A novel procedure for efficient genotyping of single nucleotide polymorphisms

doi:10.1093/nar/28.5.e13

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Nucleic Acids Research, 2000, Vol. 28, No. 5 E13-e13
© 2000 Oxford University Press

A novel procedure for efficient genotyping of single nucleotide polymorphisms

Sascha Sauer¹^,2, Doris Lechner¹, Kurt Berlin¹, Hans Lehrach¹, Jean-Louis Escary³, Nick Fox⁴ and Ivo Glynne Gut³^,*

¹Max-Planck-Institute for Molecular Genetics, Abteilung Lehrach, Ihnestrasse 73, 14195 Berlin-Dahlem, Germany, ²Freie Universität Berlin, Fachbereich Biologie, Chemie, Pharmazie, Takustrasse 3, 14195 Berlin, Germany, ³Centre National de Génotypage, Batiment G2, 2 rue Gaston Crémieux, CP 5721, 91057 Evry Cedex, France and ⁴Dementia Research Group, The National Hospital for Neurology and Neurosurgery, London WC1N 3BG, UK

Due to the surge in interest in using single nucleotide polymorphisms(SNPs) for genotyping a facile and affordable method for thisis an absolute necessity. Here we introduce a procedure thatcombines an easily automatable single tube sample preparationwith an efficient high throughput mass spectrometric analysistechnique. Known point mutations or single nucleotide polymorphismsare easily analysed by this procedure. It starts with PCR amplificationof a short stretch of genomic DNA, for example an exon of agene containing a SNP. By shrimp alkaline phosphatase digestresidual dNTPs are destroyed. Allele-specific products are generatedusing a special primer, a conditioned set of ${alpha}$ -S-dNTPs and ${alpha}$ -S-ddNTPsand a fresh DNA polymerase in a primer extension reaction. UnmodifiedDNA is removed by 5'-phosphodiesterase digestion and themodified products are alkylated to increase the detection sensitivityin the mass spectrometric analysis. All steps of the preparationare simple additions of solutions and incubations. The procedureoperates at the lowest practical sample volumes and in contrastto other genotyping protocols with mass spectrometric detectionrequires no purification. This reduces the cost and makes iteasy to implement. Here it is demonstrated in a version usingpositive ion detection on described mutations in exon 17 ofthe amyloid precursor protein gene and in a version using negativeion detection on three SNPs of the granulocyte-macrophage colonystimulating factor gene. Preparation and analysis of SNPs isshown separately and simultaneously, thus demonstrating themultiplexibility of this genotyping procedure. The preparationprotocol for genotyping is adapted to the conditions used forthe SNP discovery method by denaturing HPLC, thus demonstratinga facile link between protocols for SNP discovery and SNP genotyping.Results corresponded unanimously with the control sequencing.The procedure is useful for high throughput genotyping as itis required for gene identification and pharmacogenomics wherelarge numbers of DNA samples have to be analysed. We have namedthis procedure the ‘GOOD Assay’ for SNP analysis.

^* To whom correspondence should be addressed. Tel: +33 160 878359; Fax: +33 160 878 383; Email: ivogut@cng.fr

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