Abstract

Derning structural details for membrane-embedded proteins is limited by the availability of two- or three-dimensional crystals suitable for diffraction studies. This is even more difrcult when the structure of a ligand in its binding site is required because difference crystallography would be necessary, and with two-dimensional crystals, extramembraneous protein detail is often missing and resolution is low in the direction of the membrane normal. Also, many bioactive ligands do not have any structured form in solution (solvents, detergents, etc.), but it is usually accepted that their target site does have structural requirements which derne efrcacy and potency. To address the question of ligand structure for bound ligands, novel solid-state NMR techniques were used to derne molecular constraints at atomic resolution for ligands at their site of action, in fully functional, hydrated proteins under near physiological conditions (4°C or higher), and in a form often used for pharmacological and biochemical characterization. Using the solid-state NMR approach, the structure of retinal has been resolved in the bacterial proton pump, bacteriorhodopsin, and in the 7-TMD G-coupled receptor, mammalian rhodopsin, without any knowledge of the protein structure itself. The rrst structural details of a widely used drug analogue, an imidazopyridine inhibitor of the gastric H+-K+- ATPase, at its site of action, have been determined. Other examples for large integral proteins include the observation and kinetic description of solutes in the antimicrobial target sugar transporter proteins of bacteria, and the resolution of the chemistry of the binding site of acetylcholine when in the binding site of the nicotinic acetylcholine receptor. In addition, small peptide ion channels are amenable to study using solid-state NMR methods, and the state of oligomerization, residues involved in the channel, can now be derned, with the potential for describing functionally signircant residues and thus aid inhibitor or modulator design. The information gained and methods developed for small amounts of protein (μmolnmol of binding sites), open the way to derning structural details of peptide hormones, flexible drugs and other ligands bound at their site of action in a functional system. The results therefore have relevance to the in-vivo situation, and are of direct importance for the understanding of structural requirements for ligand-activated signal transduction and cellular activity. In some cases, the residues involved in binding are also being resolved, thereby giving a complete picture of the vital and highly relevant ligand-binding site structure and environment, in the absence of knowledge of the protein backbone or its structural arrangements.

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