Abstract:
Bax is a pro-apoptotic Bcl-2 family member that experiences a net translocation
from the cytosol to mitochondria under cell stress. It inserts and
oligomerizes irreversibly in the mitochondrial outer membrane (MOM) to
mediate its permeabilization, leading to cytochrome c release and cell death.
Bax translocation also correlates with massive mitochondrial fragmentation.
Indeed, Bax colocalizes with the dynamin-related protein 1 (Drp1) at fission
sites during apoptosis. However, the molecular basis behind Bax function
and the nature of Bax structures responsible for MOM permeabilization
remain poorly understood.
In this thesis, we studied the nanoscale spatial organization of Bax at
mitochondria of apoptotic cells using dual-color super-resolution microscopy.
We also investigated Bax interplay with Drp1 at the single-molecule level by
fluorescence cross-correlation spectroscopy (FCCS).
We show that active Bax assembled into distinct architectures including
full rings, arcs, and lines that localized in discrete foci along mitochondria
in close association with Drp1 foci. The physiological relevance of these
structures is supported by the different organization adopted by an inactive
mutant that constitutively localizes at the MOM. Remarkably, both rings
and arc-shaped oligomeric assemblies of Bax perforated the membrane, as
revealed by atomic force microscopy in lipid bilayers.
Moreover, in vitro FCCS assays with recombinant proteins in single-vesicle
approaches threw light upon the interaction between Bax and Drp1, where
the membrane environment has an active contribution.
Our data identify the supramolecular organization of Bax during apoptosis
and support a molecular mechanism in which Bax fully or partially delineates
pores of different sizes to permeabilize the MOM. Altogether, our results
contribute to the understanding of the interplay between the mitochondrial
fission machinery and cell death regulation.
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