The mRNA-Bound Proteome and Its Global Occupancy Profile on Protein-Coding Transcripts

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• 作者：Alexander  ; G. Baltz¹ ; ³ ; Mathias Munschauer¹ ; ³ ; Bjö ; rn Schwanhä ; usser¹ ; Alexandra Vasile¹ ; Yasuhiro Murakawa¹ ; Markus Schueler¹ ; Noah Youngs² ; Duncan Penfold-Brown² ; Kevin Drew² ; Miha Milek¹ ; Emanuel Wyler¹ ; Richard Bonneau² ; Matthias Selbach¹ ; Christoph Dieterich¹ ; Markus Landthaler¹ ; ^{markus.landthaler@mdc-berlin.de}
• 刊名：Molecular Cell
• 出版年：2012
• 期刊代码：111_10972765
• 类别：bio
• 出版时间：8 June, 2012
• 卷：46
• 期：5
• 页码：674-690
• 文件大小：2152 K

摘要

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Summary

Protein-RNA interactions are fundamental to core biological processes, such as mRNA splicing, localization, degradation, and translation. We developed a photoreactive nucleotide-enhanced UV crosslinking and oligo(dT) purification approach to identify the mRNA-bound proteome using quantitative proteomics and to display the protein occupancy on mRNA transcripts by next-generation sequencing. Application to a human embryonic kidney cell line identified close to 800 proteins. To our knowledge, nearly one-third were not previously annotated as RNA binding, and about 15%were not predictable by computational methods to interact with RNA. Protein occupancy profiling provides a transcriptome-wide catalog of potential cis-regulatory regions on mammalian mRNAs and showed that large stretches in 3鈥?UTRs can be contacted by the mRNA-bound proteome, with numerous putative binding sites in regions harboring disease-associated nucleotide polymorphisms. Our observations indicate the presence of a large number of mRNA binders with diverse molecular functions participating in combinatorial posttranscriptional gene-expression networks.