# Structural and functional mapping of ion access pathways in the human K+-dependent Na+/Ca2+ exchanger NCKX2 using cysteine scanning mutagenesis, thiol-modifying reagents, and homology modelling

**Authors:** Robert T. Szerencsei, Shitian Cai, Hristina R. Zhekova, Ali H. Jalloul, D. Peter Tieleman, Paul P.M. Schnetkamp

PMC · DOI: 10.1080/19336950.2025.2513268 · Channels · 2025-06-09

## TL;DR

This study identifies key pathways for ion transport in the NCKX2 protein using mutagenesis and modeling, revealing residues critical for cation binding and transport.

## Contribution

A comprehensive structural and functional map of ion access pathways in NCKX2 is provided through cysteine scanning and homology modeling.

## Key findings

- 35 out of 146 cysteine substitutions significantly affected Ca2+ transport activity upon MTSET treatment.
- Extracellular residues were sensitive to modification, while intracellular residues were inhibited by MTSEA.
- MD simulations confirmed water-accessible pathways, aligning with experimental results.

## Abstract

K+-dependent Na+/Ca2+ exchanger proteins (NCKX) are members of the CaCA superfamily with critical roles in vision, skin pigmentation, enamel formation, and neuronal functions. Despite their importance, the structural pathways governing cation transport remain unclear. To address this, we conducted a systematic study using cysteine scanning mutagenesis of human NCKX2 combined with the thiol-modifying reagents MTSET and MTSEA to probe the accessibility and functional significance of specific residues. We used homology models of outward-facing and inward-facing NCKX2 states and molecular dynamics (MD) simulations to compare and investigate residue accessibility in human NCKX2 based on the published structures of the archaeal NCK_Mj Na+/Ca2+ exchanger and the human NCX1 Na+/Ca2+ exchanger. Mutant NCKX2 proteins expressed in HEK293 cells revealed diverse effects of MTSET and MTSEA on Ca2+ transport. Of the 146 cysteine substitutions analyzed, 35 exhibited significant changes in Ca2+ transport activity upon treatment with MTSET, with 16 showing near-complete inhibition and six demonstrating increased activity. Residues within the cation binding sites and extracellular access channels were sensitive to modification, consistent with their critical role in ion transport, whereas intracellular residues showed minimal accessibility to MTSET but were inhibited by membrane-permeable MTSEA. Water accessibility maps from MD simulations corroborated these findings, providing a high-resolution view of water-accessible pathways. This study provides a comprehensive structural and functional map of NCKX2 ion access pathways, offering insights into the molecular basis of ion selectivity and transport. These findings highlight the key residues critical for cation binding and transport, advancing our understanding of the structural dynamics of NCKX2.

## Linked entities

- **Proteins:** SLC24A2 (solute carrier family 24 member 2), SLC8A1 (solute carrier family 8 member A1)
- **Chemicals:** MTSET (PubChem CID 107933), MTSEA (PubChem CID 53443082)
- **Species:** Homo sapiens (taxon 9606)

## Full-text entities

- **Genes:** SLC8A1 (solute carrier family 8 member A1) [NCBI Gene 6546] {aka NCX1}, SLC24A1 (solute carrier family 24 member 1) [NCBI Gene 9187] {aka CSNB1D, HsT17412, NCKX, NCKX1, RODX}, CRYGD (crystallin gamma D) [NCBI Gene 1421] {aka CACA, CCA3, CCP, CRYG4, CTRCT4, PCC}, SLC24A2 (solute carrier family 24 member 2) [NCBI Gene 25769] {aka NCKX2}
- **Chemicals:** K (MESH:D011188), thiol (MESH:D013438), Water (MESH:D014867), MTSET (-), cysteine (MESH:D003545), Na (MESH:D012964), MTSEA (MESH:C093171), Ca (MESH:D002118)
- **Species:** Homo sapiens (human, species) [taxon 9606]
- **Cell lines:** HEK293 — Homo sapiens (Human), Transformed cell line (CVCL_0045)

## Full text

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## Figures

16 figures with captions in the complete paper: https://tomesphere.com/paper/PMC12150658/full.md

## References

34 references — full list in the complete paper: https://tomesphere.com/paper/PMC12150658/full.md

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Source: https://tomesphere.com/paper/PMC12150658