Scansite 2.0: Proteome-wide prediction of cell signaling interactions using short sequence motifs

JC Obenauer, LC Cantley, MB Yaffe - Nucleic acids research, 2003 - academic.oup.com
Nucleic acids research, 2003academic.oup.com
Scansite identifies short protein sequence motifs that are recognized by modular signaling
domains, phosphorylated by protein Ser/Thr-or Tyr-kinases or mediate specific interactions
with protein or phospholipid ligands. Each sequence motif is represented as a position-
specific scoring matrix (PSSM) based on results from oriented peptide library and phage
display experiments. Predicted domain-motif interactions from Scansite can be sequentially
combined, allowing segments of biological pathways to be constructed in silico. The current …
Abstract
Scansite identifies short protein sequence motifs that are recognized by modular signaling domains, phosphorylated by protein Ser/Thr- or Tyr-kinases or mediate specific interactions with protein or phospholipid ligands. Each sequence motif is represented as a position-specific scoring matrix (PSSM) based on results from oriented peptide library and phage display experiments. Predicted domain-motif interactions from Scansite can be sequentially combined, allowing segments of biological pathways to be constructed in silico. The current release of Scansite, version 2.0, includes 62 motifs characterizing the binding and/or substrate specificities of many families of Ser/Thr- or Tyr-kinases, SH2, SH3, PDZ, 14-3-3 and PTB domains, together with signature motifs for PtdIns(3,4,5)P3-specific PH domains. Scansite 2.0 contains significant improvements to its original interface, including a number of new generalized user features and significantly enhanced performance. Searches of all SWISS-PROT, TrEMBL, Genpept and Ensembl protein database entries are now possible with run times reduced by ∼60% when compared with Scansite version 1.0. Scansite 2.0 allows restricted searching of species-specific proteins, as well as isoelectric point and molecular weight sorting to facilitate comparison of predictions with results from two-dimensional gel electrophoresis experiments. Support for user-defined motifs has been increased, allowing easier input of user-defined matrices and permitting user-defined motifs to be combined with pre-compiled Scansite motifs for dual motif searching. In addition, a new series of Sequence Match programs for non-quantitative user-defined motifs has been implemented. Scansite is available via the World Wide Web at http://scansite.mit.edu.
Oxford University Press