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Using synthetic oligonucleotides as standards in probe-based qPCR

  • Published:2018-04 Issue:4 Volume:64 Page:177-179
  • ISSN:0736-6205
  • Container-title:BioTechniques
  • language:en
  • Short-container-title:BioTechniques

Author:

Conte Jillian12,Potoczniak Margret J3,Tobe Shanan S34

Affiliation:

1. Keystone College, Department of Biological & Physical Sciences, One College Green, La Plume, PA 18440, USA

2. University of the Sciences, Department of Biological Sciences, Philadelphia, PA, USA

3. Arcadia University, Department of Chemistry & Physics, Glenside, PA, USA

4. College of Science & Engineering, Flinders University, Adelaide, SA 5042, Australia

Abstract

Real-time PCR (qPCR) is widely used in the life sciences. For quantifying DNA, a standard curve is required. Common methods for standard development are time consuming, costly, necessitate a specific skill set, and pose a contamination risk. Using a targeted synthetic oligonucleotide, such as a gBlocks® Gene Fragment, overcomes these drawbacks and provides researchers an accurate and quick solution to standard development. Here, we demonstrate that using a gBlocks fragment as a standard provides comparable sensitivity, reliability, and assay performance to a purified amplicon standard.

Publisher

Future Science Ltd

Subject

General Biochemistry, Genetics and Molecular Biology,Biotechnology
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