PLoS genetics, 2009-11, Vol.5 (11), p.e1000707-e1000707
2009
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Details
- Autor(en) / Beteiligte
- Titel
- The germ cell nuclear proteins hnRNP G-T and RBMY activate a testis-specific exon
- Ist Teil von
- PLoS genetics, 2009-11, Vol.5 (11), p.e1000707-e1000707
- Ort / Verlag
- United States: Public Library of Science
- Erscheinungsjahr
- 2009
- Quelle
- MEDLINE
- Beschreibungen/Notizen
- The human testis has almost as high a frequency of alternative splicing events as brain. While not as extensively studied as brain, a few candidate testis-specific splicing regulator proteins have been identified, including the nuclear RNA binding proteins RBMY and hnRNP G-T, which are germ cell-specific versions of the somatically expressed hnRNP G protein and are highly conserved in mammals. The splicing activator protein Tra2beta is also highly expressed in the testis and physically interacts with these hnRNP G family proteins. In this study, we identified a novel testis-specific cassette exon TLE4-T within intron 6 of the human transducing-like enhancer of split 4 (TLE4) gene which makes a more transcriptionally repressive TLE4 protein isoform. TLE4-T splicing is normally repressed in somatic cells because of a weak 5' splice site and surrounding splicing-repressive intronic regions. TLE4-T RNA pulls down Tra2beta and hnRNP G proteins which activate its inclusion. The germ cell-specific RBMY and hnRNP G-T proteins were more efficient in stimulating TLE4-T incorporation than somatically expressed hnRNP G protein. Tra2b bound moderately to TLE4-T RNA, but more strongly to upstream sites to potently activate an alternative 3' splice site normally weakly selected in the testis. Co-expression of Tra2beta with either hnRNP G-T or RBMY re-established the normal testis physiological splicing pattern of this exon. Although they can directly bind pre-mRNA sequences around the TLE4-T exon, RBMY and hnRNP G-T function as efficient germ cell-specific splicing co-activators of TLE4-T. Our study indicates a delicate balance between the activity of positive and negative splicing regulators combinatorially controls physiological splicing inclusion of exon TLE4-T and leads to modulation of signalling pathways in the testis. In addition, we identified a high-affinity binding site for hnRNP G-T protein, showing it is also a sequence-specific RNA binding protein.
- Sprache
- Englisch
- Identifikatoren
- ISSN: 1553-7404, 1553-7390eISSN: 1553-7404DOI: 10.1371/journal.pgen.1000707Titel-ID: cdi_plos_journals_1313510807
- Format
- –
- Schlagworte
- Alternative Splicing, Amino Acid Sequence, Animals, Anopheles, Base Sequence, Binding sites, Cell Biology/Gene Expression, Cell Line, Developmental Biology/Germ Cells, Exons, G proteins, Gene expression, Genetics, Heterogeneous-Nuclear Ribonucleoproteins - metabolism, Humans, Introns, Life Sciences, Male, Messenger RNA, Molecular Biology/RNA Splicing, Molecular Sequence Data, Nuclear Proteins - chemistry, Nuclear Proteins - genetics, Nuclear Proteins - metabolism, Physiological aspects, Protein Binding, Protein Isoforms - genetics, Protein Isoforms - metabolism, Proteins, Repressor Proteins - chemistry, Repressor Proteins - genetics, Repressor Proteins - metabolism, Ribonucleic acid, RNA, RNA-Binding Proteins - metabolism, Spermatozoa - metabolism, Testis - metabolism, Zebrafish - embryology, Zebrafish - genetics, Zebrafish - metabolism