Different length (DL) qPCR for quantification of cell killing by UV-induced DNA damage

Knut Rudi; Irina Hagen; Bente Carina Johnsrud; Guro Skjefstad; Ingun Tryland

doi:10.3390/ijerph7093376

Different length (DL) qPCR for quantification of cell killing by UV-induced DNA damage

Int J Environ Res Public Health. 2010 Sep;7(9):3376-81. doi: 10.3390/ijerph7093376. Epub 2010 Aug 31.

Authors

Knut Rudi¹, Irina Hagen, Bente Carina Johnsrud, Guro Skjefstad, Ingun Tryland

Affiliation

¹ Hedmark University College, Lærerskolealleen 1, 2418 Elverum, Norway. knut.rudi@hihm.no

Abstract

We describe the different length (DL) qPCR method for quantification of UV induced DNA damage in cell killing. The principle of DL qPCR is that DNA damage inhibits PCR. Applications with different lengths can therefore be used to detect different levels of UV-induced DNA damage. The assay was evaluated on three strains of Escherichia coli exposed to varying levels of ultraviolet (UV) radiation. We show that DL qPCR sensitivity and reproducibility are within the range of practical application to detect the effect of UV cell killing.

Keywords: UV; quantitative PCR; viable/dead cells.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Biological Assay / methods
DNA Damage*
Escherichia coli
Polymerase Chain Reaction / methods*
Sensitivity and Specificity
Ultraviolet Rays / adverse effects*