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Literature DB >> 23603221

Atomic force microscopy: a multifaceted tool to study membrane proteins and their interactions with ligands.

Abstract

Membrane proteins are embedded in lipid bilayers and facilitate the communication between the external environment and the interior of the cell. This communication is often mediated by the binding of ligands to the membrane protein. Understanding the nature of the interaction between a ligand and a membrane protein is required to both understand the mechanism of action of these proteins and for the development of novel pharmacological drugs. The highly hydrophobic nature of membrane proteins and the requirement of a lipid bilayer for native function have hampered the structural and molecular characterizations of these proteins under physiologically relevant conditions. Atomic force microscopy offers a solution to studying membrane proteins and their interactions with ligands under physiologically relevant conditions and can provide novel insights about the nature of these critical molecular interactions that facilitate cellular communication. In this review, we provide an overview of the atomic force microscopy technique and discuss its application in the study of a variety of questions related to the interaction between a membrane protein and a ligand. This article is part of a Special Issue entitled: Structural and biophysical characterization of membrane protein-ligand binding.

Entities: CellLine Chemical Disease Gene Mutation Species

Keywords: AFM; DFS; Energy landscape; Force spectroscopy; F–D; G protein-coupled receptor; GPCR; HOPG; ICAM-1; Imaging; LFA-1; LHRH; Molecular interaction; PE40; Protein structure; Pseudomonas aeruginosa exotoxin 40; SMFS; STM; atomic force microscopy; dynamic single-molecule force spectroscopy; force–distance; highly ordered pyrolytic graphite; intercellular adhesion molecule-1; leukocyte function-associated antigen-1; luteinizing hormone-releasing hormone; scanning tunneling microscopy; single-molecule force spectroscopy

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Year: 2013 PMID： 23603221 PMCID： PMC3779510 DOI： 10.1016/j.bbamem.2013.04.011

Source DB: PubMed Journal: Biochim Biophys Acta ISSN： 0006-3002

122 in total

Review 1. Imaging and manipulation of biological structures with the AFM.

Authors: Dimitrios Fotiadis; Simon Scheuring; Shirley A Müller; Andreas Engel; Daniel J Müller
Journal: Micron Date: 2002 Impact factor: 2.251

2. The unfolding kinetics of ubiquitin captured with single-molecule force-clamp techniques.

Authors: Michael Schlierf; Hongbin Li; Julio M Fernandez
Journal: Proc Natl Acad Sci U S A Date: 2004-04-27 Impact factor: 11.205

3. Dual energy landscape: the functional state of the β-barrel outer membrane protein G molds its unfolding energy landscape.

Authors: Mehdi Damaghi; K Tanuj Sapra; Stefan Köster; Özkan Yildiz; Werner Kühlbrandt; Daniel J Muller
Journal: Proteomics Date: 2010-12 Impact factor: 3.984

4. Theory, analysis, and interpretation of single-molecule force spectroscopy experiments.

Authors: Olga K Dudko; Gerhard Hummer; Attila Szabo
Journal: Proc Natl Acad Sci U S A Date: 2008-10-13 Impact factor: 11.205

5. Automated setpoint adjustment for biological contact mode atomic force microscopy imaging.

Authors: Ignacio Casuso; Simon Scheuring
Journal: Nanotechnology Date: 2010-01-22 Impact factor: 3.874

6. Voltage and pH-induced channel closure of porin OmpF visualized by atomic force microscopy.

Authors: D J Müller; A Engel
Journal: J Mol Biol Date: 1999-01-29 Impact factor: 5.469

Review 7. High-speed atomic force microscopy: Structure and dynamics of single proteins.

Authors: Ignacio Casuso; Felix Rico; Simon Scheuring
Journal: Curr Opin Chem Biol Date: 2011-05-31 Impact factor: 8.822

8. Substrate specificity of sugar transport by rabbit SGLT1: single-molecule atomic force microscopy versus transport studies.

Authors: Theeraporn Puntheeranurak; Barbara Wimmer; Francisco Castaneda; Hermann J Gruber; Peter Hinterdorfer; Rolf K H Kinne
Journal: Biochemistry Date: 2007-02-16 Impact factor: 3.162

9. Ligand-specific interactions modulate kinetic, energetic, and mechanical properties of the human β2 adrenergic receptor.

Authors: Michael Zocher; Juan J Fung; Brian K Kobilka; Daniel J Müller
Journal: Structure Date: 2012-06-28 Impact factor: 5.006

10. Interaction between pheromone and its receptor of the fission yeast Schizosaccharomyces pombe examined by a force spectroscopy study.

Authors: Shintaro Sasuga; Ryohei Abe; Osamu Nikaido; Shoichi Kiyosaki; Hiroshi Sekiguchi; Atsushi Ikai; Toshiya Osada
Journal: J Biomed Biotechnol Date: 2012-02-21

27 in total

Atomic force microscopy: a multifaceted tool to study membrane proteins and their interactions with ligands.

Review 1. Imaging and manipulation of biological structures with the AFM.

2. The unfolding kinetics of ubiquitin captured with single-molecule force-clamp techniques.

3. Dual energy landscape: the functional state of the β-barrel outer membrane protein G molds its unfolding energy landscape.

4. Theory, analysis, and interpretation of single-molecule force spectroscopy experiments.

5. Automated setpoint adjustment for biological contact mode atomic force microscopy imaging.

6. Voltage and pH-induced channel closure of porin OmpF visualized by atomic force microscopy.

Review 7. High-speed atomic force microscopy: Structure and dynamics of single proteins.

8. Substrate specificity of sugar transport by rabbit SGLT1: single-molecule atomic force microscopy versus transport studies.

9. Ligand-specific interactions modulate kinetic, energetic, and mechanical properties of the human β2 adrenergic receptor.

10. Interaction between pheromone and its receptor of the fission yeast Schizosaccharomyces pombe examined by a force spectroscopy study.

1. Switching behaviour in vascular smooth muscle cell-matrix adhesion during oscillatory loading.

2. Effect of dietary docosahexaenoic acid on rhodopsin content and packing in photoreceptor cell membranes.

Review 3. Nanoscale monitoring of drug actions on cell membrane using atomic force microscopy.

Review 4. Insights into the multifaceted application of microscopic techniques in plant tissue culture systems.

Review 5. Transient Receptor Potential Channels and Calcium Signaling.

Review 6. Rhodopsin Oligomerization and Aggregation.

7. Differentiating between Inactive and Active States of Rhodopsin by Atomic Force Microscopy in Native Membranes.

8. Dynamic single-molecule force spectroscopy of rhodopsin in native membranes.

9. Impact of reduced rhodopsin expression on the structure of rod outer segment disc membranes.

10. Peptidases and peptidase inhibitors in gut of caterpillars and in the latex of their host plants.