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A refined atomic scale model of the Saccharomyces cerevisiae K+-translocation protein Trk1p combined with experimental evidence confirms the role of selectivity filter glycines and other key residues. | LitMetric

A refined atomic scale model of the Saccharomyces cerevisiae K+-translocation protein Trk1p combined with experimental evidence confirms the role of selectivity filter glycines and other key residues.

Biochim Biophys Acta

Institute of Nanobiology and Structural Biology, Global Change Research Center, Academy of Sciences of the Czech Republic, Nove Hrady, Czech Republic; Molecular Bioenergetics, Institute of Cellular and Molecular Botany, University of Bonn, Bonn, Germany. Electronic address:

Published: May 2015

AI Article Synopsis

  • Potassium ion (K+) uptake in yeast is primarily facilitated by the Trk1/2 transport proteins, which allow survival in low external K+ concentrations.
  • A refined structural model of Trk1 was developed using advanced techniques such as homology modeling, molecular dynamics, and functional analysis to understand its properties and functions better.
  • Key residues like aspartic acid (D79) and lysine (K1147) were found to play crucial roles in the protein’s folding and function, with potential implications for ion transport mechanisms in Trk1.

Article Abstract

Potassium ion (K+) uptake in yeast is mediated mainly by the Trk1/2 proteins that enable cells to survive on external K+ concentration as low as a few μM. Fungal Trks are related to prokaryotic TRK and Ktr and plant HKT K+ transport systems. Overall sequence similarity is very low, thus requiring experimental verification of homology models. Here a refined structural model of the Saccharomyces cerevisiae Trk1 is presented that was obtained by combining homology modeling, molecular dynamics simulation and experimental verification through functional analysis of mutants. Structural models and experimental results showed that glycines within the selectivity filter, conserved among the K-channel/transporter family, are not only important for protein function, but are also required for correct folding/membrane targeting. A conserved aspartic acid in the PA helix (D79) and a lysine in the M2D helix (K1147) were proposed earlier to interact. Our results suggested individual roles of these residues in folding, structural integrity and function. While mutations of D79 completely abolished protein folding, mutations at position 1147 were tolerated to some extent. Intriguingly, a secondary interaction of D79 with R76 could enhance folding/stability of Trk1 and enable a fraction of Trk1[K1147A] to fold. The part of the ion permeation path containing the selectivity filter is shaped similar to that of ion channels. However below the selectivity filter it is obstructed or regulated by a proline containing loop. The presented model could provide the structural basis for addressing the long standing question if Trk1 is a passive or active ion-translocation system.

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Source
http://dx.doi.org/10.1016/j.bbamem.2015.02.007DOI Listing

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