"Structure-function Analysis Of The 5? End Of Yeast U1 SnRNA Highlights Genetic Interactions With The Msl5oMud2 Branchpoint-binding Complex And Other Spliceosome Assembly Factors." - Information and Links:

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"Structure-function Analysis Of The 5? End Of Yeast U1 SnRNA Highlights Genetic Interactions With The Msl5oMud2 Branchpoint-binding Complex And Other Spliceosome Assembly Factors." and the language of the book is English.


“Structure-function Analysis Of The 5? End Of Yeast U1 SnRNA Highlights Genetic Interactions With The Msl5oMud2 Branchpoint-binding Complex And Other Spliceosome Assembly Factors.” Metadata:

  • Title: ➤  Structure-function Analysis Of The 5? End Of Yeast U1 SnRNA Highlights Genetic Interactions With The Msl5oMud2 Branchpoint-binding Complex And Other Spliceosome Assembly Factors.
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  • Language: English

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  • Internet Archive ID: pubmed-PMC3753624

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This article is from <a href="//archive.org/search.php?query=journaltitle%3A%28Nucleic%20Acids%20Research%29" rel="ugc nofollow">Nucleic Acids Research</a>, <a href="//archive.org/search.php?query=journaltitle%3A%28Nucleic%20Acids%20Research%29%20AND%20volume%3A%2841%29" rel="ugc nofollow">volume 41</a>.<h2>Abstract</h2>Yeast pre-mRNA splicing initiates via formation of a complex comprising U1 snRNP bound at the 5′ splice site (5′SS) and the Msl5•Mud2 heterodimer engaged at the branchpoint (BP). Here, we present a mutational analysis of the U1 snRNA, which shows that although enlarging the 5′ leader between the TMG cap and the 3ACUUAC8 motif that anneals to the 5′SS is tolerated, there are tight constraints on the downstream spacer between 3ACUUAC8 and helix 1 of the U1 fold. We exploit U1 alleles with 5′ extensions, variations in the 3ACUUAC8 motif, downstream mutations and a longer helix 1 to discover new intra-snRNP synergies with U1 subunits Nam8 and Mud1 and the trimethylguanosine (TMG) cap. We describe novel mutations in U1 snRNA that bypass the essentiality of the DEAD-box protein Prp28. Structure-guided mutagenesis of Msl5 distinguished four essential amino acids that contact the BP sequence from nine other BP-binding residues that are inessential. We report new synthetic genetic interactions of the U1 snRNP with Msl5 and Mud2 and with the nuclear cap-binding subunit Cbc2. Our results fortify the idea that spliceosome assembly can occur via distinct genetically buffered microscopic pathways involving cross-intron-bridging interactions of the U1 snRNP•5′SS complex with the Mud2•Msl5•BP complex.

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