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Supramolecular zippers elicit interbilayer adhesion of membranes producing cell death
Authors:Víctor G. Almendro-Vedia  Carolina García  Rubén Ahijado-Guzmán  Diego de la Fuente-Herreruela  Mónica Muñoz-Úbeda  Paolo Natale  Montserrat H. Viñas  Rodrigo Queiroz Albuquerque  Andrés Guerrero-Martínez  Francisco Monroy  M. Pilar Lillo  Iván López-Montero
Affiliation:1. Dto. Química Física, Universidad Complutense de Madrid, Avenida Complutense s/n, 28040 Madrid, Spain;2. Instituto de Investigación Hospital Doce de Octubre (i+12), Avenida de Córdoba s/n, 28041 Madrid, Spain;3. Dto. Química Física Biológica, Instituto de Química-Física “Rocasolano” (CSIC), Serrano 119, 28006 Madrid, Spain.;4. ETS de Sistemas Informáticos, Universidad Politécnica de Madrid, Alan Turing s/n, 28031 Madrid, Spain;5. School of Pharmacy and Biomolecular Sciences, Liverpool John Moores University, L3 3AF Liverpool, United Kingdom;6. São Carlos Institute of Chemistry, University of São Paulo (USP), 13566-590 São Carlos, Brazil
Abstract:

Background

The fluorescent dye 10-N-nonyl acridine orange (NAO) is widely used as a mitochondrial marker. NAO was reported to have cytotoxic effects in cultured eukaryotic cells when incubated at high concentrations. Although the biochemical response of NAO-induced toxicity has been well identified, the underlying molecular mechanism has not yet been explored in detail.

Methods

We use optical techniques, including fluorescence confocal microscopy and lifetime imaging microscopy (FLIM) both in model membranes built up as giant unilamellar vesicles (GUVs) and cultured cells. These experiments are complemented with computational studies to unravel the molecular mechanism that makes NAO cytotoxic.

Results

We have obtained direct evidence that NAO promotes strong membrane adhesion of negatively charged vesicles. The attractive forces are derived from van der Waals interactions between anti-parallel H-dimers of NAO molecules from opposing bilayers. Semi-empirical calculations have confirmed the supramolecular scenario by which anti-parallel NAO molecules form a zipper of bonds at the contact region. The membrane remodeling effect of NAO, as well as the formation of H-dimers, was also confirmed in cultured fibroblasts, as shown by the ultrastructure alteration of the mitochondrial cristae.

Conclusions

We conclude that membrane adhesion induced by NAO stacking accounts for the supramolecular basis of its cytotoxicity.

General significance

Mitochondria are a potential target for cancer and gene therapies. The alteration of the mitochondrial structure by membrane remodeling agents able to form supramolecular assemblies via adhesion properties could be envisaged as a new therapeutic strategy.
Keywords:Fibroblasts  Mitochondria  Giant vesicles  H-aggregate  NAO  2P-FLIM  two-photon fluorescence-lifetime imaging microscopy  AO  acridine orange  ATP  adenosine triphosphate  CL  cardiolipin  DFT  density functional theory  DMEM  Dulbecco Modified Eagle Medium  adh  adhesion strength  GP  generalized polarization  GUV  giant unillamelar vesicle  IMM  inner mitochondrial membrane  ITO  indium tin oxide  LUV  large unilamellar vesicle  KCl  potassium chloride  MEF  mouse embryonic fibroblasts  NAO  PE  phosphatidylethnolamine  POPC  PLE  polar lipid extract  POPG  SA  stearic acid  TD-DFT  time-dependent DFT  bending rigidity  surface tension
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