Your search keyword '"Kentaro Kasai"' showing total 2 results

1. A method to determine the 5' end of the binding site of primers included in a commercially available forensic human identification kit

Author

Natsuko Mizuno, Shota Inokuchi, Koji Fujii, Kentaro Kasai, Tetsushi Kitayama, and Kazumasa Sekiguchi

Subjects

Binding Sites, 5' Flanking Region, Pcr cloning, Electrophoresis, Capillary, Computational biology, Biology, Molecular biology, DNA Fingerprinting, Pathology and Forensic Medicine, law.invention, Electropherogram, Capillary electrophoresis, law, Genetics, Microsatellite, Humans, Human genome, Fluorescein, Primer (molecular biology), Binding site, Multiplex Polymerase Chain Reaction, Polymerase chain reaction, DNA Primers, Fluorescent Dyes, Microsatellite Repeats

Abstract

Analysis for short tandem repeat (STR) loci is widely performed in forensic laboratories for human identification that utilizes commercially available kits that employ fluorescently labeled primers and capillary electrophoresis. With only a few exceptions, the sequences of the primers included in a kit are not disclosed by the kit manufacturers. Therefore, we developed a simple method to determine the 5′ end of the binding site of the primers included in commercial kits. Our method requires only custom primers and human genome sequence data and routinely used equipment and consumables. One or two custom primers are added to the PCR reaction mixture containing kit primers and input human DNA prior to amplification, and PCR products are separated by capillary electrophoresis after amplification. With this method we can determine which primer of the pair is fluorescently labeled and the 5′ end of the binding site of primers based on the changes in an electropherogram that are caused by the addition of the custom primer(s), and the human genome sequence data. This method is also useful for the determination of the shortest possible lengths of labeled kit primers.

Published

2013

2. Criterion values for multiplex SNP genotyping by the invader assay

Author

Kentaro Kasai, Kazumasa Sekiguchi, Yusuke Nakamura, Michiaki Kubo, Naoya Hosono, Hiroaki Nakahara, and Atsushi Takahashi

Subjects

Genotype, Single-nucleotide polymorphism, Biology, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Pathology and Forensic Medicine, Asian People, Japan, Genetics, SNP, Humans, Multiplex, Typing, Genotyping, DNA Primers, Base Sequence, Genome, Human, Gene Amplification, Reproducibility of Results, DNA, Forensic Medicine, DNA Fingerprinting, SNP genotyping, DNA profiling

Abstract

We have developed a multiplex, single nucleotide polymorphism (SNP) typing system for forensic identification, based on the Invader assay. Using this system, fluorescence data for 21 SNP loci were collected and analyzed. We used endpoint genotyping, commonly used with the Invader assay, and also developed more reliable typing criteria because endpoint typing was occasionally unable to clearly identify the genotype of some loci. Analysis of the fluorescence data identified criteria that had high reproducibility for each genotype. One such criterion is the climbing angle of the curve resulting from two-dimensional plots of the two kinds of fluorescence used for the Invader assay. The climbing angle was observed at the time during the reaction when either or both of the fluorescence intensities increased most significantly. The angles were remarkably associated with homozygous genotypes. On the other hand, all heterozygote endpoint fluorescence ratios were highly reproducible and had very little aberration. These values enabled SNP typing to be more clearly defined compared with typing using only the endpoint fluorescence ratio, which is commonly used with the Invader assay. The values suggested in this study are easily calculated from raw fluorescence data and will be useful for multiplex SNP typing based on the Invader assay.

Published

2009