Affinity proteomic dissection of the human nuclear cap-binding complex interactome

  • Yuhui Dou
  • , Svetlana Kalmykova
  • , Maria Pashkova
  • , Mehrnoosh Oghbaie
  • , Hua Jiang
  • , Kelly R. Molloy
  • , Brian T. Chait
  • , Michael P. Rout
  • , David Fenyo
  • , Torben Heick Jensen
  • , Ilya Altukhov
  • , John LaCava*
  • *Corresponding author for this work

    Research output: Contribution to journalArticleAcademicpeer-review

    22 Citations (Scopus)
    118 Downloads (Pure)

    Abstract

    A 5',7-methylguanosine cap is a quintessential feature of RNA polymerase II-transcribed RNAs, and a textbook aspect of co-transcriptional RNA processing. The cap is bound by the cap-binding complex (CBC), canonically consisting of nuclear cap-binding proteins 1 and 2 (NCBP1/2). Interest in the CBC has recently renewed due to its participation in RNA-fate decisions via interactions with RNA productive factors as well as with adapters of the degradative RNA exosome. A novel cap-binding protein, NCBP3, was recently proposed to form an alternative CBC together with NCBP1, and to interact with the canonical CBC along with the protein SRRT. The theme of post-transcriptional RNA fate, and how it relates to co-transcriptional ribonucleoprotein assembly, is abundant with complicated, ambiguous, and likely incomplete models. In an effort to clarify the compositions of NCBP1-, 2- and 3-related macromolecular assemblies, we have applied an affinity capture-based interactome screen where the experimental design and data processing have been modified to quantitatively identify interactome differences between targets under a range of experimental conditions. This study generated a comprehensive view of NCBP-protein interactions in the ribonucleoprotein context and demonstrates the potential of our approach to benefit the interpretation of complex biological pathways.

    Original languageEnglish
    Pages (from-to)10456-10469
    Number of pages14
    JournalNucleic Acids Research
    Volume48
    Issue number18
    DOIs
    Publication statusPublished - 9-Oct-2020

    Keywords

    • RNA EXPORT PROTEINS
    • CRYO-EM STRUCTURE
    • MESSENGER-RNA
    • MASS-SPECTROMETRY
    • COMPUTATIONAL PLATFORM
    • SPLICEOSOME
    • CBC
    • IDENTIFICATION
    • PURIFICATION
    • EXPLORATION

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