Single base pair mutation analysis by PNA directed PCR clamping

doi:10.1093/nar/21.23.5332

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Nucleic Acids Research, 1993, Vol. 21, No. 23 5332-5336
© 1993

METHODS

Single base pair mutation analysis by PNA directed PCR clamping

Henrik Ørum^*, Peter E. Nielsen¹^,*, Michael Egholm², Rolf H. Berg³, Ole Buchardt³ and Christopher Stanley^*

PNA Diagnostics A/;S Lersø Park Alle 42, DK-2100 Copenhagen ø ¹Research Center for Medical Biotechnology, Department of Biochemistry B The Panum Institute, Blegdamsvej 3C, DK-2200 Copenhagen N ²Department of Organic Chemistry, The H.C.sted Institute Universitetsparken 5, DK 2100 Copenhagen Ø ³Polymer Group, Materials Department, Risp National Laboratory DK-4000 Roskilde, Denmark

^*To whom correspondence should be addressed

Received September 16, 1993. Revised October 19, 1993. Accepted October 19, 1993.

A novel method that allows direct analysis of single base mutationby the polymerase chain reaction (PCR) is described. The methodutilizes the finding that PNAs (peptide nucleic acids) recognizeand bind to their complementary nucleic acid sequences withhigher thermal stability and specificity than the correspondingdeoxyribooligonucleotides and that they cannot function as primersfor DNA polymerases. We show that a PNA/DNA complex can effectivelyblock the formation of a PCR product when the PNA is targetedagainst one of the PCR primer sites. Furthermore, we demonstratethat this blockage allows selective amplification/suppressionof target sequences that differ by only one base pair. Finallywe show that PNAs can be designed in such a way that blockagecan be accomplished when the PNA target sequence is locatedbetween the PCR primers.

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