The 5' end domain of U2 snRNA is required to establish the interaction of U2 snRNP with U2 auxiliary factor(s) during mammalian spliceosome assembly

doi:10.1093/nar/19.4.877

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Nucleic Acids Research, 1991, Vol. 19, No. 4 877-884
© 1991

MOLECULAR BIOLOGY

The 5' end domain of U2 snRNA is required to establish the interaction of U2 snRNP with U2 auxiliary factor(s) during mammalian spliceosome assembly

Samy Khellil, Marie-Claire Daugeron, Christine Alibert, Philippe Jeanteur, Guy Cathala and Claude Brunel¹^,*

UA CNRS 1191 Génétique Moléculaire', Laboratoire de Biochimie, CRLC Val d'Aurelle-Paul Lamarque, Parc Euromédecine 34094 Montpellier Cedex 2 ¹Laboratoire de Biologie Moléculaire, Université Montpellier II, Sciences et Techniques du Languedoc Place E. Bataillon, CP 012, 34095 Montpellier Cedex 05, France

^* To whom correspondence should be addressed

Received October 15, 1990. Accepted January 25, 1991.

Stable association of U2 snRNP with the branchpoint sequenceof mammalian pre-mRNAs requires binding of a non-snRNP proteinto the polypyrimidine tract. In order to determine how U2 snRNPcontacts this protein, we have used an RNA containing the consensus5' and the (Py)_n 3' splice sites but lacking the branchpointsequence so as to prevent direct U2 snRNA base pairing to thebranchpoint. Different approaches including electrophoreticseparation of RNP complexes formed in nuclear extracts, RNaseT1 protection immunoprecipitation assays with antibodies againstsnRNPs and UV cross-linking experiments coupled to immunoprecipitationsallowed us to demonstrate that at least three splicing factorscontact this RNA at 0°C without ATP. As expected, U1 snRNPinteracts with the region comprising the 5' splice site. A proteinof approximately 65,000 molecular weight recognizes the RNAspecifically at the 5' boundary of the polypyrimidine tract.It could be either the U2 auxiliary factor (U2AF) (Zamore andGreen (1989) PNAS 86, 9243–9247), the polypyrimidine tractbinding protein (pPTB) (Garcia-Blanco et al. (1989) Genes andDev. 3, 1874–1886) or a mixture of both. U2 snRNP alsocontacts the RNA in a way depending on p65 binding, therebyfurther arguing that the latter may correspond to the previouslycharacterized U2AF and pPTB. Cleavage of U2 snRNA sequence bya complementary oligonucleotide and RNase H led us to concludethat the 5' terminus of U2 snRNA is required to ensure the contactbetween U2 snRNP and p65 bound to the RNA. More importantly,this conclusion can be extended to authentic pre-mRNAs. Whenwe have used a human ß-globin pre-mRNA instead ofthe above artificial substrate, RNA bound p65 became precipitableby anti-(U2) RNP and anti-Sm antibodies except when the 5' endof U2 snRNA was selectively cleaved.

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