Real-Time PCR-Coupled CE-SELEX for DNA Aptamer Selection
Author(s) -
Patrick Ruff,
Rekha Pai,
Francesca Storici
Publication year - 2012
Publication title -
isrn molecular biology
Language(s) - English
Resource type - Journals
ISSN - 2090-7907
DOI - 10.5402/2012/939083
Subject(s) - aptamer , systematic evolution of ligands by exponential enrichment , capillary electrophoresis , nucleic acid , dna , computational biology , chemistry , selex aptamer technique , oligonucleotide , microbiology and biotechnology , biology , biochemistry , rna , gene
Aptamers are short nucleic acid or peptide sequences capable of binding to a target molecule with high specificity and affinity. Also known as “artificial antibodies,” aptamers provide many advantages over antibodies. One of the major hurdles to aptamer isolation is the initial time and effort needed for selection. The systematic evolution of ligands by exponential enrichment (SELEX) is the traditional procedure for generating aptamers, but this process is lengthy and requires a large quantity of target and starting aptamer library. A relatively new procedure for generating aptamers using capillary electrophoresis (CE), known as CE-SELEX, is faster and more efficient than SELEX but requires laser-induced fluorescence (LIF) to detect the aptamer-target complexes. Here, we implemented an alternative system without LIF using real-time- (RT-) PCR to indirectly measure aptamer-target complexes. In three rounds of selection, as opposed to ten or more rounds common in SELEX protocols, a specific aptamer for bovine serum albumin (BSA) was obtained. The specificity of the aptamer to BSA was confirmed by electrophoretic mobility shift assays (EMSAs), an unlabeled competitor assay, and by a supershift assay. The system used here provides a cost effective and a highly efficient means of generating aptamers.
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