Literature DB >> 12664984

Development of an Alu-based, QSY 7-labeled primer PCR method for quantitation of human DNA in forensic samples.

Janice A Nicklas1, Eric Buel.   

Abstract

Determining the amount of human DNA extracted from a crime scene sample is an important step in DNA profiling. The forensic community relies almost entirely upon a technique (slot blot) to quantitate human DNA that is imprecise, time consuming, and labor intensive. This paper describes the development of a new technique based on PCR amplification of a repetitive Alu sequence. Specific primers were used to amplify a 124-bp fragment of Alu sequence; amplification was detected by SYBR Green I staining in a fluorescent plate reader. To reduce background in the plate reader assay, QSY-7 labeled primers were utilized. The assay was tested on animal DNAs, human blood spots, mock crime samples, and degraded DNA in comparison with the slot blot technique. The QSY Alu assay has a dynamic range of 10 ng to 10 pg, and is sensitive, specific, fast, quantitative, and comparable in cost to the slot blot assay.

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Year:  2003        PMID: 12664984

Source DB:  PubMed          Journal:  J Forensic Sci        ISSN: 0022-1198            Impact factor:   1.832


  3 in total

1.  Real-Time PCR: Revolutionizing Detection and Expression Analysis of Genes.

Authors:  Sa Deepak; Kr Kottapalli; R Rakwal; G Oros; Ks Rangappa; H Iwahashi; Y Masuo; Gk Agrawal
Journal:  Curr Genomics       Date:  2007-06       Impact factor: 2.236

2.  Screening for residual disease in pediatric burkitt lymphoma using consensus primer pools.

Authors:  Melissa Agsalda; Ian Kusao; David Troelstrup; Bruce Shiramizu
Journal:  Adv Hematol       Date:  2009-04-15

3.  Tracking intravenous adipose-derived mesenchymal stem cells in a model of elastase-induced emphysema.

Authors:  You-Sun Kim; Ji-Young Kim; Dong-Myung Shin; Jin Won Huh; Sei Won Lee; Yeon-Mok Oh
Journal:  Tuberc Respir Dis (Seoul)       Date:  2014-09-30
  3 in total

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