Conformational Dynamics of Activation for the Pentameric Complex of Dimeric G Protein-Coupled Receptor and Heterotrimeric G Protein

Orban, Tivadar; Jastrzębska, Beata; Gupta, Sayan; Wang, Benlian; Miyagi, Masaru; Chance, Mark R.; Palczewski, Krzysztof

doi:10.1016/j.str.2012.03.017

Cited by 63 publications

(107 citation statements)

References 74 publications

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“…These peptides were each reproduced by several hundred independent digestions of apo and various ligand-bound ␤ 2 AR from multiple batches of purifications (Ref (6) and unpublished data). The DDM solution also successfully reproduced high coverage for other GPCRs in other laboratories (76). However, devised for direct HDX, DLT did not address extensive PTMs and Cys, as they did not pose a problem in the ␤ 2 AR crystallizable construct: All PTM-bearing domains were either genetically truncated (intracellular C-terminal tail and loop 3) or deglycosylated (two adjacent extracellulardomain N-glycosylations) in purification (6).…”

Section: Direct Flow/ddm-facilitated Digestions For Hdx Deep Sequencmentioning

confidence: 97%

Less is More: Membrane Protein Digestion Beyond Urea–Trypsin Solution for Next-level Proteomics

Zhang

2015

Molecular & Cellular Proteomics

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Section: Direct Flow/ddm-facilitated Digestions For Hdx Deep Sequencmentioning

confidence: 97%

Less is More: Membrane Protein Digestion Beyond Urea–Trypsin Solution for Next-level Proteomics

Zhang

2015

Molecular & Cellular Proteomics

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“…The specific structural rearrangements that occur following activation by the tethered ligand and how cofactors and heterodimers influence the receptor allostery are remaining questions that will require alternative techniques such as structural mass spectrometry. 115,116 Targeting PARs for therapies A primary goal of structural studies is to gain insights on the mechanisms by which receptors operate at the molecular level and how they interact with potential therapeutics. These details can provide the tools required for rational drug design and high-throughput screening of chemical libraries that can be the basis for lead compound development.…”

Section: Protease-activated Receptors In Hemostasis 173mentioning

confidence: 99%

Protease-activated receptors in hemostasis

Nieman

2016

Blood

114

123

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Protease signaling in cells elicits multiple physiologically important responses via protease-activated receptors (PARs). There are 4 members of this family of G-protein–coupled receptors (PAR1-4). PARs are activated by proteolysis of the N terminus to reveal a tethered ligand. The rate-limiting step of PAR signaling is determined by the efficiency of proteolysis of the N terminus, which is regulated by allosteric binding sites, cofactors, membrane localization, and receptor dimerization. This ultimately controls the initiation of PAR signaling. In addition, these factors also control the cellular response by directing signaling toward G-protein or β-arrestin pathways. PAR1 signaling on endothelial cells is controlled by the activating protease and heterodimerization with PAR2 or PAR3. As a consequence, the genetic and epigenetic control of PARs and their cofactors in physiologic and pathophysiologic conditions have the potential to influence cellular behavior. Recent studies have uncovered polymorphisms that result in PAR4 sequence variants with altered reactivity that interact to influence platelet response. This further demonstrates how interactions within the plasma membrane can control the physiological output. Understanding the structural rearrangement following PAR activation and how PARs are allosterically controlled within the plasma membrane will determine how best to target this family of receptors therapeutically. The purpose of this article is to review how signaling from PARs is influenced by alternative cleavage sites and the physical interactions within the membrane. Going forward, it will be important to relate the altered signaling to the molecular arrangement of PARs in the cell membrane and to determine how these may be influenced genetically.

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“…In particular in the photo-activation processes, which are well studied in the example of mammalian rhodopsin, demonstrated the involvement of transient intermediates leading to the socalled Meta II state that is competent of G-protein binding 71 . The available X-ray crystal structures of rhodopsin and its several photo-intermediates have dramatically increased our understanding of structural rearrangements upon the activation of GPCRs.…”

Section: Xf-ms In Study Of Gpcrsmentioning

confidence: 99%

“…The local conformational changes arising from the isomerization of the covalently bound retinal appear to be propagated to the cytoplasmic surface by means of water reorganization, and rearrangement of H-bonding network between bound water and amino-acid side chains in the TM domain as demonstrated by 18 O-labeled water exchange studies 62 . Combined XF and HDX experiments included the investigation of conformation changes due to the binding of heterotrimeric G-protein 71 . Monitoring the amount of HO…”

Section: Xf-ms In Study Of Gpcrsmentioning

confidence: 99%

Oxidative footprinting in the study of structure and function of membrane proteins: current state and perspectives

Bavro

Gupta

Ralston

2015

Biochemical Society Transactions

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Abstract:Membrane proteins, such as receptors, transporters and ion channels control the vast majority of cellular signaling and metabolite exchange processes and as such are increasingly becoming the key pharmacological targets. Difficulties of handling membrane proteins in high concentrations and requirements of membrane environments for their stabilization have made them difficult to study using traditional structural biology techniques, requiring the use of a hybrid, integrative approaches to study their dynamic properties and functional aspects in physiologically relevant conditions. In recent years significant progress has been made in the field of oxidative labeling techniques, and particularly X-radiolytic labeling in combination of mass spectroscopy (XF-MS) allowing these approaches to mature and provide valuable insights into structure and function of proteins, including membrane targets, which is difficult to obtain by other techniques, complementing available structural data. XF-MS has demonstrated unique capability for identification of structural waters and conformational changes in proteins at both high degree of spatial and temporal resolution. Here we provide a perspective of the place of XF-MS amongst other structural biology methods and showcase some of latest developments in usage of XF-MS in solving water meditated transmembrane signaling, ion transport, ion gating as well as ligand induced allosteric conformation changes in these membrane protein complexes.

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Conformational Dynamics of Activation for the Pentameric Complex of Dimeric G Protein-Coupled Receptor and Heterotrimeric G Protein

Cited by 63 publications

References 74 publications

Less is More: Membrane Protein Digestion Beyond Urea–Trypsin Solution for Next-level Proteomics

Less is More: Membrane Protein Digestion Beyond Urea–Trypsin Solution for Next-level Proteomics

Protease-activated receptors in hemostasis

Oxidative footprinting in the study of structure and function of membrane proteins: current state and perspectives

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