The Evolutionarily Conserved Core Design of the Catalytic Activation Step of the Yeast Spliceosome

2009 | journal article. A publication with affiliation to the University of Göttingen.

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​The Evolutionarily Conserved Core Design of the Catalytic Activation Step of the Yeast Spliceosome​
Fabrizio, P.; Dannenberg, J. ; Dube, P.; Kastner, B.; Stark, H. ; Urlaub, H.   & Lührmann, R. ​ (2009) 
Molecular Cell36(4) pp. 593​-608​.​ DOI: https://doi.org/10.1016/j.molcel.2009.09.040 

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Authors
Fabrizio, Patrizia; Dannenberg, Julia ; Dube, Prakash; Kastner, Berthold; Stark, Holger ; Urlaub, Henning ; Lührmann, Reinhard 
Abstract
Metazoan spliceosomes exhibit an elaborate protein composition required for canonical and alternative splicing. Thus, the minimal set of proteins essential for activation and catalysis remains elusive. We therefore purified in vitro assembled, precatalytic spliceosomal complex B, activated Bact, and step 1 complex C from the simple eukaryote Saccharomyces cerevisiae. Mass spectrometry revealed that yeast spliceosomes contain fewer proteins than metazoans and that each functional stage is very homogeneous. Dramatic compositional changes convert B to Bact, which is composed of similar to 40 evolutionarily conserved proteins that organize the catalytic core. Additional remodeling occurs concomitant with step 1, during which nine proteins are recruited to form complex C. The moderate number of proteins recruited to complex C will allow investigations of the chemical reactions in a fully defined system. Electron microscopy reveals high-quality images of yeast spliceosomes at defined functional stages, indicating that they are well-suited for three-dimensional structure analyses.
Issue Date
2009
Status
published
Publisher
Cell Press
Journal
Molecular Cell 
ISSN
1097-2765
Sponsor
European Commission [EURASNET-518238]; Ernst Jung Stiftung

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