CBRC SEVENS






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Previous Ver.
  1.60(2009/06/23)
  1.50(2008/07/17)
  1.40(2006/08/15)
  1.30(2005/05/17)
  1.21(2004/02/06)
  1.20(2003/10/09)

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  Ensembl
  Broad Institute
  BCM
  dictyBase
  IRGSP
  Swiss-Prot
  PROSITE
  Pfam
What's SEVENS

We have developed SEVENS database which includes G-protein coupled receptors (GPCR) genes with seven transmembrane helices (TMH), that are identified with high accuracy from complete genomes of 56 eukaryotes, by a pipeline integrating such software as a gene finder, a sequence alignment tool, a motif and domain assignment tool, and a TMH predictor. To perform an overview of the "GPCR universe", it is necessary to treat a larger data space than that in currently available databases, which should include not only the expressed sequences but also the newly identified sequences that cannot be detected by in vivo experiments, although they definitely exist on the genome sequence and are just waiting for the opportunity to express their functions. For this purpose, we introduce this database.

Contents

  • Content Search
  • Retrieve GPCR candidate sequences by the "AND" combination of (1) Keyword in nr.aa database search results, (2)Chromosome number, (3)Data level, (4)Predicted exon number, (5) Gene length, (6)Protein length, (7)E-value of sequence search against Swiss-Prot, nr.aa, or UniGene, (8) PROSITE motifs, (9) Pfam domains. (10) Novel or not. and (11) Family.

    After selection with some of contents, GPCR candidates will be appear at the chromosomal viewer and the gene lists which navigate to the detailed analysis for each gene.


  • News
  • Release Information and news concerning updates of analysis.


  • What's SEVENS
  • Introduction for SEVENS database and it's usage.


  • Statistics
  • Release information of data statistics.


    How we found GPCR sequences.

    Condidate GPCR genes were collected from 56 eukaryote genomes by using the GPCR gene discovery pipeline, composed of two stages: (1) the gene finding stage, and (2) the GPCR gene screening stage.

    1)Gene finding stage  (i.e., translation of genomic sequences into amino acid sequences).
    2)GPCR gene screening stage  of GPCR candidates by assessing genes with sequence search, motif- and domain assignment, and transmembrane helix (TMH) prediction.

    (1) Gene finding stage:

    Genomic sequences were obtained from ftp sites of NCBI, UCSC, Ensembl, Broad Institute, Baylor College of Medicine, dictyBase, and IRGSP. To maximize the number of gene candidates, we detected two kinds of sequence sets,

    (a)"6f-sequences" which were all possible combination between initial and stop codons in 6 reading frames with the rule of using the most upstream ATG possible.
    (b)"ALN-sequences" The genomic regions where at least partial regions of the known GPCR sequences hit with significant score of TBLASTN are listed. Around these regions full gene structure is constructed by using ALN which performs dynamic alignment of known GPCR and genome sequence by considering exon/intron boundary.

    Candidate sequences selected by the above process still contain the following redundancies. (1) Perfect matches or overlaps at the same genomic position (chromosome number, relative position on the genome). We regarded them as the same gene and adjusted the double count accordingly. (2) Multiple sequence copies in different genomic positions. We regarded them as different genes. (3) Separate sequence fragments linked by a known protein sequence. They originate in an erroneous prediction by the gene finding programs. We merged them using the linker sequence.
    These redundancies were detected by the following clustering method for each level. First, Swith-Waterman sequence alignment was applied to the candidate sequences in an all-against-all fashion. Then sequences were linked together only when they hit for more than 50 amino acids with more than 95% identity, and shared the same chromosome number and overlapping genomic position. If chromosome numbers were unknown for (either/both) sequences, they were linked with more than 99% identity. After computing transitive closures of the links, each of the known human GPCR sequences from the Swiss-Prot was aligned against all the candidate sequences. All clusters that hit for more than 50 amino acids with more than 99% identity were merged. Finally, in each cluster, the longest sequence was selected as the representative.


  • ALN
  •  (Gotoh,O. Bioinformatics 16(3),190-202(2000))

    Using a new convention for encoding a DNA sequence into a series of 23 possible letters, a dynamic programming algorithm ('aln' written in ANSI-C) was developed to align a DNA sequence and a protein sequence or profile so that the spliced and translated sequence optimally matches the reference the same as the standard protein sequence alignment allowing for long gaps. The objective function also takes account of frame shift errors, coding potentials, and translation initiation, termination and splicing signals. This method was tested on Caenorhabditis elegans genes of known structures. The accuracy of prediction measured in terms of a correlation coefficient was about 95% at the nucleotide level for the 288 genes tested, and 97.0% for the 170 genes whose product and closest homologue share more than 30% identical amino acids.


    (2) Gene screening stage:

    Each analysis tool was first assessed to determine two threshold settings, best specificity and best sensitivity, with a reference dataset: GPCR sequences and non-GPCR sequences in the Swiss-Prot database. The best specificity threshold is intended to achieve, when applied to the reference dataset, almost 100% specificity and with minimum false-negatives. On the other hand, the best sensitivity threshold is intended to achieve almost 100% sensitivity and with minimum false-positives.
    Using the thresholds shown in Table 1, those GPCR candidates were selected that showed significant sequence similarity or contained characteristic motifs and domains, and transmembrane helices.
    Four confidence levels of the datasets were determined by combining the best specificity and best sensitivity thresholds. Level A data, expected to show the best specificity, were obtained by adding the candidate sequences given by best specificity thresholds of the sequence similarity search, motif- and domain assignments. To discover remote GPCR homologues, we combined candidates from the three-level thresholds for TMH prediction (see Table 1) with the sequences that were obtained by the best sensitivity thresholds of sequence search and motif- and domain assignment, and level D data are expected to show the best sensitivity.


    Table 1. Thresholds used for GPCR discovery.
      Level A
    (Best specificity)
    Level B Level C Level D
    (Best sensitivity)
    Sequence search
    with BLASTP
    E < 10-80 E < 10-30 E < 10-30 E < 10-30
    Domain assignment
    with Pfam
    E < 10-10 E < 1.0 E < 1.0 E < 1.0
    Motif assignment
    with PROSITE
    Not used Match Match Match
    TMH Prediction Not used TMwindows(7)
    AND
    SOSUI(7)
    TMwindows(7)
    AND
    SOSUI(6-8)
    TMwindows(7)
    OR
    SOSUI(7)
    Sensitivity 99.4% 99.8% 99.9% 99.9%
    Specificity 96.6% 70.0% 48.4% 20.0%

    Thresholds of the programs are shown.

    Using BLASTP (Altschul, S. F., et al Nucleic Acids Res.25,3389-3402 (1997)) known GPCR seguences were searched against the reference dataset, and the sensitivity and specificity of E values were computed for discriminating correct pairs.
    Using HMMER (Bateman, A., Birney, E., Durbin, R., Eddy, S. R., Howe, K, L. & Sonnhammer, E. L. Nucleic Acids Res.28,263-266 (2000).), GPCR specific Hidden Markov Models ( Pfam domain ) were assigned to reference sequences, and the sensitivity and specificity of E values were computed for correct assignment.
    Since PROSITE patterns are written by regular expression, we determined the P value, which is calculated as the multiplication of each residue frequency in the Swiss-Prot database; the sensitivity and specificity of P values were computed for correct assignment.
    For TMH prediction we used the TMwindows program, our original program along with the SOSUI . We treated the results as GPCR outputs when the predicted helix number was dispersed between n and m. Here we used n-m ranges 7-7, 6 -8, 5-9, and 4-10 and combined the sequences obtained from each range of the two programs. For example, the descriptor {TMwindows(7) OR SOSUI(6-8) } unifies ("OR"), the sequences within range 7-7 that were obtained by TMwindows and the sequences within range 6-8 that were obtained by SOSUI.


  • SOSUI

  • A useful tool for secondary structure prediction of membrane proteins from a protein sequence. The basic idea of prediction in this system is based on the physicochemical properties of amino acid sequences such as hydrophobicity and charges. The system deals with three types of prediction: discrimination of membrane proteins from soluble ones, prediction of the existence of transmembrane helices and determination of transmembrane helical regions.
    (Hirokawa, T., Boon-Chieng, S. & Mitaku, S. Bioinformatics.14,378-379 (1998).)


  • TMwindows

  • Predicts transmembrane helices by the following procedures.
    (1) It assigns the Engelman-Steitz-Goldman (Annual Review of Biophysics and Biophysical Chemistry.15,321-353 (1986).) hydropathy index to amino acid sequences and calculates average hydrophobicity within a pre-determined window. The index was selected, after comparing all indices in the AAindex database (Protein Eng. 9, 27-36 (1996). as the most powerful for discriminating membrane proteins from others using total average hydrophobicity.
    (2) The window size is changed from 19 to 27 and if the average hydrophobicity within each window exceeds 2.5, the region is regarded as a transmembrane helix. The total number of helices computed for each window size gives the range of predicted helix number.


    (3) Databases used for analysis:

    Genome DataBases
    Homo sapiensUCSC hg18
    Pan troglodytesUCSC panTro2
    Gorilla gorillaEnsembl 1.56
    Pongo abeliiUCSC ponAbe2
    Papio hamadryasBaylor College of Medicine 2008/11/20
    Rhesus macaqueUCSC rheMac2
    Microcebus murinusEnsembl 1.56
    Tarsius syrichtaEnsembl 1.56
    Callithrix jacchusUCSC calJac1
    Ottolemur garnettiUCSC otoGar1
    Tupaia belangeriUCSC tupBel1
    Erinaceus europaeuUCSC eriEur1
    Sorex araneusUCSC sorAra1
    Echinops telfairiUCSC echTel1
    Cavia porcellusUCSC cavPor2
    Rattus norvegicusUCSC rn4
    Mus musculusUCSC mm9
    Spermophilus tridecemlineatusBroad Institute speTri1
    Procavia capensisEnsembl 1.56
    Pteropus vampyrusEnsembl 1.56
    Myotis lucifugusEnsembl 1.56
    Canis familiarisUCSC canFam2
    Felis catusUCSC felCat3
    Bos taurusUCSC bosTau3
    Vicugna pacosEnsembl 1.56
    Tursiops truncatusBaylor College of Medicine 2007/04/19
    Oryctolagus cuniculusUCSC oryCun1
    Ochotona princepsBroad Institute OchPri2.0
    Loxodonta africanaUCSC loxAfr1
    Dasypus novemcinctusUCSC dasNov1
    Monodelphis domesticaUCSC monDom5
    Macropus eugeniiEnsembl 1.56
    Ornithorhynchus anatinusUCSC ornAna1
    Gallus gallusUCSC galGal3
    Taeniopygia guttataUCSC taeGut1
    Anolis carolinensisUCSC anoCar1
    Xenopus tropicalisUCSC xenTro2
    Oryzias latipesUCSC oryLat1
    Gasterosteus aculeatusUCSC gasAcu1
    Tetraodon nigroviridisUCSC tetNig1
    Fugu rubripesUCSC fr2
    Danio rerioUCSC danRer5
    Petromyzon marinusUCSC petMar1
    Ciona intestinalisUCSC ci2
    Drosophila melanogasterUCSC dm3
    Drosophila simulansUCSC droSim1
    Drosophila yakubaUCSC droYak2
    Anopheles gambiaeUCSC anoGam1
    Caenorhabditis elegansUCSC ce4
    Caenorhabditis remaneiUCSC caeRem2
    Caenorhabditis brenneriUCSC caePb1
    Caenorhabditis briggsaeUCSC cb3
    Arabidopsis thalianaNCBI 2000/12/14
    Oryza sativaIRGSP build 4.0
    Dictyostelium discoideumdictyBase 2007/12/11
    Saccharomyces cerevisiaeUCSC sacCer1
    Sequence DataBases
    Swiss-Prot ver.54.2
    GPCRDB release 10.0
    nr.aa release at 2007/10/25
    UniGene release at 2007/10/25
    Sequence DataBases
    Pfam release 22.0
    PROSITE release 20.19

    Comments or questions to m-suwa@aist.go.jp
    Recent Revise on 2010/04/27.