The flash-small-pool PCR: how to transform blotting and numerous hybridization steps into a simple denatured PCR

Elodie Dandelot; Geneviève Gourdon

doi:10.2144/btn-2018-0035

BioTechniques (Jun 2018)

The flash-small-pool PCR: how to transform blotting and numerous hybridization steps into a simple denatured PCR

Elodie Dandelot,
Geneviève Gourdon

Affiliations

Elodie Dandelot: 1Laboratory CTGDM, Inserm UMR1163, 75015 Paris, France
Geneviève Gourdon: 1Laboratory CTGDM, Inserm UMR1163, 75015 Paris, France

DOI: https://doi.org/10.2144/btn-2018-0035
Journal volume & issue: Vol. 64, no. 6
pp. 262 – 265

Abstract

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Numerous human diseases are associated with abnormal expansion of unstable trinucleotide repeats (TNRs). TNR instability mechanisms are complex, and remain only partially understood. Small-pool-PCR (SP-PCR) is the reference method to assess TNR instability. SP-PCR amplifies a low number of DNA molecules and is followed by Southern blot. However, SP-PCR remains expensive and time consuming. Here, we describe an optimized SP-PCR that can be done in a day, which reduces cost and experimental biases: the flash-small-pool PCR (FSP-PCR). This method consists of a fluorescent PCR on a few DNA molecules, followed by an alkaline gel electrophoresis revealed with a near infra-red detector system. With reduced experimental steps, cost, and time consumption, microsatellite analysis will become more accessible due to FSP-PCR.

Published in BioTechniques

ISSN: 0736-6205 (Print); 1940-9818 (Online)
Publisher: Taylor & Francis Group
Country of publisher: United Kingdom
LCC subjects: Science: Biology (General)
Website: https://www.tandfonline.com/journals/ibtn20

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