Multiplex genotyping of PCR products with MassTag-labeled primers.

AUTOR(ES)

Haff, L A

RESUMO

A simple mass spectrometric based assay, the PinPoint assay, has previously been described for typing single nucleotide polymorphisms. The identity of a polymorphism is determined by mass differences of single base extended genotyping primers as determined by MALDI-TOF mass spectrometry. A simple method for multiplexing the assay is described, employing multiple primers with 5'oligo(dT) sequences (MassTags) which serve to mass discriminate the peaks of multiple extended and non-extended primers. The assay is extremely rapid and requires no labeling reagents.

Documentos Relacionados

• PCR with detachable primers.
• Multiplex quantitative PCR using self-quenched primers labeled with a single fluorophore
• Fingerprinting genomes using PCR with arbitrary primers.
• High-Throughput SNP Genotyping by Allele-Specific PCR with Universal Energy-Transfer-Labeled Primers
• Rapid sequencing of unpurified PCR products by thermal asymmetric PCR cycle sequencing using unlabeled sequencing primers.