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Spontaneous oligomerization of BAK/BAX is suppressed by hetero-dimerization with MCL-1

biorxiv. 2019; 
?Basile I. M.?Wicky,?Kallol?Gupta,?Tristan O. C.?Kwan,?Carol V.?Robinson,Jane?Clarke
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Codon Optimization Coding DNA sequences for human BAK, BAX and MCL-1 were ordered from Genscript (codon-optimized for?Escherichia coli), and sub-cloned into expression vectors by scarless insertion using the In-Fusion kit (Takara). Cysteine residues were mutated to serines to avoid the use of reducing agents. MCL-1 (UniProt:Q07820, residues 168–327, C286S) was sub-cloned into a modified version of the pRSET A vector containing a N-terminal hexahistidine-tag followed by a thrombin cleavage site. The disordered N-terminus, and the C-terminal transmembrane regions were excluded, in line with literature reports.? Get A Quote

摘要

BCL-2 proteins control the intrinsic pathway of programmed cell death. Composed of anti- and pro-apoptotic members, their network of interactions forms a molecular switch that controls mitochondrial outer-membrane permeability. Apoptotic stimulation leads to BAK/BAX oligomerization and pore formation, yet the molecular details of this pivotal step remain poorly understood, and controversy persists regarding the activation mechanism. Here we use native mass spectrometry and kinetics to show that the homo-oligomerization of BAK and BAX is spontaneous in hydrophobic environments. This process is abrogated by hetero-dimerization of both BAK and BAX with the anti-apoptotic BCL-2 protein MCL-1. Pro-apoptotic BH3-only... More

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