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Article
Nature 452, 846-850 (17 April 2008) | doi:10.1038/nature06842; Received 11 December 2007; Accepted 19 February 2008; Published online 5 March 2008
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Isolation of an active step I spliceosome and composition of its RNP core
Sergey Bessonov1, Maria Anokhina1, Cindy L. Will1, Henning Urlaub2 & Reinhard Lührmann1
- Department of Cellular Biochemistry, and,
- Bioanalytical Mass Spectrometry Group, Max Planck Institute of Biophysical Chemistry, D-37077 Göttingen, Germany
Correspondence to: Reinhard Lührmann1 Correspondence and requests for materials should be addressed to R.L. (Email: reinhard.luehrmann@mpi-bpc.mpg.de).
Abstract
Formation of catalytically active RNA structures within the spliceosome requires the assistance of proteins. However, little is known about the number and nature of proteins needed to establish and maintain the spliceosome's active site. Here we affinity-purified human spliceosomal C complexes and show that they catalyse exon ligation in the absence of added factors. Comparisons of the composition of the precatalytic versus the catalytic spliceosome revealed a marked exchange of proteins during the transition from the B to the C complex, with apparent stabilization of Prp19–CDC5 complex proteins and destabilization of SF3a/b proteins. Disruption of purified C complexes led to the isolation of a salt-stable ribonucleoprotein (RNP) core that contained both splicing intermediates and U2, U5 and U6 small nuclear RNA plus predominantly U5 and human Prp19–CDC5 proteins and Prp19-related factors. Our data provide insights into the spliceosome's catalytic RNP domain and indicate a central role for the aforementioned proteins in sustaining its catalytically active structure.
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