Literature DB >> 34916296

Symmetric activation and modulation of the human calcium-sensing receptor.

Jinseo Park1, Hao Zuo1, Aurel Frangaj1, Ziao Fu2, Laura Y Yen3, Zhening Zhang2, Lidia Mosyak1, Vesna N Slavkovich4, Jonathan Liu1, Kimberly M Ray1, Baohua Cao1, Francesca Vallese5,6, Yong Geng1, Shaoxia Chen7, Robert Grassucci2, Venkata P Dandey3, Yong Zi Tan3,8,9,10, Edward Eng3, Yeji Lee1, Brian Kloss11, Zheng Liu2, Wayne A Hendrickson12,8,11, Clinton S Potter2,3, Bridget Carragher2,3, Joseph Graziano4, Arthur D Conigrave13, Joachim Frank12,14, Oliver B Clarke15,6,8, Qing R Fan16,17.   

Abstract

The human extracellular calcium-sensing (CaS) receptor controls plasma Ca2+ levels and contributes to nutrient-dependent maintenance and metabolism of diverse organs. Allosteric modulation of the CaS receptor corrects disorders of calcium homeostasis. Here, we report the cryogenic-electron microscopy reconstructions of a near-full-length CaS receptor in the absence and presence of allosteric modulators. Activation of the homodimeric CaS receptor requires a break in the transmembrane 6 (TM6) helix of each subunit, which facilitates the formation of a TM6-mediated homodimer interface and expansion of homodimer interactions. This transformation in TM6 occurs without a positive allosteric modulator. Two modulators with opposite functional roles bind to overlapping sites within the transmembrane domain through common interactions, acting to stabilize distinct rotamer conformations of key residues on the TM6 helix. The positive modulator reinforces TM6 distortion and maximizes subunit contact to enhance receptor activity, while the negative modulator strengthens an intact TM6 to dampen receptor function. In both active and inactive states, the receptor displays symmetrical transmembrane conformations that are consistent with its homodimeric assembly.

Entities:  

Keywords:  activation mechanism; allosteric modulation; calcium-sensing receptor; cryo-EM structure; symmetry

Mesh:

Substances:

Year:  2021        PMID: 34916296      PMCID: PMC8713963          DOI: 10.1073/pnas.2115849118

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   12.779


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