5,724 research outputs found
Identification of Histamine H3 Receptor Ligands Using a New Crystal Structure Fragment-based Method
GPCRdb:an information system for G protein-coupled receptors
Recent developments in G protein-coupled receptor (GPCR) structural biology and pharmacology have greatly enhanced our knowledge of receptor structure-function relations, and have helped improve the scientific foundation for drug design studies. The GPCR database, GPCRdb, serves a dual role in disseminating and enabling new scientific developments by providing reference data, analysis tools and interactive diagrams. This paper highlights new features in the fifth major GPCRdb release: (i) GPCR crystal structure browsing, superposition and display of ligand interactions; (ii) direct deposition by users of point mutations and their effects on ligand binding; (iii) refined snake and helix box residue diagram looks; and (iii) phylogenetic trees with receptor classification colour schemes. Under the hood, the entire GPCRdb front- and back-ends have been re-coded within one infrastructure, ensuring a smooth browsing experience and development. GPCRdb is available at http://www.gpcrdb.org/ and it's open source code at https://bitbucket.org/gpcr/protwis
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The Promises and Pitfalls of Genoeconomics
This article reviews existing research at the intersection of genetics and economics, presents some new findings that illustrate the state of genoeconomics research, and surveys the prospects of this emerging field. Twin studies suggest that economic outcomes and preferences, once corrected for measurement error, appear to be about as heritable as many medical conditions and personality traits. Consistent with this pattern, we present new evidence on the heritability of permanent income and wealth. Turning to genetic association studies, we survey the main ways that the direct measurement of genetic variation across individuals is likely to contribute to economics, and we outline the challenges that have slowed progress in making these contributions. The most urgent problem facing researchers in this field is that most existing efforts to find associations between genetic variation and economic behavior are based on samples that are too small to ensure adequate statistical power. This has led to many false positives in the literature. We suggest a number of possible strategies to improve and remedy this problem: (a) pooling data sets, (b) using statistical techniques that exploit the greater information content of many genes jointly, and (c) focusing on economically relevant traits that are most proximate to known biological mechanisms.EconomicsSociolog
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Most Reported Genetic Associations with General Intelligence Are Probably False Positives
General intelligence (g) and virtually all other behavioral traits are heritable. Associations between g and specific single-nucleotide polymorphisms (SNPs) in several candidate genes involved in brain function have been reported. We sought to replicate published associations between g and 12 specific genetic variants (in the genes DTNBP1, CTSD, DRD2, ANKK1, CHRM2, SSADH, COMT, BDNF, CHRNA4, DISC1, APOE, and SNAP25) using data sets from three independent, well-characterized longitudinal studies with samples of 5,571, 1,759, and 2,441 individuals. Of 32 independent tests across all three data sets, only 1 was nominally significant. By contrast, power analyses showed that we should have expected 10 to 15 significant associations, given reasonable assumptions for genotype effect sizes. For positive controls, we confirmed accepted genetic associations for Alzheimerâs disease and body mass index, and we used SNP-based calculations of genetic relatedness to replicate previous estimates that about half of the variance in g is accounted for by common genetic variation among individuals. We conclude that the molecular genetics of psychology and social science requires approaches that go beyond the examination of candidate genes.Economic
Receptor selectivity between the G proteins GÎą12 and GÎą13 is defined by a single leucine-to-isoleucine variation
Despite recent advances in structural definition of GPCRâG protein complexes, the basis of receptor selectivity between G proteins remains unclear. The GÎą12 and GÎą13 subtypes together form the least studied group of heterotrimeric G proteins. G proteinâcoupled receptor 35 (GPR35) has been suggested to couple efficiently to GÎą13 but weakly to GÎą12. Using combinations of cells genome-edited to not express G proteins and bioluminescence resonance energy transferâbased sensors, we confirmed marked selectivity of GPR35 for GÎą13. Incorporating GÎą12/GÎą13 chimeras and individual residue swap mutations into these sensors defined that selectivity between GÎą13 and GÎą12 was imbued largely by a single leucine-to-isoleucine variation at position G.H5.23. Indeed, leucine could not be substituted by other amino acids in GÎą13 without almost complete loss of GPR35 coupling. The critical importance of leucine at G.H5.23 for GPR35âG protein interaction was further demonstrated by introduction of this leucine into GÎąq, resulting in the gain of coupling to GPR35. These studies demonstrate that GÎą13 is markedly the most effective G protein for interaction with GPR35 and that selection between GÎą13 and GÎą12 is dictated largely by a single conservative amino acid variation.âMackenzie, A. E., Quon, T., Lin, L.-C., Hauser, A. S., Jenkins, L., Inoue, A., Tobin, A. B., Gloriam, D. E., Hudson, B. D., Milligan, G. Receptor selectivity between the G proteins GÎą12 and GÎą13 is defined by a single leucine-to-isoleucine variation
The orphan G protein-coupled receptor GPR139 is activated by the peptides:Adrenocorticotropic hormone (ACTH), ι-, and β-melanocyte stimulating hormone (ι-MSH, and β-MSH), and the conserved core motif HFRW
GPR139 is an orphan G protein-coupled receptor that is expressed primarily in the brain. Not much is known regarding the function of GPR139. Recently we have shown that GPR139 is activated by the amino acids l-tryptophan and l-phenylalanine (EC(50) values of 220 ΟM and 320 ΟM, respectively), as well as di-peptides comprised of aromatic amino acids. This led us to hypothesize that GPR139 may be activated by peptides. Sequence alignment of the binding cavities of all class A GPCRs, revealed that the binding pocket of the melanocortin 4 receptor is similar to that of GPR139. Based on the chemogenomics principle âsimilar targets bind similar ligandsâ, we tested three known endogenous melanocortin 4 receptor agonists; adrenocorticotropic hormone (ACTH) and Îą- and β-melanocyte stimulating hormone (Îą-MSH and β-MSH) on CHO-k1 cells stably expressing the human GPR139 in a Fluo-4 Ca(2+)-assay. All three peptides, as well as their conserved core motif HFRW, were found to activate GPR139 in the low micromolar range. Moreover, we found that peptides consisting of nine or ten N-terminal residues of Îą-MSH activate GPR139 in the submicromolar range. Îą-MSH(1-9) was found to correspond to the product of a predicted cleavage site in the pre-pro-protein pro-opiomelanocortin (POMC). Our results demonstrate that GPR139 is a peptide receptor, activated by ACTH, Îą-MSH, β-MSH, the conserved core motif HFRW as well as a potential endogenous peptide Îą-MSH(1-9). Further studies are needed to determine the functional relevance of GPR139 mediated signaling by these peptides
A New Era in Extragalactic Background Light Measurements: The Cosmic History of Accretion, Nucleosynthesis and Reionization
(Brief Summary) What is the total radiative content of the Universe since the
epoch of recombination? The extragalactic background light (EBL) spectrum
captures the redshifted energy released from the first stellar objects,
protogalaxies, and galaxies throughout cosmic history. Yet, we have not
determined the brightness of the extragalactic sky from UV/optical to
far-infrared wavelengths with sufficient accuracy to establish the radiative
content of the Universe to better than an order of magnitude. Among many
science topics, an accurate measurement of the EBL spectrum from optical to
far-IR wavelengths, will address: What is the total energy released by stellar
nucleosynthesis over cosmic history? Was significant energy released by
non-stellar processes? Is there a diffuse component to the EBL anywhere from
optical to sub-millimeter? When did first stars appear and how luminous was the
reionization epoch? Absolute optical to mid-IR EBL spectrum to an
astrophysically interesting accuracy can be established by wide field imagingat
a distance of 5 AU or above the ecliptic plane where the zodiacal foreground is
reduced by more than two orders of magnitude.Comment: 7 pages; Science White Paper for the US Astro 2010-2020 Decadal
Survey. If interested in further community-wide efforts on this topic please
contact the first autho
Type VI Secretion System in Pseudomonas aeruginosa: Secretion and Multimerization of VgrG Proteins
Pseudomonas aeruginosa is a Gram-negative bacterium causing chronic infections in cystic fibrosis patients. Such infections are associated with an active type VI secretion system (T6SS), which consists of about 15 conserved components, including the AAA+ ATPase, ClpV. The T6SS secretes two categories of proteins, VgrG and Hcp. Hcp is structurally similar to a phage tail tube component, whereas VgrG proteins show similarity to the puncturing device at the tip of the phage tube. In P. aeruginosa, three T6SSs are known. The expression of H1-T6SS genes is controlled by the RetS sensor. Here, 10 vgrG genes were identified in the PAO1 genome, among which three are co-regulated with H1-T6SS, namely vgrG1a/b/c. Whereas VgrG1a and VgrG1c were secreted in a ClpV1-dependent manner, secretion of VgrG1b was ClpV1-independent. We show that VgrG1a and VgrG1c form multimers, which confirmed the VgrG model predicting trimers similar to the tail spike. We demonstrate that Hcp1 secretion requires either VgrG1a or VgrG1c, which may act independently to puncture the bacterial envelope and give Hcp1 access to the surface. VgrG1b is not required for Hcp1 secretion. Thus, VgrG1b does not require H1-T6SS for secretion nor does H1-T6SS require VgrG1b for its function. Finally, we show that VgrG proteins are required for secretion of a genuine H1-T6SS substrate, Tse3. Our results demonstrate that VgrG proteins are not only secreted components but are essential for secretion of other T6SS substrates. Overall, we emphasize variability in behavior of three P. aeruginosa VgrGs, suggesting that, although very similar, distinct VgrGs achieve specific functions
Search for the standard model Higgs boson in the H to ZZ to 2l 2nu channel in pp collisions at sqrt(s) = 7 TeV
A search for the standard model Higgs boson in the H to ZZ to 2l 2nu decay
channel, where l = e or mu, in pp collisions at a center-of-mass energy of 7
TeV is presented. The data were collected at the LHC, with the CMS detector,
and correspond to an integrated luminosity of 4.6 inverse femtobarns. No
significant excess is observed above the background expectation, and upper
limits are set on the Higgs boson production cross section. The presence of the
standard model Higgs boson with a mass in the 270-440 GeV range is excluded at
95% confidence level.Comment: Submitted to JHE
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