Bridging the gap between structure and kinetics of human SGLT1

The Na+-glucose cotransporter hSGLT1 is a member of a class of membrane proteins that harness Na+ electrochemical gradients to drive uphill solute transport. Although hSGLT1 belongs to one gene family (SLC5), recent structural studies of bacterial Na+ cotransporters have shown that Na+ transporters in different gene families have the same structural fold. We have constructed homology models of hSGLT1 in two conformations, the inward-facing occluded (based on vSGLT) and the outward open conformations (based on Mhp1), mutated in turn each of the conserved gates and ligand binding residues, expressed the SGLT1 mutants in Xenopus oocytes, and determined the functional consequences using biophysical and biochemical assays. The results establish that mutating the ligand binding residues produces profound changes in the ligand affinity (the half-saturation concentration, K0.5); e.g., mutating sugar binding residues increases the glucose K0.5 by up to three orders of magnitude. Mutation of the external gate residues increases the Na+ to sugar transport stoichiometry, demonstrating that these residues are critical for efficient cotransport. The changes in phlorizin inhibition constant ( Ki) are proportional to the changes in sugar K0.5, except in the case of F101C, where phlorizin Ki increases by orders of magnitude without a change in glucose K0.5. We conclude that glucose and phlorizin occupy the same binding site and that F101 is involved in binding to the phloretin group of the inhibitor. Substituted-cysteine accessibility methods show that the cysteine residues at the position of the gates and sugar binding site are largely accessible only to external hydrophilic methanethiosulfonate reagents in the presence of external Na+, demonstrating that the external sugar (and phlorizin) binding vestibule is opened by the presence of external Na+ and closes after the binding of sugar and phlorizin. Overall, the present results provide a bridge between kinetics and structural studies of cotransporters.

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Evaluation of the rate constants of sugar transport through maltoporin (LamB) of Escherichia coli from the sugar-induced current noise.

The Journal of General Physiology ◽

10.1085/jgp.105.3.385 ◽

1995 ◽

Vol 105 (3) ◽

pp. 385-401 ◽

Cited By ~ 53

Author(s):

C Andersen ◽

M Jordy ◽

R Benz

Keyword(s):

Escherichia Coli ◽

Binding Site ◽

Outer Membrane ◽

Rate Constants ◽

Sugar Transport ◽

Current Noise ◽

Induced Current ◽

Lipid Bilayer Membranes ◽

Sugar Binding ◽

Different Temperatures

LamB (maltoporin) of Escherichia coli outer membrane was reconstituted into artificial lipid bilayer membranes. The channel contains a binding site for sugars and is blocked for ions when the site is occupied by a sugar. The on and off reactions of sugar binding cause an increase of the noise of the current through the channel. The sugar-induced current noise of maltoporin was used for the evaluation of the sugar-binding kinetics for different sugars of the maltooligosaccharide series and for sucrose. The on rate constant for sugar binding was between 10(6) and 10(7) M-1.s-1 for the maltooligosaccharides and corresponds to the movement of the sugars from the aqueous phase to the central binding site. The off rate (corresponding to the release of the sugars from the channel) decreased with increasing number of glucose residues in the maltooligosaccharides from approximately 2,000 s-1 for maltotriose to 180 s-1 for maltoheptaose. The kinetics for sucrose movement was considerably slower. The activation energies of the stability constant and of the rate constants for sugar binding were evaluated from noise experiments at different temperatures. The role of LamB in the transport of maltooligosaccharides across the outer membrane is discussed.

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Functional Consequences of Natural Substitutions in the GluR6 Kainate Receptor Subunit Ligand-Binding Site

Channels ◽

10.4161/chan.1.6.5589 ◽

2007 ◽

Vol 1 (6) ◽

pp. 417-428 ◽

Cited By ~ 3

Author(s):

Tara M. Kistler ◽

Mark W. Fleck

Keyword(s):

Ligand Binding ◽

Binding Site ◽

Kainate Receptor ◽

Receptor Subunit ◽

Ligand Binding Site ◽

Functional Consequences

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The ligand binding site of the neurokinin 2 receptor. Site-directed mutagenesis and identification of neurokinin A binding residues in the human neurokinin 2 receptor.

Journal of Biological Chemistry ◽

10.1016/s0021-9258(18)46979-7 ◽

1994 ◽

Vol 269 (44) ◽

pp. 27269-27274

Author(s):

N Bhogal ◽

D Donnelly ◽

J B Findlay

Keyword(s):

Ligand Binding ◽

Binding Site ◽

Receptor Site ◽

Site Directed Mutagenesis ◽

Directed Mutagenesis ◽

Neurokinin A ◽

Ligand Binding Site ◽

Binding Residues

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Evolution of (p)ppGpp-HPRT regulation through diversification of an allosteric oligomeric interaction

10.1101/621474 ◽

2019 ◽

Author(s):

Brent W. Anderson ◽

Kuanqing Liu ◽

Christine Wolak ◽

Katarzyna Dubiel ◽

Kenneth A. Satyshur ◽

...

Keyword(s):

Ligand Binding ◽

Binding Site ◽

Protein Interactions ◽

Binding Motif ◽

Protein Ligand Interactions ◽

Protein Interfaces ◽

Ligand Interactions ◽

Binding Residues ◽

The Common ◽

Ligand Regulation

ABSTRACTThe signaling ligand (p)ppGpp binds diverse targets across bacteria, yet the mechanistic and evolutionary basis underlying these ligand-protein interactions remains poorly understood. Here we identify a novel (p)ppGpp binding motif in the enzyme HPRT, where (p)ppGpp shares identical binding residues for PRPP and nucleobase substrates to regulate purine homeostasis. Intriguingly, HPRTs across species share the conserved binding site yet strongly differ in ligand binding, from strong inhibition by basal (p)ppGpp levels to weak regulation at induced concentrations. Surprisingly, strong ligand binding requires an HPRT dimer-dimer interaction that allosterically opens the (p)ppGpp pocket. This dimer-dimer interaction is absent in the common ancestor but evolved to favor (p)ppGpp binding in the vast majority of bacteria. We propose that the evolutionary plasticity of oligomeric interfaces enables allosteric adjustment of ligand regulation, bypassing constraints of the ligand binding site. Since most ligands bind near protein-protein interfaces, this principle likely extends to other protein-ligand interactions.

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