Two-photon excitation microscopy with crisp-17 revealed rapid, reversible increases in intracellular Cu(I) availability upon addition of the ionophoric complex CuGTSM or the thiol-selective oxidant 2,2'-dithiodipyridine (DTDP). While the latter effect was dramatically enhanced in 3T3 cells grown in the presence of supplemental copper and in cultured Menkes mutant fibroblasts exhibiting impaired copper efflux, basal Cu(I) availability in these cells showed little difference from controls, despite large increases in total copper content. Intracellular copper is thus tightly buffered by endogenous thiol ligands with significantly higher affinity than glutathione. The dual utility of crisp-17 to detect normal intracellular buffered Cu(I) levels as well as to probe the depth of the labile copper pool in conjunction with DTDP provides a promising strategy to characterize perturbations of cellular copper homeostasis.

Entities:  

Keywords:  Menkes disease; copper homeostasis; fluorescent probes; glutathione; two-photon microscopy

Year:  2019        PMID: 31160463      PMCID: PMC6589653          DOI: 10.1073/pnas.1900172116

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  36 in total

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Review 10.  Getting out what you put in: Copper in mitochondria and its impacts on human disease.

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