Competitive polymerase chain reaction using an internal standard: application to the quantitation of viral DNA.

Telenti A; Imboden P; Germann D

doi:10.1016/0166-0934(92)90099-y

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Journal article

Competitive polymerase chain reaction using an internal standard: application to the quantitation of viral DNA.

Telenti A Institute of Medical Microbiology, University of Berne, Switzerland.
Imboden P
Germann D

1992-09-01

Published in:

Journal of virological methods. - 1992

English A general strategy for the construction of an internal standard for the polymerase chain reaction (PCR) is described together with its application in the evaluation of clinical samples. This internal standard is a plasmid containing a modified target sequence that is co-amplified with the native target using the same set of primers. The co-amplification reaction will generate two fragments of different size that are readily separated without the need for restriction enzyme digestion. Thereafter, they are detected and quantitated by hybridization to the same probe. Detection of HIV proviral DNA was chosen as a model for this competitive PCR. The assay proved to be a sensitive tool for the detection of PCR inhibitors and allowed quantitation of HIV with a 20-30% variation coefficient. Despite limitations that appear inherent to the amplification process, internal standards appear to be useful tools for quantitative analysis by PCR.

Language

English

Open access status

closed

Identifiers

DOI 10.1016/0166-0934(92)90099-y
PMID 1430070

Persistent URL

https://sonar.rero.ch/global/documents/74992

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Journal article

Competitive polymerase chain reaction using an internal standard: application to the quantitation of viral DNA.

Base Sequence

Binding, Competitive

Cloning, Molecular

DNA, Viral

HIV Infections

Humans

Molecular Sequence Data

Polymerase Chain Reaction

Statistics