Chaperone BiP controls ER stress sensor Ire1 through interactions with its oligomers

Author:

Dawes Sam12,Hurst Nicholas1ORCID,Grey Gabriel1,Wieteska Lukasz1,Wright Nathan V1,Manfield Iain W1ORCID,Hussain Mohammed H1ORCID,Kalverda Arnout P1,Lewandowski Jozef R3ORCID,Chen Beining2,Zhuravleva Anastasia1ORCID

Affiliation:

1. School of Molecular and Cellular Biology, Faculty of Biological Sciences & Astbury Centre for Structural Molecular Biology, University of Leeds

2. Chemistry Department, University of Sheffield, Sheffield, UK

3. Department of Chemistry, University of Warwick, Coventry, UK

Abstract

The complex multistep activation cascade of Ire1 involves changes in the Ire1 conformation and oligomeric state. Ire1 activation enhances ER folding capacity, in part by overexpressing the ER Hsp70 molecular chaperone BiP; in turn, BiP provides tight negative control of Ire1 activation. This study demonstrates that BiP regulates Ire1 activation through a direct interaction with Ire1 oligomers. Particularly, we demonstrated that the binding of Ire1 luminal domain (LD) to unfolded protein substrates not only trigger conformational changes in Ire1-LD that favour the formation of Ire1-LD oligomers but also exposes BiP binding motifs, enabling the molecular chaperone BiP to directly bind to Ire1-LD in an ATP-dependent manner. These transient interactions between BiP and two short motifs in the disordered region of Ire1-LD are reminiscent of interactions between clathrin and another Hsp70, cytoplasmic Hsc70. BiP binding to substrate-bound Ire1-LD oligomers enables unfolded protein substrates and BiP to synergistically and dynamically control Ire1-LD oligomerisation, helping to return Ire1 to its deactivated state when an ER stress response is no longer required.

Funder

UKRI | Biotechnology and Biological Sciences Research Council

Publisher

Life Science Alliance, LLC

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