4.6 Article

Mutations of the nACh Receptor M4 Helix Reveal Different Phenotypes in Different Expression Systems: Could Lipids be Responsible?

Journal

FRONTIERS IN PHYSIOLOGY
Volume 13, Issue -, Pages -

Publisher

FRONTIERS MEDIA SA
DOI: 10.3389/fphys.2022.850782

Keywords

Cys-loop receptor; M4; mutagenesis; aromatic interaction; nACh receptor

Categories

Funding

  1. AstraZeneca studentship
  2. MRC grant [MR/L021676/1]
  3. MRC [MR/L021676/1] Funding Source: UKRI

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The role of the M4 helix in the pLGIC family is not yet fully understood, but it is known to be involved in receptor assembly and signaling. This study compares the sensitivity of M4 in different expression systems and finds that the lipid content of the plasma membrane may explain the observed differences. Furthermore, the study shows that most of the identified nonfunctional M4 mutants are functional when expressed in oocytes, suggesting that the expression system used is important for studying the function of M4.
The role of the outermost helix (M4) in the pentameric ligand-gated ion channel (pLGIC) family is currently not fully understood. It is known that M4 is important for receptor assembly, possibly via interactions with neighboring M1 and M3 helices. M4 can also transmit information on the lipid content of the membrane to the gating mechanism, and it may form a link to the extracellular domain via the Cys-loop. Our previous study examining the alpha 4 beta 2 nACh receptor M4 helix using HEK cells indicated M4 here is more sensitive to change than those of other pLGIC. Many of these other studies, however, were performed in Xenopus oocytes. Here we examine the nine previously identified nonfunctional alpha 4 beta 2 nACh receptor M4 mutant receptors using this system. The data reveal that seven of these mutant receptors do function when expressed in oocytes, with only 2, the conserved Asp at the intracellular end of M4 and a Phe in the center, having a similar phenotype (nonfunctional) in both HEK cells and oocytes. The oocyte data are more consistent with studies in other pLGIC and demonstrate the importance of the expression system used. Of the many differences between these two expression systems, we suggest that the different lipid content of the plasma membrane is a possible candidate for explaining these discrepancies.

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