4.5 Article

Intramolecular Disulfide Bonds for Biogenesis of CALHM1 Ion Channel Are Dispensable for Voltage-Dependent Activation

MOLECULES AND CELLS (2021)

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Journal

MOLECULES AND CELLS
Volume 44, Issue 10, Pages 758-769

Publisher

KOREAN SOC MOLECULAR & CELLULAR BIOLOGY
DOI: 10.14348/molcells.2021.0131

Keywords

CALHM1; disulfide bond; membrane trafficking; oligomerization; reducing agent

Categories

Biochemistry & Molecular Biology Cell Biology

Funding

  1. National Research Foundation of Korea [NRF-2018R1A5A2025964]
  2. EDISON (EDucation-research Integration through Simulation On the Net) Program [NRF-2016M3C1A6936605]
  3. Korea Health Technology R&D Project, through the Korea Health Industry Development Institute (KHIDI) - Ministry of Health & Welfare, Republic of Korea [HP20C0199]
  4. M.D., Ph.D./Medical Scientist Training Programs through KHIDI

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The study found that specific cysteine residues in the CALHM1 channel are crucial for protein biogenesis and ionic current, with disruption of these residues affecting protein expression on the membrane. Furthermore, it was highlighted that extracellular disulfide bonds play a significant role in folding, oligomerization, and trafficking of CALHM1, while being dispensable for voltage-dependent activation once on the plasma membrane.
Calcium homeostasis modulator 1 (CALHM1) is a membrane protein with four transmembrane helices that form an octameric ion channel with voltage-dependent activation. There are four conserved cysteine (Cys) residues in the extracellular domain that form two intramolecular disulfide bonds. We investigated the roles of C42-C127 and C44-C161 in human CALHM1 channel biogenesis and the ionic current (I-CALHM1). Replacing Cys with Ser or Ala abolished the membrane trafficking as well as I-CALHM1. Immunoblotting analysis revealed dithiothreitol-sensitive multimeric CALHM1, which was markedly reduced in C44S and C161S, but preserved in C42S and C127S. The mixed expression of C42S and wild-type did not show a dominant-negative effect. While the heteromeric assembly of CALHM1 and CALHM3 formed active ion channels, the co-expression of C42S and CALHM3 did not produce functional channels. Despite the critical structural role of the extracellular cysteine residues, a treatment with the membrane-impermeable reducing agent tris(2-carboxyethyl) phosphine (TCEP, 2 mM) did not affect I-CALHM1 for up to 30 min. Interestingly, incubation with TCEP (2 mM) for 2-6 h reduced both I-CALHM1 and the surface expression of CALHM1 in a time-dependent manner. We propose that the intramolecular disulfide bonds are essential for folding, oligomerization, trafficking and maintenance of CALHM1 in the plasma membrane, but dispensable for the voltage-dependent activation once expressed on the plasma membrane.

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