Difference between revisions of "MSigDB v3.0 Release Notes"

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Major changes in Release 3.0 of the Molecular Signatures Database (MSigDB) include the following:

• removed all gene sets with fewer than ten (C1, C2:CP, C3-C5) or five (C2:CGP) human gene symbols
• C2 collection: extensively reviewed and added many new gene sets as detailed below
• gene families: updated and added new gene families
• MSigDB gene sets now support human Entrez Gene IDs
• enhanced features in the MSigDB XML file format
• fixed a bug in the Compute Overlaps algorithm
• archived MSigDB v2.5 files
• changes in gene set names are documented here

Gene Sets Update

The following describes the changes made to the gene set collections for MSigDB v3.0.

Size Filtering

After mapping to human Entrez Gene IDs, sets with fewer than five genes were not included in the v3.0 release.

C1: Positional gene sets (-60)

• 60 gene sets have been deprecated due to small size (fewer than five human Entrez Gene IDs).

No other changes were made in the C1 gene sets. For a description of this collection, see the <a href="http://www.broad.mit.edu/gsea/msigdb/collections.jsp">Browse Collections</a> page. 

C2: Curated gene sets (+1,380)

The C2 collection consists of gene sets collected from various sources such as online pathway databases, publications in PubMed, and knowledge of domain experts.  Gene sets in this collection have been extensively revised and expanded.
Note that all the gene set names for C2 have changed.  Many of the names used in v2.5 were confusing or wrong, so these have been clarified or corrected.  For CGP, the new naming convention is that all gene set names begin with the surname of the first author of the source paper.  For CP, the names now begin with the contributor organization.

• CGP: chemical and genetic perturbations (2,392 gene sets). See <a href="http://www.broadinstitute.org/cancer/software/gsea/wiki/index.php/Msigdb_mapping_v2.5_to_v3">this page</a> for information about MSigDB 2.5 gene sets that have been renamed, retired, recombined, or replaced in the MSigDB 3.0 release.  All these gene sets have been verified against the original sources.  During the reviewing process, we have:
  • renamed gene sets to follow consistent conventions throughout the whole collection
  • wrote new, enhanced, brief descriptions according to consistent conventions throughout the whole collection
  • validated and corrected, if necessary, every attribute for each existing gene set
  • added the exact source of the gene set (e.g., Table 1)
  • added GEO or ArrayExpress ID when available
  • added links to human Entrez Gene entries and PubChem Compound entries as appropriate
  • used the original gene identifiers as reported in the source paper (not all gene sets did this originally)
    
  • resolved cases of redundant gene sets
  In addition, we made an aggressive effort to identify new gene sets and add them to the database, using the same stringent set of criteria for reviewing these new additions.
• CP: canonical pathways (880 gene sets).
  • We have deprecated all gene sets:
    • from GenMAPP gene sets because the majority of them in the previous release are based on KEGG or GO information that we already have
    • from GO in this collection because they are already represented by C5
    • based on NetAffx annotations because these are largely based on GO and thus are already represented by C5
    • with untraceable origins
  • We have replaced all existing BioCarta and KEGG gene sets with updated versions from these resources.
  • In collaboration with Reactome, we added 430 new canonical pathway sets
  • To reduce redundancy in canonical pathways from BioCarta, KEGG, and Reactome, we developed and applied the following filters:
    • Source priority: KEGG > Reactome > BioCarta
    • Size priority: keep the set with the smaller size
    • Name length priority: keep the set with the shorter name
    • External ID priority: keep the set with the smaller ID (applied to Reactome sets only)
  • For convenience, we have organized gene sets from BioCarta, KEGG, and Reactome as separate, third-level divisions within C2:CP

C3: Motif gene sets (-1)

• Thanks to a sharp user, we fixed an error in the description of the gene set "V$NRF2_01".
• All uncategorized gene sets in this collection have been assigned to the TFT subcollection.
• One gene set in the MIR subcollection has been deprecated due to small size (less than five human Entrez Gene IDs).
• No other changes were made in the C3 gene sets.

Gene sets in the C3 collection consist of genes sharing a cis-regulatory motif. This collection contains the following two subcollections:

Transcription factor targets (TFT)

These sets share upstream cis-regulatory motifs which can function as potential transcripton factor binding sites. We used two approaches to generate these gene sets.

We extracted 460 mammalian transcriptional regulatory motifs from v7.4 TRANSFAC database. We then generated the motif gene sets consisting of the inferred target genes for each motif. Every such set consists of human genes whose promoters (defined as regions -2kb to +2kb around transcription start site) contain at least one instance of the motif. We named these sets by the corresponding TRANSFAC matrix identifiers, e.g., V$MIF1_01. The set’s full description is the TRANSFAC entry for the matching matrix, in a format described here.

Motif gene sets of ‘conserved instances’ consist of the inferred target genes for each motif m of 174 upstream motifs highly conserved among five mammalian species. The motifs are catalogued in Xie, et al. (2005, Nature 434, 338–345) and represent potential transcription factor binding sites. Each motif gene set consists of all human genes whose promoters (defined as regions -kb to +2kb around transcription start site) contained at least one conserved instance of motif m. If the motif’s sequence matched a transcription factor binding site documented in the TRANSFAC database (see above), then we appended the name of the TRANSFAC binding matrix to the motif sequence in the gene name, e.g.: MOTIFSEQ_FOO, where MOTIFSEQ is the sequence of motif m and FOO is the TRANSFAC matrix name (e.g., V$MIF1_01). The set’s full description in this case is the TRANSFAC entry for the matching matrix. If the motif’s sequence matched no transcription factor binding site from TRANSFAC v.7.4, then we named the set as MOTIFSEQ_UNKNOWN where MOTIFSEQ is the sequence of motif m.

microRNA Targets (MIR)

These gene sets consist of the inferred target gene for each motif m of 221 3'-UTR motifs highly conserved among five mammalian species. The motifs are catalogued catalogued in Xie, et al. 2005, Nature 434, 338–345 and represent potential microRNA binding sites. Each motif gene set consists of all genes whose 3’-UTR contained at least one conserved instance of motif m.

C4: Computational gene sets (-2)

• Two gene sets in the CM subcollection have been deprecated due to small size (fewer than five human Entrez Gene IDs).

No other changes were made in the C4 gene sets. For a description of this collection, see the <a href="http://www.broad.mit.edu/gsea/msigdb/collections.jsp">Browse Collections</a> page.

Cancer gene neighborhoods (CGN)

Starting with a curated list of 380 cancer-associated genes (Brentani et al. 2003, Proc. Natl. Acad. Sci. USA 100, 13418-13423), Subramanian, Tamayo et al. (2005 Proc. Natl. Acad. Sci. USA 102, 15545-15550) mined four expression compendia for correlated gene sets. Gene neighborhoods with fewer than 25 genes at a Pearson correlation threshold of 0.8 were omitted yielding 427 sets.

Gene set names indicate the corresponding expression compendia and the seed cancer-associated genes.