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10. The EH1 motif in metazoan transcription factors

Author

Copley Richard R

Subjects
Biotechnology, TP248.13-248.65, Genetics, QH426-470
Abstract

Abstract Background The Engrailed Homology 1 (EH1) motif is a small region, believed to have evolved convergently in homeobox and forkhead containing proteins, that interacts with the Drosophila protein groucho (C. elegans unc-37, Human Transducin-like Enhancers of Split). The small size of the motif makes its reliable identification by computational means difficult. I have systematically searched the predicted proteomes of Drosophila, C. elegans and human for further instances of the motif. Results Using motif identification methods and database searching techniques, I delimit which homeobox and forkhead domain containing proteins also have likely EH1 motifs. I show that despite low database search scores, there is a significant association of the motif with transcription factor function. I further show that likely EH1 motifs are found in combination with T-Box, Zinc Finger and Doublesex domains as well as discussing other plausible candidate associations. I identify strong candidate EH1 motifs in basal metazoan phyla. Conclusion Candidate EH1 motifs exist in combination with a variety of transcription factor domains, suggesting that these proteins have repressor functions. The distribution of the EH1 motif is suggestive of convergent evolution, although in many cases, the motif has been conserved throughout bilaterian orthologs. Groucho mediated repression was established prior to the evolution of bilateria.

Published
2005
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11. Variation in structural location and amino acid conservation of functional sites in protein domain families

Author

Copley Richard R, Pils Birgit, and Schultz Jörg

Subjects
Computer applications to medicine. Medical informatics, R858-859.7, Biology (General), QH301-705.5
Abstract

Abstract Background The functional sites of a protein present important information for determining its cellular function and are fundamental in drug design. Accordingly, accurate methods for the prediction of functional sites are of immense value. Most available methods are based on a set of homologous sequences and structural or evolutionary information, and assume that functional sites are more conserved than the average. In the analysis presented here, we have investigated the conservation of location and type of amino acids at functional sites, and compared the behaviour of functional sites between different protein domains. Results Functional sites were extracted from experimentally determined structural complexes from the Protein Data Bank harbouring a conserved protein domain from the SMART database. In general, functional (i.e. interacting) sites whose location is more highly conserved are also more conserved in their type of amino acid. However, even highly conserved functional sites can present a wide spectrum of amino acids. The degree of conservation strongly depends on the function of the protein domain and ranges from highly conserved in location and amino acid to very variable. Differentiation by binding partner shows that ion binding sites tend to be more conserved than functional sites binding peptides or nucleotides. Conclusion The results gained by this analysis will help improve the accuracy of functional site prediction and facilitate the characterization of unknown protein sequences.

Published
2005
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13. Adoption by clinicians of electronic order communications in NHS secondary care: a descriptive account.

Author

Coleman JJ, Atia J, Evison F, Wilson L, Gallier S, Sames R, Capewell A, Copley R, Gyves H, Ball S, and Pankhurst T

Subjects
Humans, Retrospective Studies, United Kingdom, Medical Order Entry Systems, Secondary Care, State Medicine
Abstract

Background: Due to the rapid advancement in information technology, changes to communication modalities are increasingly implemented in healthcare. One such modality is Computerised Provider Order Entry (CPOE) systems which replace paper, verbal or telephone orders with electronic booking of requests. We aimed to understand the uptake, and user acceptability, of CPOE in a large National Health Service hospital system., Methods: This retrospective single-centre study investigates the longitudinal uptake of communications through the Prescribing, Information and Communication System (PICS). The development and configuration of PICS are led by the doctors, nurses and allied health professionals that use it and requests for CPOE driven by clinical need have been described.Records of every request (imaging, specialty review, procedure, laboratory) made through PICS were collected between October 2008 and July 2019 and resulting counts were presented. An estimate of the proportion of completed requests made through the system has been provided for three example requests. User surveys were completed., Results: In the first 6 months of implementation, a total of 832 new request types (imaging types and specialty referrals) were added to the system. Subsequently, an average of 6.6 new request types were added monthly. In total, 8 035 132 orders were requested through PICS. In three example request types (imaging, endoscopy and full blood count), increases in the proportion of requests being made via PICS were seen. User feedback at 6 months reported improved communications using the electronic system., Conclusion: CPOE was popular, rapidly adopted and diversified across specialties encompassing wide-ranging requests., Competing Interests: Competing interests: None declared., (© Author(s) (or their employer(s)) 2024. Re-use permitted under CC BY-NC. No commercial re-use. See rights and permissions. Published by BMJ.)

Published
2024
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14. Effect of Tart Cherry on Aromatase Inhibitor-Induced Arthralgia (AIA) in Nonmetastatic Hormone-Positive Breast Cancer Patients: A Randomized Double-Blind Placebo-Controlled Trial.

Author

Shenouda M, Copley R, Pacioles T, Lebowicz Y, Jamil M, Akpanudo S, and Tirona MT

Subjects
Adult, Arthralgia chemically induced, Breast Neoplasms pathology, Double-Blind Method, Female, Humans, Middle Aged, Musculoskeletal Pain prevention & control, Quality of Life, Antineoplastic Agents adverse effects, Aromatase Inhibitors adverse effects, Arthralgia prevention & control, Breast Neoplasms drug therapy, Prunus avium
Abstract

Background: Aromatase Inhibitor induced Arthralgia (AIA) can cause noncompliance leading to decreased breast-cancer survival. Effective interventions for AIA are limited. Tart cherry (TC) showed beneficial effect on musculoskeletal pain. 48 patients (Pts) randomized to TC versus placebo over 6 weeks, TC (23pts) had 34.7% mean pain decrease versus 1.4% in Placebo (25pts). TC can improve AIA in nonmetastatic breast-cancer patients., Methods: Randomized, placebo-controlled, double-blind trial. Eligible patients with NMHPBC on AI for at least 4 weeks were randomized to TC concentrate [50 tart cherries] vs. placebo (P) [syrup] in 1:1 model. Patients instructed to consume 1 Oz of concentrate in 8 Oz water daily for 6 weeks, and document their pain intensity at baseline, weekly and at study completion in a diary using Visual Analog Scale (VAS), with 0 mm indicating no pain, and 100 mm indicating highest pain., Results: Sixty patients were enrolled. Two patients did not complete the study due to diarrhea, and 10 patients were noncompliant. Forty-eight patients were included in the final analysis. TC group (23 pts) had 34.7% mean decrease in pain compared to 1.4% in P group (25 pts). This difference was statistically significant (Mann-Whitney U Test, P = .034)., Conclusions: Tart cherry can significantly improve AIA in nonmetastatic breast cancer patient., Competing Interests: Disclosure This clinical trial was supported by a grant from the Cherry Marketing Institute, Dewitt, Michigan. The authors otherwise declare that there is no conflict of interest., (Copyright © 2021 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2022
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15. Structure and function of CYP108D1 from Novosphingobium aromaticivorans DSM12444: an aromatic hydrocarbon-binding P450 enzyme.

Author

Bell SG, Yang W, Yorke JA, Zhou W, Wang H, Harmer J, Copley R, Zhang A, Zhou R, Bartlam M, Rao Z, and Wong LL

Subjects
Bacterial Proteins genetics, Bacterial Proteins metabolism, Binding Sites physiology, Biocatalysis, Biodegradation, Environmental, Catalytic Domain, Crystallography, X-Ray, Cytochrome P-450 Enzyme System genetics, Cytochrome P-450 Enzyme System metabolism, Ferredoxins metabolism, Protein Structure, Secondary, Sphingomonadaceae metabolism, Substrate Specificity, Bacterial Proteins chemistry, Cytochrome P-450 Enzyme System chemistry, Ferredoxins chemistry, Hydrocarbons, Aromatic chemistry, Sphingomonadaceae enzymology
Abstract

CYP108D1 from Novosphingobium aromaticivorans DSM12444 binds a range of aromatic hydrocarbons such as phenanthrene, biphenyl and phenylcyclohexane. Its structure, which is reported here at 2.2 Å resolution, is closely related to that of CYP108A1 (P450terp), an α-terpineol-oxidizing enzyme. The compositions and structures of the active sites of these two enzymes are very similar; the most significant changes are the replacement of Glu77 and Thr103 in CYP108A1 by Thr79 and Val105 in CYP108D1. Other residue differences lead to a larger and more hydrophobic access channel in CYP108D1. These structural features are likely to account for the weaker α-terpineol binding by CYP108D1 and, when combined with the presence of three hydrophobic phenylalanine residues in the active site, promote the binding of aromatic hydrocarbons. The haem-proximal surface of CYP108D1 shows a different charge distribution and topology to those of CYP101D1, CYP101A1 and CYP108A1, including a pronounced kink in the proximal loop of CYP108D1, which may result in poor complementarity with the [2Fe-2S] ferredoxins Arx, putidaredoxin and terpredoxin that are the respective redox partners of these three P450 enzymes. The unexpectedly low reduction potential of phenylcyclohexane-bound CYP108D1 (-401 mV) may also contribute to the low activity observed with these ferredoxins. CYP108D1 appears to function as an aromatic hydrocarbon hydroxylase that requires a different electron-transfer cofactor protein.

Published
2012
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16. Dynamic and physical clustering of gene expression during epidermal barrier formation in differentiating keratinocytes.

Author

Taylor JM, Street TL, Hao L, Copley R, Taylor MS, Hayden PJ, Stolper G, Mott R, Hein J, Moffatt MF, and Cookson WO

Subjects
Algorithms, Cell Differentiation, Cluster Analysis, False Positive Reactions, Gene Expression Profiling, Humans, Immune System, Models, Biological, Multigene Family, Nucleic Acid Hybridization, Oligonucleotide Array Sequence Analysis, Promoter Regions, Genetic, Epidermal Cells, Gene Expression Regulation, Keratinocytes cytology
Abstract

The mammalian epidermis is a continually renewing structure that provides the interface between the organism and an innately hostile environment. The keratinocyte is its principal cell. Keratinocyte proteins form a physical epithelial barrier, protect against microbial damage, and prepare immune responses to danger. Epithelial immunity is disordered in many common diseases and disordered epithelial differentiation underlies many cancers. In order to identify the genes that mediate epithelial development we used a tissue model of the skin derived from primary human keratinocytes. We measured global gene expression in triplicate at five times over the ten days that the keratinocytes took to fully differentiate. We identified 1282 gene transcripts that significantly changed during differentiation (false discovery rate <0.01%). We robustly grouped these transcripts by K-means clustering into modules with distinct temporal expression patterns, shared regulatory motifs, and biological functions. We found a striking cluster of late expressed genes that form the structural and innate immune defences of the epithelial barrier. Gene Ontology analyses showed that undifferentiated keratinocytes were characterised by genes for motility and the adaptive immune response. We systematically identified calcium-binding genes, which may operate with the epidermal calcium gradient to control keratinocyte division during skin repair. The results provide multiple novel insights into keratinocyte biology, in particular providing a comprehensive list of known and previously unrecognised major components of the epidermal barrier. The findings provide a reference for subsequent understanding of how the barrier functions in health and disease.

Published
2009
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17. Deploying a new system for recording and managing information during an emergency to aid decision making.

Author

Senior A and Copley R

Abstract

The management of the huge amount of information generated during an emergency is an important tool for effective response and short-term recovery. A key part of that management is the ability to make the information accessible to everyone responding to and affected by the emergency. This paper describes an IT-based emergency planning information management system developed by Rotherham Metropolitan Borough Council in partnership with BT, which allows for the logging, actioning and dissemination of information generated during an emergency. A key component of the management system is its geographical information system capability and how this can be used to enhance emergency response. Furthermore, a description of how the system is used during emergency response is also included.

Published
2008

18. New developments in the InterPro database.

Author

Mulder NJ, Apweiler R, Attwood TK, Bairoch A, Bateman A, Binns D, Bork P, Buillard V, Cerutti L, Copley R, Courcelle E, Das U, Daugherty L, Dibley M, Finn R, Fleischmann W, Gough J, Haft D, Hulo N, Hunter S, Kahn D, Kanapin A, Kejariwal A, Labarga A, Langendijk-Genevaux PS, Lonsdale D, Lopez R, Letunic I, Madera M, Maslen J, McAnulla C, McDowall J, Mistry J, Mitchell A, Nikolskaya AN, Orchard S, Orengo C, Petryszak R, Selengut JD, Sigrist CJ, Thomas PD, Valentin F, Wilson D, Wu CH, and Yeats C

Subjects
Internet, Protein Structure, Tertiary, Proteins chemistry, Proteins classification, Proteins physiology, Sequence Analysis, Protein, Systems Integration, User-Computer Interface, Databases, Protein
Abstract

InterPro is an integrated resource for protein families, domains and functional sites, which integrates the following protein signature databases: PROSITE, PRINTS, ProDom, Pfam, SMART, TIGRFAMs, PIRSF, SUPERFAMILY, Gene3D and PANTHER. The latter two new member databases have been integrated since the last publication in this journal. There have been several new developments in InterPro, including an additional reading field, new database links, extensions to the web interface and additional match XML files. InterPro has always provided matches to UniProtKB proteins on the website and in the match XML file on the FTP site. Additional matches to proteins in UniParc (UniProt archive) are now available for download in the new match XML files only. The latest InterPro release (13.0) contains more than 13 000 entries, covering over 78% of all proteins in UniProtKB. The database is available for text- and sequence-based searches via a webserver (http://www.ebi.ac.uk/interpro), and for download by anonymous FTP (ftp://ftp.ebi.ac.uk/pub/databases/interpro). The InterProScan search tool is now also available via a web service at http://www.ebi.ac.uk/Tools/webservices/WSInterProScan.html.

Published
2007
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19. Dissociated nonsteroidal glucocorticoid receptor modulators; discovery of the agonist trigger in a tetrahydronaphthalene-benzoxazine series.

Author

Barker M, Clackers M, Copley R, Demaine DA, Humphreys D, Inglis GG, Johnston MJ, Jones HT, Haase MV, House D, Loiseau R, Nisbet L, Pacquet F, Skone PA, Shanahan SE, Tape D, Vinader VM, Washington M, Uings I, Upton R, McLay IM, and Macdonald SJ

Subjects
Administration, Topical, Animals, Anti-Inflammatory Agents, Non-Steroidal chemistry, Anti-Inflammatory Agents, Non-Steroidal pharmacology, Benzoxazines chemistry, Benzoxazines pharmacology, Binding, Competitive, Cell Line, Dexamethasone pharmacology, Humans, Hypersensitivity, Delayed drug therapy, Mice, Models, Molecular, Radioligand Assay, Receptors, Glucocorticoid antagonists & inhibitors, Receptors, Glucocorticoid genetics, Stereoisomerism, Structure-Activity Relationship, Tetrahydronaphthalenes chemistry, Tetrahydronaphthalenes pharmacology, Transcription, Genetic drug effects, Transcriptional Activation drug effects, Anti-Inflammatory Agents, Non-Steroidal chemical synthesis, Benzoxazines chemical synthesis, Receptors, Glucocorticoid agonists, Tetrahydronaphthalenes chemical synthesis
Abstract

The tetrahydronaphthalene-benzoxazine glucocorticoid receptor (GR) partial agonist 4b was optimized to produce potent full agonists of GR. Aromatic ring substitution of the tetrahydronaphthalene leads to weak GR antagonists. Discovery of an "agonist trigger" substituent on the saturated ring of the tetrahydronaphthalene leads to increased potency and efficacious GR agonism. These compounds are efficacy selective in an NFkB GR agonist assay (representing transrepression effects) over an MMTV GR agonist assay (representing transactivation effects). 52 and 60 have NFkB pIC(50) = 8.92 (105%) and 8.69 (92%) and MMTV pEC(50) = 8.20 (47%) and 7.75 (39%), respectively. The impact of the trigger substituent on agonism is modeled within GR and discussed. 36, 52, and 60 have anti-inflammatory activity in a mouse model of inflammation after topical dosing with 52 and 60, having an effect similar to that of dexamethasone. The original lead was discovered by a manual agreement docking method, and automation of this method is also described.

Published
2006
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20. InterPro, progress and status in 2005.

Author

Mulder NJ, Apweiler R, Attwood TK, Bairoch A, Bateman A, Binns D, Bradley P, Bork P, Bucher P, Cerutti L, Copley R, Courcelle E, Das U, Durbin R, Fleischmann W, Gough J, Haft D, Harte N, Hulo N, Kahn D, Kanapin A, Krestyaninova M, Lonsdale D, Lopez R, Letunic I, Madera M, Maslen J, McDowall J, Mitchell A, Nikolskaya AN, Orchard S, Pagni M, Ponting CP, Quevillon E, Selengut J, Sigrist CJ, Silventoinen V, Studholme DJ, Vaughan R, and Wu CH

Subjects
Humans, Protein Structure, Tertiary, Sequence Alignment, Systems Integration, Databases, Protein trends, Proteins chemistry, Proteins classification, Sequence Analysis, Protein
Abstract

InterPro, an integrated documentation resource of protein families, domains and functional sites, was created to integrate the major protein signature databases. Currently, it includes PROSITE, Pfam, PRINTS, ProDom, SMART, TIGRFAMs, PIRSF and SUPERFAMILY. Signatures are manually integrated into InterPro entries that are curated to provide biological and functional information. Annotation is provided in an abstract, Gene Ontology mapping and links to specialized databases. New features of InterPro include extended protein match views, taxonomic range information and protein 3D structure data. One of the new match views is the InterPro Domain Architecture view, which shows the domain composition of protein matches. Two new entry types were introduced to better describe InterPro entries: these are active site and binding site. PIRSF and the structure-based SUPERFAMILY are the latest member databases to join InterPro, and CATH and PANTHER are soon to be integrated. InterPro release 8.0 contains 11 007 entries, representing 2573 domains, 8166 families, 201 repeats, 26 active sites, 21 binding sites and 20 post-translational modification sites. InterPro covers over 78% of all proteins in the Swiss-Prot and TrEMBL components of UniProt. The database is available for text- and sequence-based searches via a webserver (http://www.ebi.ac.uk/interpro), and for download by anonymous FTP (ftp://ftp.ebi.ac.uk/pub/databases/interpro).

Published
2005
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21. InterPro: an integrated documentation resource for protein families, domains and functional sites.

Author

Mulder NJ, Apweiler R, Attwood TK, Bairoch A, Bateman A, Binns D, Biswas M, Bradley P, Bork P, Bucher P, Copley R, Courcelle E, Durbin R, Falquet L, Fleischmann W, Gouzy J, Griffith-Jones S, Haft D, Hermjakob H, Hulo N, Kahn D, Kanapin A, Krestyaninova M, Lopez R, Letunic I, Orchard S, Pagni M, Peyruc D, Ponting CP, Servant F, and Sigrist CJ

Subjects
Algorithms, Humans, Information Services, Internet, Software, Computational Biology, Databases, Protein, Proteins chemistry, Proteins classification
Abstract

The exponential increase in the submission of nucleotide sequences to the nucleotide sequence database by genome sequencing centres has resulted in a need for rapid, automatic methods for classification of the resulting protein sequences. There are several signature and sequence cluster-based methods for protein classification, each resource having distinct areas of optimum application owing to the differences in the underlying analysis methods. In recognition of this, InterPro was developed as an integrated documentation resource for protein families, domains and functional sites, to rationalise the complementary efforts of the individual protein signature database projects. The member databases - PRINTS, PROSITE, Pfam, ProDom, SMART and TIGRFAMs - form the InterPro core. Related signatures from each member database are unified into single InterPro entries. Each InterPro entry includes a unique accession number, functional descriptions and literature references, and links are made back to the relevant member database(s). Release 4.0 of InterPro (November 2001) contains 4,691 entries, representing 3,532 families, 1,068 domains, 74 repeats and 15 sites of post-translational modification (PTMs) encoded by different regular expressions, profiles, fingerprints and hidden Markov models (HMMs). Each InterPro entry lists all the matches against SWISS-PROT and TrEMBL (2,141,621 InterPro hits from 586,124 SWISS-PROT and TrEMBL protein sequences). The database is freely accessible for text- and sequence-based searches.

Published
2002
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22. Novel protein domains and repeats in Drosophila melanogaster: insights into structure, function, and evolution.

Author

Ponting CP, Mott R, Bork P, and Copley RR

Subjects
Amino Acid Sequence genetics, Amino Acid Transport Systems, Neutral, Animals, Antigens, Differentiation, B-Lymphocyte chemistry, Antigens, Differentiation, B-Lymphocyte genetics, Antigens, Differentiation, B-Lymphocyte physiology, Aspartate-tRNA Ligase chemistry, Aspartate-tRNA Ligase genetics, Aspartate-tRNA Ligase physiology, Cystinosis genetics, Drosophila Proteins genetics, Drosophila melanogaster enzymology, Drosophila melanogaster genetics, Exons genetics, GTP-Binding Proteins, Gene Duplication, Glycoside Hydrolases chemistry, Glycoside Hydrolases genetics, Glycoside Hydrolases physiology, Histocompatibility Antigens Class II chemistry, Histocompatibility Antigens Class II genetics, Histocompatibility Antigens Class II physiology, Humans, Insect Proteins chemistry, Insect Proteins genetics, Insect Proteins physiology, Intracellular Signaling Peptides and Proteins, Membrane Proteins chemistry, Membrane Proteins genetics, Membrane Proteins physiology, Membrane Transport Proteins, Molecular Sequence Data, Muscular Dystrophies genetics, Protein Structure, Secondary, Protein Structure, Tertiary, Proteins chemistry, Proteins genetics, Proteins physiology, Retinitis Pigmentosa genetics, Signal Transduction genetics, Species Specificity, Tandem Repeat Sequences, Drosophila Proteins chemistry, Drosophila Proteins physiology, Drosophila melanogaster chemistry, Evolution, Molecular, Eye Proteins, Glycoproteins, Repetitive Sequences, Amino Acid
Abstract

Sequence database searching methods such as BLAST, are invaluable for predicting molecular function on the basis of sequence similarities among single regions of proteins. Searches of whole databases however, are not optimized to detect multiple homologous regions within a single polypeptide. Here we have used the prospero algorithm to perform self-comparisons of all predicted Drosophila melanogaster gene products. Predicted repeats, and their homologs from all species, were analyzed further to detect hitherto unappreciated evolutionary relationships. Results included the identification of novel tandem repeats in the human X-linked retinitis pigmentosa type-2 gene product, repeated segments in cystinosin, associated with a defect in cystine transport, and 'nested' homologous domains in dysferlin, whose gene is mutated in limb girdle muscular dystrophy. Novel signaling domain families were found that may regulate the microtubule-based cytoskeleton and ubiquitin-mediated proteolysis, respectively. Two families of glycosyl hydrolases were shown to contain internal repetitions that hint at their evolution via a piecemeal, modular approach. In addition, three examples of fruit fly genes were detected with tandem exons that appear to have arisen via internal duplication. These findings demonstrate how completely sequenced genomes can be exploited to further understand the relationships between molecular structure, function, and evolution.

Published
2001
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23. Synthesis of chiral 1,2-diamines by asymmetric lithiation-substitution.

Author

Coldham I, Copley RC, Haxell TF, and Howard S

Abstract

[reaction--see text] The imidazolidine (tetrahydroimidazole) 2, prepared in one step from N-iso-propylethylenediamine, was subjected to asymmetric lithiation and substitution using sec-butyllithium, (-)-sparteine and a range of electrophiles. Substituted imidazolidines were formed with high optical purity and could be hydrolyzed under acidic conditions to chiral, substituted ethylenediamines. Kinetic data indicate that the conformation of the carbonyl group is crucial to the extent of deprotonation, and this has implications for the lithiation of unsymmetrical carbamates and carboxylic amides.

Published
2001
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24. General method for the description, visualization and comparison of metal coordination spheres: geometrical preferences, deformations and interconversion pathways.

Author

Yao JW, Copley RC, Howard JA, Allen FH, and Motherwell WD

Abstract

The coordination sphere geometry of metal atoms (M) in their complexes with organic and inorganic ligands (L) is often compared with the geometry of archetypal forms for the appropriate coordination number, n in ML(n) species, by use of the k = n( n- 1)/2 L-M-L valence angles subtended at the metal centre. Here, a Euclidean dissimilarity metric, R(c)(x), is introduced as a one-dimensional comparator of these k-dimensional valence-angle spaces. The computational procedure for R(c)(x), where x is an appropriate archetypal form (e.g. an octahedron in ML(6) species), takes account of the atomic permutational symmetry inherent in ML(n) systems when no distinction is made between the individual ligand atoms. It is this permutational symmetry, of order n!, that precludes the routine application of multivariate analytical techniques, such as principal component analysis (PCA), to valence angle data for all but the lowest metal coordination numbers. It is shown that histograms of R(c)(x) values and, particularly, scatterplots of R(c)(x) values computed with respect to two or more different appropriate archetypal forms (e.g. tetrahedral and square-planar four-coordinations), provide information-rich visualizations of the observed geometrical preferences of metal coordination spheres retrieved from, e.g. the Cambridge Structural Database. These mappings reveal the highly populated clusters of similar geometries, together with the pathways that map their geometrical interconversions. Application of R(c)(x) analysis to the geometry of four- and seven-coordination spheres provides information that is at least comparable to, and in some cases is more complete than, that obtained by PCA.

Published
2001
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25. DDT -- a novel domain in different transcription and chromosome remodeling factors.

Author

Doerks T, Copley R, and Bork P

Subjects
Amino Acid Sequence, Homeodomain Proteins chemistry, Molecular Sequence Data, Sequence Homology, Amino Acid, Chromosomes, Transcription Factors chemistry
Abstract

Homology-based sequence analyses have revealed the presence of a novel domain (DDT) in bromodomain PHD finger transcription factors (BPTFs), chromatin remodeling factors of the BAZ-family and other putative nuclear proteins. This domain is characterized by a number of conserved aromatic and charged residues and is predicted to consist of three alpha helices. Recent studies indicate a likely DNA-binding function for the DDT domain.

Published
2001
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27. Initial sequencing and analysis of the human genome.

Author

Lander ES, Linton LM, Birren B, Nusbaum C, Zody MC, Baldwin J, Devon K, Dewar K, Doyle M, FitzHugh W, Funke R, Gage D, Harris K, Heaford A, Howland J, Kann L, Lehoczky J, LeVine R, McEwan P, McKernan K, Meldrim J, Mesirov JP, Miranda C, Morris W, Naylor J, Raymond C, Rosetti M, Santos R, Sheridan A, Sougnez C, Stange-Thomann Y, Stojanovic N, Subramanian A, Wyman D, Rogers J, Sulston J, Ainscough R, Beck S, Bentley D, Burton J, Clee C, Carter N, Coulson A, Deadman R, Deloukas P, Dunham A, Dunham I, Durbin R, French L, Grafham D, Gregory S, Hubbard T, Humphray S, Hunt A, Jones M, Lloyd C, McMurray A, Matthews L, Mercer S, Milne S, Mullikin JC, Mungall A, Plumb R, Ross M, Shownkeen R, Sims S, Waterston RH, Wilson RK, Hillier LW, McPherson JD, Marra MA, Mardis ER, Fulton LA, Chinwalla AT, Pepin KH, Gish WR, Chissoe SL, Wendl MC, Delehaunty KD, Miner TL, Delehaunty A, Kramer JB, Cook LL, Fulton RS, Johnson DL, Minx PJ, Clifton SW, Hawkins T, Branscomb E, Predki P, Richardson P, Wenning S, Slezak T, Doggett N, Cheng JF, Olsen A, Lucas S, Elkin C, Uberbacher E, Frazier M, Gibbs RA, Muzny DM, Scherer SE, Bouck JB, Sodergren EJ, Worley KC, Rives CM, Gorrell JH, Metzker ML, Naylor SL, Kucherlapati RS, Nelson DL, Weinstock GM, Sakaki Y, Fujiyama A, Hattori M, Yada T, Toyoda A, Itoh T, Kawagoe C, Watanabe H, Totoki Y, Taylor T, Weissenbach J, Heilig R, Saurin W, Artiguenave F, Brottier P, Bruls T, Pelletier E, Robert C, Wincker P, Smith DR, Doucette-Stamm L, Rubenfield M, Weinstock K, Lee HM, Dubois J, Rosenthal A, Platzer M, Nyakatura G, Taudien S, Rump A, Yang H, Yu J, Wang J, Huang G, Gu J, Hood L, Rowen L, Madan A, Qin S, Davis RW, Federspiel NA, Abola AP, Proctor MJ, Myers RM, Schmutz J, Dickson M, Grimwood J, Cox DR, Olson MV, Kaul R, Raymond C, Shimizu N, Kawasaki K, Minoshima S, Evans GA, Athanasiou M, Schultz R, Roe BA, Chen F, Pan H, Ramser J, Lehrach H, Reinhardt R, McCombie WR, de la Bastide M, Dedhia N, Blöcker H, Hornischer K, Nordsiek G, Agarwala R, Aravind L, Bailey JA, Bateman A, Batzoglou S, Birney E, Bork P, Brown DG, Burge CB, Cerutti L, Chen HC, Church D, Clamp M, Copley RR, Doerks T, Eddy SR, Eichler EE, Furey TS, Galagan J, Gilbert JG, Harmon C, Hayashizaki Y, Haussler D, Hermjakob H, Hokamp K, Jang W, Johnson LS, Jones TA, Kasif S, Kaspryzk A, Kennedy S, Kent WJ, Kitts P, Koonin EV, Korf I, Kulp D, Lancet D, Lowe TM, McLysaght A, Mikkelsen T, Moran JV, Mulder N, Pollara VJ, Ponting CP, Schuler G, Schultz J, Slater G, Smit AF, Stupka E, Szustakowki J, Thierry-Mieg D, Thierry-Mieg J, Wagner L, Wallis J, Wheeler R, Williams A, Wolf YI, Wolfe KH, Yang SP, Yeh RF, Collins F, Guyer MS, Peterson J, Felsenfeld A, Wetterstrand KA, Patrinos A, Morgan MJ, de Jong P, Catanese JJ, Osoegawa K, Shizuya H, Choi S, Chen YJ, and Szustakowki J

Subjects
Animals, Chromosome Mapping, Conserved Sequence, CpG Islands, DNA Transposable Elements, Databases, Factual, Drug Industry, Evolution, Molecular, Forecasting, GC Rich Sequence, Gene Duplication, Genes, Genetic Diseases, Inborn, Genetics, Medical, Humans, Mutation, Private Sector, Proteins genetics, Proteome, Public Sector, RNA genetics, Repetitive Sequences, Nucleic Acid, Species Specificity, Genome, Human, Human Genome Project, Sequence Analysis, DNA methods
Abstract

The human genome holds an extraordinary trove of information about human development, physiology, medicine and evolution. Here we report the results of an international collaboration to produce and make freely available a draft sequence of the human genome. We also present an initial analysis of the data, describing some of the insights that can be gleaned from the sequence.

Published
2001
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28. Sialidase-like Asp-boxes: sequence-similar structures within different protein folds.

Author

Copley RR, Russell RB, and Ponting CP

Subjects
Acetylglucosaminidase chemistry, Amino Acid Motifs, Amino Acid Sequence, Databases, Factual, Evolution, Molecular, Models, Molecular, Molecular Sequence Data, Protein Folding, Protein Structure, Tertiary, Ribonucleases chemistry, Sequence Homology, Amino Acid, Water chemistry, Aspartic Acid chemistry, Neuraminidase chemistry
Abstract

Sequence similarity is the most common measure currently used to infer homology between proteins. Typically, homologous protein domains show sequence similarity over their entire lengths. Here we identify Asp box motifs, initially found as repeats in sialidases and neuraminidases, in new structural and sequence contexts. These motifs represent significantly similar sequences, localized to beta hairpins within proteins that are otherwise different in sequence and three-dimensional structure. By performing a combined sequence- and structure-based analysis we detect Asp boxes in more than nine protein families, including bacterial ribonucleases, sulfite oxidases, reelin, netrins, some lipoprotein receptors, and a variety of glycosyl hydrolases. Although the function common to each of these proteins, if any, remains unclear, we discuss possible functions of Asp boxes on the basis of previously determined experimental results and discuss different evolutionary scenarios for the origin of Asp-box containing proteins.

Published
2001
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29. Functional genomic analysis of cell division in C. elegans using RNAi of genes on chromosome III.

Author

Gönczy P, Echeverri C, Oegema K, Coulson A, Jones SJ, Copley RR, Duperon J, Oegema J, Brehm M, Cassin E, Hannak E, Kirkham M, Pichler S, Flohrs K, Goessen A, Leidel S, Alleaume AM, Martin C, Ozlü N, Bork P, and Hyman AA

Subjects
Animals, Caenorhabditis elegans physiology, Chromosomes, Genomics, Open Reading Frames, Caenorhabditis elegans genetics, Cell Division genetics, Genes, Helminth, RNA, Helminth
Abstract

Genome sequencing projects generate a wealth of information; however, the ultimate goal of such projects is to accelerate the identification of the biological function of genes. This creates a need for comprehensive studies to fill the gap between sequence and function. Here we report the results of a functional genomic screen to identify genes required for cell division in Caenorhabditis elegans. We inhibited the expression of approximately 96% of the approximately 2,300 predicted open reading frames on chromosome III using RNA-mediated interference (RNAi). By using an in vivo time-lapse differential interference contrast microscopy assay, we identified 133 genes (approximately 6%) necessary for distinct cellular processes in early embryos. Our results indicate that these genes represent most of the genes on chromosome III that are required for proper cell division in C. elegans embryos. The complete data set, including sample time-lapse recordings, has been deposited in an open access database. We found that approximately 47% of the genes associated with a differential interference contrast phenotype have clear orthologues in other eukaryotes, indicating that this screen provides putative gene functions for other species as well.

Published
2000
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30. Homology among (betaalpha)(8) barrels: implications for the evolution of metabolic pathways.

Author

Copley RR and Bork P

Subjects
Aldehyde-Lyases chemistry, Aldehyde-Lyases metabolism, Amino Acid Sequence, Animals, Binding Sites, Computational Biology, Databases as Topic, Humans, Models, Molecular, Molecular Sequence Data, Multigene Family, Phosphates metabolism, Phosphopyruvate Hydratase chemistry, Phosphopyruvate Hydratase metabolism, Phylogeny, Protein Structure, Secondary, Pyruvate Kinase chemistry, Pyruvate Kinase metabolism, Sequence Alignment, Sequence Homology, Amino Acid, Enzymes chemistry, Enzymes metabolism, Evolution, Molecular, Protein Structure, Tertiary
Abstract

We provide statistically reliable sequence evidence indicating that at least 12 of 23 SCOP (betaalpha)(8) (TIM) barrel superfamilies share a common origin. This includes all but one of the known and predicted TIM barrels found in central metabolism. The statistical evidence is complemented by an examination of the details of protein structure, with certain structural locations favouring catalytic residues even though the nature of their molecular function may change. The combined analysis of sequence, structure and function also enables us to propose a phylogeny of TIM barrels. Based on these data, we are able to examine differing theories of pathway and enzyme evolution, by mapping known TIM barrel folds to the pathways of central metabolism. The results favour widespread recruitment of enzymes between pathways, rather than a "backwards evolution" model, and support the idea that modern proteins may have arisen from common ancestors that bound key metabolites., (Copyright 2000 Academic Press.)

Published
2000
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31. Inhibitors of bacterial tyrosyl tRNA synthetase: synthesis of four stereoisomeric analogues of the natural product SB-219383.

Author

Berge JM, Copley RC, Eggleston DS, Hamprecht DW, Jarvest RL, Mensah LM, O'Hanlon PJ, and Pope AJ

Subjects
Bacterial Physiological Phenomena, Chemistry, Organic, Enzyme Inhibitors chemical synthesis, Magnetic Resonance Spectroscopy, Molecular Structure, Organic Chemistry Phenomena, Stereoisomerism, Bridged Bicyclo Compounds, Heterocyclic chemical synthesis, Bridged Bicyclo Compounds, Heterocyclic chemistry, Enzyme Inhibitors chemistry, Furans chemical synthesis, Furans chemistry, Tyrosine-tRNA Ligase antagonists & inhibitors
Abstract

Synthetic analogues of the microbial metabolite SB-219383 have been synthesised with defined stereochemistry. Densely functionalised hydroxylamine containing amino acids were prepared by the addition of a glycine anion equivalent to sugar-derived cyclic nitrones. One of four stereoisomeric dipeptides incorporating these novel amino acids was found to be a potent and selective inhibitor of bacterial tyrosyl tRNA synthetase, suggesting analogous stereochemistry of the natural product.

Published
2000
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32. SB-253514 and analogues: novel inhibitors of lipoprotein associated phospholipase A2 produced by Pseudomonas fluorescens DSM 11579. II. Physico-chemical properties and structure elucidation.

Author

Busby DJ, Copley RC, Hueso JA, Readshaw SA, and Rivera A

Subjects
1-Alkyl-2-acetylglycerophosphocholine Esterase, Bridged Bicyclo Compounds, Heterocyclic chemistry, Crystallography, X-Ray, Magnetic Resonance Spectroscopy, Molecular Structure, Phospholipases A2, Pseudomonas fluorescens metabolism, Pyrans chemistry, Enzyme Inhibitors chemistry, Phospholipases A antagonists & inhibitors
Abstract

A series of novel inhibitors of lipoprotein associated phospholipase A2 were isolated from the culture broths of Pseudomonas fluorescens strain DSM11579. The inhibitors fall into two structurally isomeric classes each of which comprise compounds incorporating glycosylated hydrocarbon chains. The structure elucidation for the major member of each structural class is reported. The crystal structure of a non-glycosylated analogue of the 5,5-series, produced through biotransformation, is also reported.

Published
2000

33. More than 1,000 putative new human signalling proteins revealed by EST data mining.

Author

Schultz J, Doerks T, Ponting CP, Copley RR, and Bork P

Subjects
Amino Acid Sequence, Automation, Catalytic Domain, Cloning, Molecular methods, Databases, Factual, Genome, Human, Humans, Internet, Molecular Sequence Data, Monomeric GTP-Binding Proteins chemistry, Monomeric GTP-Binding Proteins genetics, Monomeric GTP-Binding Proteins metabolism, Protein Structure, Tertiary, Proteins chemistry, Sequence Alignment, Sequence Homology, Amino Acid, Software, Computational Biology methods, Expressed Sequence Tags, Proteins genetics, Proteins metabolism, Signal Transduction
Abstract

Cloning procedures aided by homology searches of EST databases have accelerated the pace of discovery of new genes, but EST database searching remains an involved and onerous task. More than 1.6 million human EST sequences have been deposited in public databases, making it difficult to identify ESTs that represent new genes. Compounding the problems of scale are difficulties in detection associated with a high sequencing error rate and low sequence similarity between distant homologues. We have developed a new method, coupling BLAST-based searches with a domain identification protocol, that filters candidate homologues. Application of this method in a large-scale analysis of 100 signalling domain families has led to the identification of ESTs representing more than 1,000 novel human signalling genes. The 4,206 publicly available ESTs representing these genes are a valuable resource for rapid cloning of novel human signalling proteins. For example, we were able to identify ESTs of at least 106 new small GTPases, of which 6 are likely to belong to new subfamilies. In some cases, further analyses of genomic DNA led to the discovery of previously unidentified full-length protein sequences. This is exemplified by the in silico cloning (prediction of a gene product sequence using only genomic and EST sequence data) of a new type of GTPase with two catalytic domains.

Published
2000
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34. Evolution of domain families.

Author

Ponting CP, Schultz J, Copley RR, Andrade MA, and Bork P

Subjects
Amino Acid Motifs, Amino Acid Sequence, Animals, Archaea chemistry, Bacteria chemistry, Eukaryotic Cells chemistry, Humans, Molecular Sequence Data, Sequence Homology, Amino Acid, Evolution, Molecular, Protein Structure, Tertiary, Proteins chemistry
Published
2000
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35. SMART: a web-based tool for the study of genetically mobile domains.

Author

Schultz J, Copley RR, Doerks T, Ponting CP, and Bork P

Subjects
Information Storage and Retrieval, Proteins chemistry, Database Management Systems, Internet, Sequence Alignment
Abstract

SMART (a Simple Modular Architecture Research Tool) allows the identification and annotation of genetically mobile domains and the analysis of domain architectures (http://SMART.embl-heidelberg.de ). More than 400 domain families found in signalling, extra-cellular and chromatin-associated proteins are detectable. These domains are extensively annotated with respect to phyletic distributions, functional class, tertiary structures and functionally important residues. Each domain found in a non-redundant protein database as well as search parameters and taxonomic information are stored in a relational database system. User interfaces to this database allow searches for proteins containing specific combinations of domains in defined taxa.

Published
2000
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36. Phospholipases A2 and Wnts are unlikely to share a common ancestor.

Author

Copley RR, Ponting CP, and Bork P

Subjects
Conserved Sequence, Crystallography, X-Ray, Cysteine chemistry, Evolution, Molecular, Phospholipases A chemistry, Phylogeny, Proto-Oncogene Proteins chemistry, Sequence Homology, Amino Acid, Wnt Proteins, Phospholipases A genetics, Proto-Oncogene Proteins genetics, Zebrafish Proteins
Published
1999
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37. A lipid-binding domain in Wnt: a case of mistaken identity?

Author

Barnes MR, Russell RB, Copley RR, Ponting CP, Bork P, Cumberledge S, Reichsman F, and Moore HM

Subjects
Amino Acid Sequence, Animals, Caenorhabditis elegans genetics, Cell Membrane metabolism, Drosophila melanogaster genetics, Frizzled Receptors, Humans, Molecular Sequence Data, Phospholipases A metabolism, Protein Binding, Protein Structure, Tertiary, Proteins metabolism, Sequence Homology, Amino Acid, Wnt Proteins, Lipid Metabolism, Proto-Oncogene Proteins metabolism, Proto-Oncogene Proteins physiology, Zebrafish Proteins
Published
1999
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38. Protein families in multicellular organisms.

Author

Copley RR, Schultz J, Ponting CP, and Bork P

Subjects
Animals, Conserved Sequence, Genome, Humans, Intracellular Fluid physiology, Phylogeny, Proteins physiology, Signal Transduction genetics, Multigene Family, Proteins chemistry, Proteins genetics
Abstract

The complete sequence of the nematode worm Caenorhabditis elegans contains the genetic machinery that is required to undertake the core biological processes of single cells. However, the genome also encodes proteins that are associated with multicellularity, as well as others that are lineage-specific expansions of phylogenetically widespread families and yet more that are absent in non-nematodes. Ongoing analysis is beginning to illuminate the similarities and differences among human proteins and proteins that are encoded by the genomes of the multicellular worm and the unicellular yeast, and will be essential in determining the reliability of transferring experimental data among phylogenetically distant species.

Published
1999
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40. Fold recognition using sequence and secondary structure information.

Author

Koretke KK, Russell RB, Copley RR, and Lupas AN

Subjects
Algorithms, Amino Acid Sequence, Bacterial Proteins chemistry, Models, Molecular, Molecular Sequence Data, Sequence Alignment, Protein Folding, Protein Structure, Secondary, Proteins chemistry
Abstract

We applied a succession of sequence search and structure prediction methods to the targets in the fold recognition part of the CASP3 experiment. For each target, we expanded an initial sequence space, obtained through PSI-BLAST, by searching for statistically significant relationships to low-scoring sequences and then by searching for conserved sequence patterns. We then divided the proteins in the sequence space into families and built an alignment hierarchically, using the multiple alignment program MACAW. If no significant similarity to a protein of known structure was apparent at this point, we submitted the alignment to the Jpred server for consensus secondary structure prediction and searched the structure space using the secondary structure mapping program MAP. Failing this, we compared the structural properties that we believed we recognized in the aligned proteins to the folds in the SCOP database, using visual inspection. If all these methods failed to uncover a plausible match, we predicted that the target would adopt a novel fold. This procedure yielded correct answers for seven of twenty-one targets and a partly correct answer for one. A retrospective analysis shows that automating the sequence search procedures would have represented a significant improvement, with at least three additional correct predictions.

Published
1999
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41. Protein fold recognition by mapping predicted secondary structures.

Author

Russell RB, Copley RR, and Barton GJ

Subjects
Algorithms, Amino Acid Sequence, Cysteine Endopeptidases chemistry, Molecular Sequence Data, Multienzyme Complexes chemistry, Phosphotyrosine metabolism, Proteasome Endopeptidase Complex, Proteins chemistry, Proteins metabolism, Sequence Alignment methods, Software, von Willebrand Factor chemistry, Models, Molecular, Protein Folding, Protein Structure, Secondary
Abstract

A strategy is presented for protein fold recognition from secondary structure assignments (alpha-helix and beta-strand). The method can detect similarities between protein folds in the absence of sequence similarity. Secondary structure mapping first identifies all possible matches (maps) between a query string of secondary structures and the secondary structures of protein domains of known three-dimensional structure. The maps are then passed through a series of structural filters to remove those that do not obey simple rules of protein structure. The surviving maps are ranked by scores from the alignment of predicted and experimental accessibilities. Searches made with secondary structure assignments for a test set of 11 fold-families put the correct sequence-dissimilar fold in the first rank 8/11 times. With cross-validated predictions of secondary structure this drops to 4/11 which compares favourably with the widely used THREADER program (1/11). The structural class is correctly predicted 10/11 times by the method in contrast to 5/11 for THREADER. The new technique obtains comparable accuracy in the alignment of amino acid residues and secondary structure elements. Searches are also performed with published secondary structure predictions for the von-Willebrand factor type A domain, the proteasome 20 S alpha subunit and the phosphotyrosine interaction domain. These searches demonstrate how the method can find the correct fold for a protein from a carefully constructed secondary structure prediction, multiple sequence alignment and distant restraints. Scans with experimentally determined secondary structures and accessibility, recognise the correct fold with high alignment accuracy (86% on secondary structures). This suggests that the accuracy of mapping will improve alongside any improvements in the prediction of secondary structure or accessibility. Application to NMR structure determination is also discussed.

Published
1996
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42. A structural analysis of phosphate and sulphate binding sites in proteins. Estimation of propensities for binding and conservation of phosphate binding sites.

Author

Copley RR and Barton GJ

Subjects
Crystallography, X-Ray, Protein Conformation, Phosphates metabolism, Protein Binding, Sulfates metabolism
Abstract

The high resolution X-ray structures of 38 proteins that bind phosphate containing groups and 36 proteins binding sulphate ions were analysed to characterise the structural features of anion binding sites in proteins. 34 of the 66 phosphates found were in close proximity to the amino terminus of an alpha-helix. 27% of phosphate groups bind to only one amino acid, but there is a wide distribution, with 3% of phosphates binding to seven residues. Similarly, there is a large variability in the number of contacts each phosphate group makes to the protein. This ranges from none (3% of phosphates) to nine (3% of phosphates). The most common number of contacts is two (23% of phosphates). The most commonly found residue at helix-type binding sites is glycine, followed by Arg, Thr, Ser and Lys. At non-helix binding sites, the most commonly found residue is Arg followed by Tyr, His, Lys and Ser. There is no typical phosphate binding site. There are marked differences between propensities for phosphate binding at helix and non-helix type binding sites. Non-helix binding sites show more discrimination between the types of residues involved in binding when compared to the helix set. The propensities for binding of the amino acids reveal the expected trend of positively charged and polar residues being good at binding (although that for lysine is unexpectedly low) with the bulky non-polar residues being poor at binding. Bulky residues are less likely to bind with the amide nitrogen. Sulphate binding sites show similar trends. Analysis of multiple sequence alignments that include phosphate and sulphate binding proteins reveals the degree of conservation at the binding site residues compared to the average conservation of residues in the protein. Phosphate binding site residues are more conserved than sulphate binding sites.

Published
1994
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43. Patient radiation dose in conventional and xerographic cephalography.

Author

Copley RL, Glaze SA, Bushong SC, and West DC

Subjects
Fluorides, Humans, Lithium, Models, Anatomic, Radiographic Image Enhancement, Thermoluminescent Dosimetry methods, Cephalometry methods, Radiation Dosage, Xeroradiography methods
Abstract

A comparison of the radiation doses for xeroradiographic and conventional film screen cephalography was made. Alderson tissue-equivalent phantoms were used for patient stimulation. An optimum technique in terms of patient dose and imaqe quality was established for the xeroradhe data indicated that the dose for the Xerox process ranged from five to eleven times greater than that for the conventional process for entrance and exit exposures, respectively. The most commonly reported dose, the entrance dose, was found to be 206 mrad, which is five Imes that for the conventional cephalogram. This dose, however, falls within an acceptable range for other dental and medical radiation doses. It is recommended that conventional cephalography be used for routine purposes and that xeroradiography be reserved for situations requiring the increased image quality that the process affords.

Published
1979
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45. Panoramic dental radiography for mass screening?

Author

Bushong SC, Glaze SA, Foster JK, Copley RL, and Miller JT

Subjects
Eyelids, Humans, Mandible, Mastoid, Occipital Bone, Radiation Dosage, Temporomandibular Joint, Thyroid Gland, Mass Screening, Radiation Protection, Radiography, Panoramic
Published
1973
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