Elsevier

Journal of Biotechnology

Volume 78, Issue 2, 10 March 2000, Pages 201-204
Journal of Biotechnology

Short communication
A simple method for non-radioactive PCR-SSCP using MDE™ gel solution and a midi gel format:: Application for the detection of variants in the GLUT1 and CTLA-4 genes

https://doi.org/10.1016/S0168-1656(99)00241-2Get rights and content

Abstract

The need to identify disease-causing mutations and DNA polymorphisms has increased with the continuing identification of new candidate genes. PCR single-strand conformation polymorphism (PCR-SSCP) is one of the techniques most widely used to identify a mutant sequence or a polymorphism in a known gene. However, the original SSCP protocols using the incorporation of radioactive label and polyacrylamide gel electrophoresis on sequencing gels for detection were labour intensive and time-consuming. Here we describe a simple SSCP protocol using MDE™ gel solution and a midi gel format to detect SSCP variations in the glucose transporter gene GLUT1, that we have previously analysed with the standard radioactive SSCP protocol, and we have also tested this method on the previously described point mutation (A/G transition in exon 1) of the CTLA-4 (cytotoxic T lymphocyte associated-4) gene. All known variants were detected. Based on the results, this technique appears to be simple, with no use of radioactive labels and with easy handling of the gel. Furthermore, it needs little optimisation, is relatively rapid and highly sensitive. We propose this method for the first screening for candidate gene variants.

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Acknowledgements

Financial support to this work was provided by Telethon Italy (grant no. E252) and the Ente Cassa di Risparmio di Roma. We wish to thank Dr G.I. Bell (University of Chicago) for kindly providing the genomic sequence of the human GLUT1 gene.

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