Lipid Bilayer Induces Contraction of the Denatured State Ensemble of a Helical-Bundle Membrane Protein

Defining the denatured state ensemble (DSE) and intrinsically disordered proteins is essential to understanding protein folding, chaperone action, degradation, translocation and cell signaling. While a majority of studies have focused on water-soluble proteins, the DSE of membrane proteins is much less characterized. Here, we reconstituted the DSE of a helical bundle membrane protein GlpG of Escherichia coli in native lipid bilayers and measured its conformation and compactness. The DSE was obtained using steric trapping, which couples spontaneous denaturation of a doubly biotinylated GlpG to binding of two bulky monovalent streptavidin molecules. Using limited proteolysis and mass spectrometry, we mapped the flexible regions in the DSE. Using our paramagnetic biotin derivative and double electron-electron resonance spectroscopy, we determined the dimensions of the DSE. Finally, we employed our Upside model for molecular dynamics simulations to generate the DSE including the collapsed and fully expanded states in a bilayer. We find that the DSE is highly dynamic involving the topology changes of transmembrane segments and their unfolding. The DSE is expanded relative to the native state, but only to 55-90% of the fully expanded condition. The degree of expansion depends on the chemical potential with regards to local packing and the lipid composition. Our result suggests that the native lipid bilayer promotes the association of helices in the DSE of membrane proteins and, probably in general, facilitating interhelical interactions. This tendency may be the outcome of a general lipophobic effect of proteins within the cell membranes.

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Lipid bilayer induces contraction of the denatured state ensemble of a helical-bundle membrane protein

Proceedings of the National Academy of Sciences ◽

10.1073/pnas.2109169119 ◽

2021 ◽

Vol 119 (1) ◽

pp. e2109169119

Author(s):

Kristen A. Gaffney ◽

Ruiqiong Guo ◽

Michael D. Bridges ◽

Shaima Muhammednazaar ◽

Daoyang Chen ◽

...

Keyword(s):

Membrane Protein ◽

Lipid Bilayer ◽

Lipid Bilayers ◽

Limited Proteolysis ◽

Water Soluble ◽

Disordered Proteins ◽

Resonance Spectroscopy ◽

Denatured State ◽

E Coli ◽

State Ensemble

Defining the denatured state ensemble (DSE) and disordered proteins is essential to understanding folding, chaperone action, degradation, and translocation. As compared with water-soluble proteins, the DSE of membrane proteins is much less characterized. Here, we measure the DSE of the helical membrane protein GlpG of Escherichia coli (E. coli) in native-like lipid bilayers. The DSE was obtained using our steric trapping method, which couples denaturation of doubly biotinylated GlpG to binding of two streptavidin molecules. The helices and loops are probed using limited proteolysis and mass spectrometry, while the dimensions are determined using our paramagnetic biotin derivative and double electron–electron resonance spectroscopy. These data, along with our Upside simulations, identify the DSE as being highly dynamic, involving the topology changes and unfolding of some of the transmembrane (TM) helices. The DSE is expanded relative to the native state but only to 15 to 75% of the fully expanded condition. The degree of expansion depends on the local protein packing and the lipid composition. E. coli’s lipid bilayer promotes the association of TM helices in the DSE and, probably in general, facilitates interhelical interactions. This tendency may be the outcome of a general lipophobic effect of proteins within the cell membranes.

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Quantitation and topography of membrane proteins in highly water-permeable vesicles from ADH-stimulated toad bladder

AJP Cell Physiology ◽

10.1152/ajpcell.1991.261.1.c143 ◽

1991 ◽

Vol 261 (1) ◽

pp. C143-C153 ◽

Cited By ~ 10

Author(s):

H. W. Harris ◽

M. L. Zeidel ◽

C. Hosselet

Keyword(s):

Membrane Proteins ◽

Membrane Protein ◽

Lipid Bilayer ◽

Apical Membrane ◽

Water Channel ◽

Protein S ◽

Water Channels ◽

Toad Bladder ◽

Western Blots ◽

Vesicle Protein

Antidiuretic hormone (ADH) stimulation of toad bladder granular cells rapidly increases the osmotic water permeability (Pf) of their apical membranes by insertion of highly selective water channels. Before ADH stimulation, these water channels are stored in large cytoplasmic vesicles called aggrephores. ADH causes aggrephores to fuse with the apical membrane. Termination of ADH stimulation results in prompt endocytosis of water channel-containing membranes via retrieval of these specialized regions of apical membrane. Protein components of the ADH water channel contained within these retrieved vesicles would be expected to be integral membrane protein(s) that span the vesicle's lipid bilayer to create narrow aqueous channels. Our previous work has identified proteins of 55 (actually a 55/53-kDa doublet), 17, 15, and 7 kDa as candidate ADH water channel components. We now have investigated these candidate ADH water channel proteins in purified retrieved vesicles. These vesicles do not contain a functional proton pump as assayed by Western blots of purified vesicle protein probed with anti-H(+)-ATPase antisera. Approximately 60% of vesicle protein is accounted for by three protein bands of 55, 53, and 46 kDa. Smaller contributions to vesicle protein are made by the 17- and 15-kDa proteins. Triton X-114-partitioning analysis shows that the 55, 53, 46, and 17 kDa are integral membrane proteins. Vectorial labeling analysis with two membrane-impermeant reagents shows that the 55-, 53-, and 46-kDa protein species span the lipid bilayer of these vesicles. Thus the 55-, 53-, and 46-kDa proteins possess characteristics expected for ADH water channel components. These data show that the 55- and 53- and perhaps the 46-, 17-, and 15-kDa proteins are likely components of aqueous transmembrane pores that constitute ADH water channels contained within these vesicles.

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YidC Occupies the Lateral Gate of the SecYEG Translocon and Is Sequentially Displaced by a Nascent Membrane Protein

Journal of Biological Chemistry ◽

10.1074/jbc.m112.446583 ◽

2013 ◽

Vol 288 (23) ◽

pp. 16295-16307 ◽

Cited By ~ 63

Author(s):

Ilie Sachelaru ◽

Narcis Adrian Petriman ◽

Renuka Kudva ◽

Patrick Kuhn ◽

Thomas Welte ◽

...

Keyword(s):

Membrane Proteins ◽

Membrane Protein ◽

Lipid Bilayer ◽

Transmembrane Domains ◽

Cross Linking ◽

Lipid Phase ◽

Lipid Transfer ◽

Lateral Gate

Most membrane proteins are co-translationally inserted into the lipid bilayer via the universally conserved SecY complex and they access the lipid phase presumably via a lateral gate in SecY. In bacteria, the lipid transfer of membrane proteins from the SecY channel is assisted by the SecY-associated protein YidC, but details on the SecY-YidC interaction are unknown. By employing an in vivo and in vitro site-directed cross-linking approach, we have mapped the SecY-YidC interface and found YidC in contact with all four transmembrane domains of the lateral gate. This interaction did not require the SecDFYajC complex and was not influenced by SecA binding to SecY. In contrast, ribosomes dissociated the YidC contacts to lateral gate helices 2b and 8. The major contact between YidC and the lateral gate was lost in the presence of ribosome nascent chains and new SecY-YidC contacts appeared. These data demonstrate that the SecY-YidC interaction is influenced by nascent-membrane-induced lateral gate movements.

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Exploring intrinsically disordered proteins using site-directed spin labeling electron paramagnetic resonance spectroscopy

Frontiers in Molecular Biosciences ◽

10.3389/fmolb.2015.00021 ◽

2015 ◽

Vol 2 ◽

Cited By ~ 23

Author(s):

Nolwenn Le Breton ◽

MarlÃ¨ne Martinho ◽

Elisabetta Mileo ◽

Emilien Etienne ◽

Guillaume Gerbaud ◽

...

Keyword(s):

Electron Paramagnetic Resonance ◽

Intrinsically Disordered Proteins ◽

Electron Paramagnetic Resonance Spectroscopy ◽

Spin Labeling ◽

Disordered Proteins ◽

Resonance Spectroscopy ◽

Paramagnetic Resonance ◽

Intrinsically Disordered ◽

Site Directed Spin Labeling ◽

Electron Paramagnetic

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The Peptidisc, a simple method for stabilizing membrane proteins in detergent-free solution

eLife ◽

10.7554/elife.34085 ◽

2018 ◽

Vol 7 ◽

Cited By ~ 39

Author(s):

Michael Luke Carlson ◽

John William Young ◽

Zhiyu Zhao ◽

Lucien Fabre ◽

Daniel Jun ◽

...

Keyword(s):

Membrane Proteins ◽

Membrane Protein ◽

Cost Effective ◽

Water Soluble ◽

Protein Assemblies ◽

Simple Method ◽

Helical Peptide ◽

Biological Studies ◽

Multiple Copies ◽

Exposed Part

Membrane proteins are difficult to work with due to their insolubility in aqueous solution and quite often their poor stability in detergent micelles. Here, we present the peptidisc for their facile capture into water-soluble particles. Unlike the nanodisc, which requires scaffold proteins of different lengths and precise amounts of matching lipids, reconstitution of detergent solubilized proteins in peptidisc only requires a short amphipathic bi-helical peptide (NSPr) and no extra lipids. Multiple copies of the peptide wrap around to shield the membrane-exposed part of the target protein. We demonstrate the effectiveness of this ‘one size fits all’ method using five different membrane protein assemblies (MalFGK2, FhuA, SecYEG, OmpF, BRC) during ‘on-column’, ‘in-gel’, and ‘on-bead’ reconstitution embedded within the membrane protein purification protocol. The peptidisc method is rapid and cost-effective, and it may emerge as a universal tool for high-throughput stabilization of membrane proteins to advance modern biological studies.

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Membrane protein-based biosensors

Journal of The Royal Society Interface ◽

10.1098/rsif.2017.0952 ◽

2018 ◽

Vol 15 (141) ◽

pp. 20170952 ◽

Cited By ~ 24

Author(s):

Nobuo Misawa ◽

Toshihisa Osaki ◽

Shoji Takeuchi

Keyword(s):

Membrane Proteins ◽

Membrane Protein ◽

Lipid Bilayer ◽

Recent Progress ◽

Biological Membranes ◽

Cultured Cell ◽

Sensor Device ◽

Fundamental Information ◽

Essential Components ◽

Target Molecules

This review highlights recent development of biosensors that use the functions of membrane proteins. Membrane proteins are essential components of biological membranes and have a central role in detection of various environmental stimuli such as olfaction and gustation. A number of studies have attempted for development of biosensors using the sensing property of these membrane proteins. Their specificity to target molecules is particularly attractive as it is significantly superior to that of traditional human-made sensors. In this review, we classified the membrane protein-based biosensors into two platforms: the lipid bilayer-based platform and the cell-based platform. On lipid bilayer platforms, the membrane proteins are embedded in a lipid bilayer that bridges between the protein and a sensor device. On cell-based platforms, the membrane proteins are expressed in a cultured cell, which is then integrated in a sensor device. For both platforms we introduce the fundamental information and the recent progress in the development of the biosensors, and remark on the outlook for practical biosensing applications.

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The molecular mechanism of nuclear transport revealed by atomic-scale measurements

eLife ◽

10.7554/elife.10027 ◽

2015 ◽

Vol 4 ◽

Cited By ~ 76

Author(s):

Loren E Hough ◽

Kaushik Dutta ◽

Samuel Sparks ◽

Deniz B Temel ◽

Alia Kamal ◽

...

Keyword(s):

Intrinsically Disordered Proteins ◽

Atomic Scale ◽

Disordered Proteins ◽

Nuclear Pore ◽

Resonance Spectroscopy ◽

Nuclear Pore Complexes ◽

Selective Filter ◽

Intrinsically Disordered ◽

Cellular Environment ◽

Pore Complexes

Nuclear pore complexes (NPCs) form a selective filter that allows the rapid passage of transport factors (TFs) and their cargoes across the nuclear envelope, while blocking the passage of other macromolecules. Intrinsically disordered proteins (IDPs) containing phenylalanyl-glycyl (FG)-rich repeats line the pore and interact with TFs. However, the reason that transport can be both fast and specific remains undetermined, through lack of atomic-scale information on the behavior of FGs and their interaction with TFs. We used nuclear magnetic resonance spectroscopy to address these issues. We show that FG repeats are highly dynamic IDPs, stabilized by the cellular environment. Fast transport of TFs is supported because the rapid motion of FG motifs allows them to exchange on and off TFs extremely quickly through transient interactions. Because TFs uniquely carry multiple pockets for FG repeats, only they can form the many frequent interactions needed for specific passage between FG repeats to cross the NPC.

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Structure and dynamics conspire in the evolution of affinity between intrinsically disordered proteins

Science Advances ◽

10.1126/sciadv.aau4130 ◽

2018 ◽

Vol 4 (10) ◽

pp. eaau4130 ◽

Cited By ~ 14

Author(s):

Per Jemth ◽

Elin Karlsson ◽

Beat Vögeli ◽

Brenda Guzovsky ◽

Eva Andersson ◽

...

Keyword(s):

Protein Interaction ◽

Protein Interactions ◽

Intrinsically Disordered Proteins ◽

Disordered Proteins ◽

Solvent Accessible Surface Area ◽

Resonance Spectroscopy ◽

Protein Protein Interactions ◽

Structural Dynamic ◽

Intrinsically Disordered ◽

Structure And Dynamics

In every established species, protein-protein interactions have evolved such that they are fit for purpose. However, the molecular details of the evolution of new protein-protein interactions are poorly understood. We have used nuclear magnetic resonance spectroscopy to investigate the changes in structure and dynamics during the evolution of a protein-protein interaction involving the intrinsically disordered CREBBP (CREB-binding protein) interaction domain (CID) and nuclear coactivator binding domain (NCBD) from the transcriptional coregulators NCOA (nuclear receptor coactivator) and CREBBP/p300, respectively. The most ancient low-affinity “Cambrian-like” [540 to 600 million years (Ma) ago] CID/NCBD complex contained less secondary structure and was more dynamic than the complexes from an evolutionarily younger “Ordovician-Silurian” fish ancestor (ca. 440 Ma ago) and extant human. The most ancient Cambrian-like CID/NCBD complex lacked one helix and several interdomain interactions, resulting in a larger solvent-accessible surface area. Furthermore, the most ancient complex had a high degree of millisecond-to-microsecond dynamics distributed along the entire sequences of both CID and NCBD. These motions were reduced in the Ordovician-Silurian CID/NCBD complex and further redistributed in the extant human CID/NCBD complex. Isothermal calorimetry experiments show that complex formation is enthalpically favorable and that affinity is modulated by a largely unfavorable entropic contribution to binding. Our data demonstrate how changes in structure and motion conspire to shape affinity during the evolution of a protein-protein complex and provide direct evidence for the role of structural, dynamic, and frustrational plasticity in the evolution of interactions between intrinsically disordered proteins.

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Dynamical Oligomerisation of Histidine Rich Intrinsically Disordered Proteins Is Regulated through Zinc-Histidine Interactions

Biomolecules ◽

10.3390/biom9050168 ◽

2019 ◽

Vol 9 (5) ◽

pp. 168 ◽

Cited By ~ 6

Author(s):

Carolina Cragnell ◽

Lasse Staby ◽

Samuel Lenton ◽

Birthe Kragelund ◽

Marie Skepö

Keyword(s):

Nuclear Magnetic Resonance ◽

Intrinsically Disordered Proteins ◽

Divalent Cations ◽

Disordered Proteins ◽

Resonance Spectroscopy ◽

Binding Motifs ◽

Histatin 5 ◽

X Ray ◽

Intrinsically Disordered ◽

X Ray Scattering

Intrinsically disordered proteins (IDPs) can form functional oligomers and in some cases, insoluble disease related aggregates. It is therefore vital to understand processes and mechanisms that control pathway distribution. Divalent cations including Zn2+ can initiate IDP oligomerisation through the interaction with histidine residues but the mechanisms of doing so are far from understood. Here we apply a multi-disciplinary approach using small angle X-ray scattering, nuclear magnetic resonance spectroscopy, calorimetry and computations to show that that saliva protein Histatin 5 forms highly dynamic oligomers in the presence of Zn2+. The process is critically dependent upon interaction between Zn2+ ions and distinct histidine rich binding motifs which allows for thermodynamic switching between states. We propose a molecular mechanism of oligomerisation, which may be generally applicable to other histidine rich IDPs. Finally, as Histatin 5 is an important saliva component, we suggest that Zn2+ induced oligomerisation may be crucial for maintaining saliva homeostasis.

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