Use of a competitive probe in assay design for genotyping of the UGT1A1*28 microsatellite polymorphism by the smart amplification process
Author(s) -
Jun Watanabe,
Yasumasa Mitani,
Yuki Kawai,
Takeshi Kikuchi,
Yasushi Kogo,
Atsuko Oguchi-Katayama,
Hajime Kanamori,
Kengo Usui,
Masayoshi Itoh,
Paul E. Cizdziel,
Alexander Lezhava,
Kenji Tatsumi,
Yasushi Ichikawa,
Shinji Togo,
Hiroshi Shimada,
Yoshihide Hayashizaki
Publication year - 2007
Publication title -
biotechniques
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.617
H-Index - 131
eISSN - 1940-9818
pISSN - 0736-6205
DOI - 10.2144/000112563
Subject(s) - genotyping , biology , microsatellite , thermus aquaticus , taq polymerase , microbiology and biotechnology , genotype , genetics , polymerase chain reaction , primer (cosmetics) , allele , chemistry , gene , organic chemistry
A key feature of the smart amplification process version 2 (SMAP-2) is the ability to suppress mismatch amplification by using a unique asymmetric primer design and Thermus aquaticus MutS (Taq MutS). However we report here that use of SMAP-2 for polymorphism determination of the UGT1A1 *28 allele required a further ancillary approach for complete background suppression. The UGT1A1 *28 allele is a microsatellite copy number polymorphism. This is the first reported SMAP-2 assay designed for genotyping genetic variations of microsatellites. We found that by the addition of a primer to the amplification reaction, called a competitive probe (CP), assay specificity could be significantly enhanced. Including sample preparation time and use of a CP-enhanced SMAP-2 assay, we could rapidly detect the UGT1A1 *28 polymorphism within 60 min. To test our method, we compared results from PCR sequencing and the CP-enhanced SMAP-2 assay on 116 human blood samples for UGT1A1 *28 polymorphism and demonstrated perfect concordance. These results illustrate the versatility of SMAP-2 for molecular diagnostics and provide a new approach for enhancing SMAP-2 assay specificity.
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