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Non-radioactive detection of trinucleotide repeat size variability.

PLoS currents (2014-03-13)
Stéphanie Tomé, Annie Nicole, Mario Gomes-Pereira, Genevieve Gourdon
ABSTRACT

Many human diseases are associated with the abnormal expansion of unstable trinucleotide repeat sequences. The mechanisms of trinucleotide repeat size mutation have not been fully dissected, and their understanding must be grounded on the detailed analysis of repeat size distributions in human tissues and animal models. Small-pool PCR (SP-PCR) is a robust, highly sensitive and efficient PCR-based approach to assess the levels of repeat size variation, providing both quantitative and qualitative data. The method relies on the amplification of a very low number of DNA molecules, through sucessive dilution of a stock genomic DNA solution. Radioactive Southern blot hybridization is sensitive enough to detect SP-PCR products derived from single template molecules, separated by agarose gel electrophoresis and transferred onto DNA membranes. We describe a variation of the detection method that uses digoxigenin-labelled locked nucleic acid probes. This protocol keeps the sensitivity of the original method, while eliminating the health risks associated with the manipulation of radiolabelled probes, and the burden associated with their regulation, manipulation and waste disposal.

MATERIALS
Product Number
Brand
Product Description

Roche
DNA Molecular Weight Marker VI, DIG-labeled, solution, pkg of 500 μL (10 μg/ml)
Roche
Anti-Digoxigenin-AP, Fab fragments, from sheep
Roche
Blocking Reagent, For nucleic acid hybridization and detection
Roche
DNA Molecular Weight Marker III, DIG-labeled, 10 μg/mL, pkg of 500 μL (10 μg/ml), solution