AI Article Synopsis

  • Cap-binding proteins are typically isolated using m⁷GTP-Sepharose, but this method is not very effective for certain proteins like DcpS due to its interactions and hydrolysis issues.
  • The study introduces new affinity resins, m⁷GpCH₂pp- and m⁷GpCH₂ppA-Sepharoses, designed to resist hydrolysis by DcpS, allowing for more efficient purification.
  • Biochemical tests demonstrated that these novel resins specifically bind cap-binding proteins, including DcpS, highlighting their utility in isolating these proteins for research purposes.

Article Abstract

Cap-binding proteins have been routinely isolated using m⁷GTP-Sepharose; however, this resin is inefficient for proteins such as DcpS (scavenger decapping enzyme), which interacts not only with the 7-methylguanosine, but also with the second cap base. In addition, DcpS purification may be hindered by the reduced resin capacity due to the ability of DcpS to hydrolyze m⁷GTP. Here, we report the synthesis of new affinity resins, m⁷GpCH₂pp- and m⁷GpCH₂ppA-Sepharoses, with attached cap analogs resistant to hydrolysis by DcpS. Biochemical tests showed that these matrices, as well as a hydrolyzable m⁷GpppA-Sepharose, bind recombinant mouse eIF4E²⁸⁻²¹⁷ specifically and at high capacity. In addition, purification of cap-binding proteins from yeast extracts confirmed the presence of all expected cap-binding proteins, including DcpS in the case of m⁷GpCH₂pp- and m⁷GpCH₂ppA-Sepharoses. In contrast, binding studies in vitro demonstrated that recombinant human DcpS efficiently bound only m⁷GpCH₂ppA-Sepharose. Our data prove the applicability of these novel resins, especially m⁷GpCH₂ppA-Sepharose, in biochemical studies such as the isolation and identification of cap-binding proteins from different organisms.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3383972PMC
http://dx.doi.org/10.1261/rna.032078.111DOI Listing

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