BioTechniques (Oct 2002)

Mammalian Expression Cloning of Nucleic Acid Binding Proteins by Agarose Thin-Layer Gelshift Clone Selection

  • A. Dobi,
  • W. Debnam,
  • C. Dalgard,
  • A. Owusu,
  • D.v. Agoston

DOI
https://doi.org/10.2144/02334rr03
Journal volume & issue
Vol. 33, no. 4
pp. 868 – 872

Abstract

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Here we report a functional screening technique to identify cDNAs encoding mammalian nucleic acid binding proteins. We have combined cDNA expression cloning with the agarose thin-layer gelshift assay technique to detect specific nucleic acid binding proteins from a mammalian expression library. We divided this cDNA expression library into multiple pools and transfected mammalian cells with the individual pools. Following transfection, we tested the expressed proteins for DNA-binding activity by agarose thin-layer electrophoretic gelshift assay. After we identified a single expression pool for the presence of a DNA-binding protein, the corresponding cDNA pool was further divided into smaller aliquots. Then, the cDNA expression and gelshift clone selection was repeated until a single clone was isolated. In contrast to traditional polyacrylamide gels, the agarose thin-layer is significantly faster and resolves larger DNA-protein complexes. This method can be widely used for the cDNA cloning of DNA- and RNA-binding proteins from various mammalian host cells.