BioTechniques (Jun 1999)

Fast and Reliable Screening of Mutations in Human Tumors: Use of Multiple Fluorescence-Based Long Linker Arm Nucleotides Assay (mf-LLA)

  • L.A. Marcelino,
  • M. Galvin,
  • G.M. Martins,
  • M.J. Proença,
  • E. Mayrand,
  • J.A. Rueff,
  • C.J. Monteiro

DOI
https://doi.org/10.2144/99266rr01
Journal volume & issue
Vol. 26, no. 6
pp. 1134 – 1148

Abstract

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Human tumor samples were screened for point mutations by adapting a mobilityshift assay to automated DNA sizing. This screen identifies the type of point mutation and relative amount of mutated DNA sequences present in a sample. Test samples having known hypoxanthine-guanine phosphoribosyl transferase (hprt)/exon-3 sequence mutations were characterized by: (i) PCR amplification, (ii) fluorescent dyeprimer extension with 36-atom linker derived deoxycytosine or deoxyuridine triphosphate and the remaining three natural nucleotides and (iii) sizing of the resulting fluorescently labeled modified strands, using an automated DNA sequencer. Routinely, a range of sizes is observed among the sequence variants of a single DNA target sequence. This is because nucleotide analogs are incorporated into DNA strands in a sequence-dependent manner, resulting in composition-dependent electrophoretic mobility. Thus, point mutations are identified as shifts in mobility between the fluorescently labeled modified strands of the control and test samples. The twenty different hprt/exon-3 single-base substitution mutations tested were easily identified, even at fourfold dilution with control DNA.