Elevated furin levels in human cystic fibrosis cells result in hypersusceptibility to exotoxin A–induced cytotoxicity
Wojciech Ornatowski, Jens F. Poschet, Elizabeth Perkett, Jennifer L. Taylor-Cousar, Vojo Deretic
Wojciech Ornatowski, Jens F. Poschet, Elizabeth Perkett, Jennifer L. Taylor-Cousar, Vojo Deretic
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Research Article Cell biology

Elevated furin levels in human cystic fibrosis cells result in hypersusceptibility to exotoxin A–induced cytotoxicity

Abstract

Progressive pulmonary disease and infections with Pseudomonas aeruginosa remain an intractable problem in cystic fibrosis (CF). At the cellular level, CF is characterized by organellar hyperacidification, which results in altered protein and lipid glycosylation. Altered pH of the trans-Golgi network (TGN) may further disrupt the protein processing and packaging that occurs in this organelle. Here we measured activity of the major TGN endoprotease furin and demonstrated a marked upregulation in human CF cells. Increased furin activity was linked to elevated production in CF of the immunosuppressive and tissue remodeling cytokine TGF-β and its downstream effects, including macrophage deactivation and augmented collagen secretion by epithelial cells. As furin is responsible for the proteolytic processing of a range of endogenous and exogenous substrates including growth factors and bacterial toxins, we determined that elevated furin-dependent activation of exotoxin A caused increased cell death in CF respiratory epithelial cells compared with genetically matched CF transmembrane conductance regulator–corrected cells. Thus elevated furin levels in CF respiratory epithelial cells contributes to bacterial toxin–induced cell death, fibrosis, and local immunosuppression. These data suggest that the use of furin inhibitors may represent a strategy for pharmacotherapy in CF.

Authors

Wojciech Ornatowski, Jens F. Poschet, Elizabeth Perkett, Jennifer L. Taylor-Cousar, Vojo Deretic

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Figure 6

Furin-dependent processing of ExoA is increased in CF cells.

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Furin-dependent processing of ExoA is increased in CF cells. (A) Localiz...
(A) Localization of ExoA in CFTR mutant IB3-1 cells by fluorescence microscopy (insets, close apposition). Cells were transfected with GFP-furin or cellubrevin-pHluorin GFP and incubated with ExoA conjugated to secondary Alexa Fluor 568 (red). EEA1 was visualized using primary human anti-EEA1 antibody and Alexa Fluor 468–conjugated antibody (green). Scale bars: 5 μm; 2 μm (insets). (B) SDS-PAGE analysis of ExoA processing in IB3-1 (CFTR mutant) cells, IB3-1 cells incubated with CMK (50 μM), and S9 (CFTR-corrected IB3-1) cells. Proteins in cell extracts were separated by SDS-PAGE and immunoblotted with anti-ExoA. ExoA66, full size, inactive ExoA toxin precursor; ExoA37, proteolytically processed 37-kDa active ExoA fragment. (C) Densitometry analysis of ExoA66/ExoA37 ratio.