Acute Exercise Modulates BDNF and pro-BDNF Protein Content in Immune Cells

G protein-coupled receptors (GPCRs) transduce physiological and sensory stimuli into appropriate cellular responses and mediate the actions of one-third of drugs. GPCR structural studies have revealed the general bases of receptor activation, signalling, drug action and allosteric modulation, but so far cover only 13% of non-olfactory receptors. We broadly surveyed the receptor modifications/engineering and methods used to produce all available GPCR crystal and cryo-EM structures and present an interactive resource integrated in GPCRdb (www.gpcrdb.org) to assist users in designing constructs and browsing appropriate experimental conditions for structure studies.

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Distinct G protein-coupled receptor phosphorylation motifs modulate arrestin affinity and activation and global conformation

Mayer

Damberger

Samarasimhareddy

et al. 2019

Nat Commun

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Cellular functions of arrestins are determined in part by the pattern of phosphorylation on the G protein-coupled receptors (GPCRs) to which arrestins bind. Despite high-resolution structural data of arrestins bound to phosphorylated receptor C-termini, the functional role of each phosphorylation site remains obscure. Here, we employ a library of synthetic phosphopeptide analogues of the GPCR rhodopsin C-terminus and determine the ability of these peptides to bind and activate arrestins using a variety of biochemical and biophysical methods. We further characterize how these peptides modulate the conformation of arrestin-1 by nuclear magnetic resonance (NMR). Our results indicate different functional classes of phosphorylation sites: ‘key sites’ required for arrestin binding and activation, an ‘inhibitory site’ that abrogates arrestin binding, and ‘modulator sites’ that influence the global conformation of arrestin. These functional motifs allow a better understanding of how different GPCR phosphorylation patterns might control how arrestin functions in the cell.

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Crystal structure of jumping spider rhodopsin-1 as a light sensitive GPCR

Varma

Mutt

Mühle

et al. 2019

Proc. Natl. Acad. Sci. U.S.A.

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Light-sensitive G protein-coupled receptors (GPCRs)—rhodopsins—absorb photons to isomerize their covalently bound retinal, triggering conformational changes that result in downstream signaling cascades. Monostable rhodopsins release retinal upon isomerization as opposed to the retinal in bistable rhodopsins that “reisomerize” upon absorption of a second photon. Understanding the mechanistic differences between these light-sensitive GPCRs has been hindered by the scarcity of recombinant models of the latter. Here, we reveal the high-resolution crystal structure of a recombinant bistable rhodopsin, jumping spider rhodopsin-1, bound to the inverse agonist 9-cis retinal. We observe a water-mediated network around the ligand hinting toward the basis of their bistable nature. In contrast to bovine rhodopsin (monostable), the transmembrane bundle of jumping spider rhodopsin-1 as well that of the bistable squid rhodopsin adopts a more “activation-ready” conformation often observed in other nonphotosensitive class A GPCRs. These similarities suggest the role of jumping spider rhodopsin-1 as a potential model system in the study of the structure–function relationship of both photosensitive and nonphotosensitive class A GPCRs.

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Genome sequencing of herb Tulsi (Ocimum tenuiflorum) unravels key genes behind its strong medicinal properties

et al. 2015

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BackgroundKrishna Tulsi, a member of Lamiaceae family, is a herb well known for its spiritual, religious and medicinal importance in India. The common name of this plant is ‘Tulsi’ (or ‘Tulasi’ or ‘Thulasi’) and is considered sacred by Hindus. We present the draft genome of Ocimum tenuiflurum L (subtype Krishna Tulsi) in this report. The paired-end and mate-pair sequence libraries were generated for the whole genome sequenced with the Illumina Hiseq 1000, resulting in an assembled genome of 374 Mb, with a genome coverage of 61 % (612 Mb estimated genome size). We have also studied transcriptomes (RNA-Seq) of two subtypes of O. tenuiflorum, Krishna and Rama Tulsi and report the relative expression of genes in both the varieties.ResultsThe pathways leading to the production of medicinally-important specialized metabolites have been studied in detail, in relation to similar pathways in Arabidopsis thaliana and other plants. Expression levels of anthocyanin biosynthesis-related genes in leaf samples of Krishna Tulsi were observed to be relatively high, explaining the purple colouration of Krishna Tulsi leaves. The expression of six important genes identified from genome data were validated by performing q-RT-PCR in different tissues of five different species, which shows the high extent of urosolic acid-producing genes in young leaves of the Rama subtype. In addition, the presence of eugenol and ursolic acid, implied as potential drugs in the cure of many diseases including cancer was confirmed using mass spectrometry.ConclusionsThe availability of the whole genome of O.tenuiflorum and our sequence analysis suggests that small amino acid changes at the functional sites of genes involved in metabolite synthesis pathways confer special medicinal properties to this herb.Electronic supplementary materialThe online version of this article (doi:10.1186/s12870-015-0562-x) contains supplementary material, which is available to authorized users.

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The counterion–retinylidene Schiff base interaction of an invertebrate rhodopsin rearranges upon light activation

et al. 2019

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Animals sense light using photosensitive proteins—rhodopsins—containing a chromophore—retinal—that intrinsically absorbs in the ultraviolet. Visible light-sensitivity depends primarily on protonation of the retinylidene Schiff base (SB), which requires a negatively-charged amino acid residue—counterion—for stabilization. Little is known about how the most common counterion among varied rhodopsins, Glu181, functions. Here, we demonstrate that in a spider visual rhodopsin, orthologue of mammal melanopsins relevant to circadian rhythms, the Glu181 counterion functions likely by forming a hydrogen-bonding network, where Ser186 is a key mediator of the Glu181–SB interaction. We also suggest that upon light activation, the Glu181–SB interaction rearranges while Ser186 changes its contribution. This is in contrast to how the counterion of vertebrate visual rhodopsins, Glu113, functions, which forms a salt bridge with the SB. Our results shed light on the molecular mechanisms of visible light-sensitivity relevant to invertebrate vision and vertebrate non-visual photoreception.

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The transcriptome enables the identification of candidate genes behind medicinal value of Drumstick tree (Moringa oleifera)

et al. 2020

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Conservation of gene architecture and domains amidst sequence divergence in the hsrω lncRNA gene across the Drosophila genus: an in silico analysis

Sahu

Mutt

Lakhotia

2020

J Genet

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Convergent evolution of tertiary structure in rhodopsin visual proteins from vertebrates and box jellyfish

Gerrard

Mutt

Nagata

et al. 2018

Proc. Natl. Acad. Sci. U.S.A.

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SignificanceComplex photoreceptors have independently evolved in animals with radial and bilateral symmetry, but little is known about the proteins that transduce light information (opsins) in radially symmetrical animals. We use homology modeling and heterologous action spectroscopy to study the structure of an opsin (JellyOp) from the lens eye of the visually competent box jellyfish, Carybdea rastonii. We find that a key structural feature of animal opsins—the counterion—maintains visible-light sensitivity in JellyOp from a unique location, E94 in the transmembrane bundle. This unique position for the counterion, the third only discovered in animal opsins, closely mirrors the location in vertebrate visual proteins, which was thought to be a unique adaptation in vertebrates to achieve higher fidelity photoreception.

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Eshita Mutt

An online resource for GPCR structure determination and analysis

Distinct G protein-coupled receptor phosphorylation motifs modulate arrestin affinity and activation and global conformation

Crystal structure of jumping spider rhodopsin-1 as a light sensitive GPCR

Genome sequencing of herb Tulsi (Ocimum tenuiflorum) unravels key genes behind its strong medicinal properties

The counterion–retinylidene Schiff base interaction of an invertebrate rhodopsin rearranges upon light activation

The transcriptome enables the identification of candidate genes behind medicinal value of Drumstick tree (Moringa oleifera)

Conservation of gene architecture and domains amidst sequence divergence in the hsrω lncRNA gene across the Drosophila genus: an in silico analysis

Convergent evolution of tertiary structure in rhodopsin visual proteins from vertebrates and box jellyfish

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