DNase footprinting assay

DNase I footprint of a protein binding to a radiolabelled DNA fragment. Lanes "GA" and "TC" are Maxam-Gilbert chemical sequencing lanes, see DNA Sequencing. The lane labelled "control" is for quality control purposes and contains the DNA fragment but not treated with DNase I.

A DNase footprinting assay^[1] is a DNA footprinting technique from molecular biology/biochemistry that detects DNA-protein interaction using the fact that a protein bound to DNA will often protect that DNA from enzymatic cleavage. This makes it possible to locate a protein binding site on a particular DNA molecule. The method uses an enzyme, deoxyribonuclease (DNase, for short), to cut the radioactively end-labeled DNA, followed by gel electrophoresis to detect the resulting cleavage pattern.

For example, the DNA fragment of interest may be PCR amplified using a ³²P 5' labeled primer, with the result being many DNA molecules with a radioactive label on one end of one strand of each double stranded molecule. Cleavage by DNase will produce fragments. The fragments which are smaller with respect to the ³²P-labelled end will appear further on the gel than the longer fragments. The gel is then used to expose a special photographic film.

The cleavage pattern of the DNA in the absence of a DNA binding protein, typically referred to as free DNA, is compared to the cleavage pattern of DNA in the presence of a DNA binding protein. If the protein binds DNA, the binding site is protected from enzymatic cleavage. This protection will result in a clear area on the gel which is referred to as the "footprint".

By varying the concentration of the DNA-binding protein, the binding affinity of the protein can be estimated according to the minimum concentration of protein at which a footprint is observed.

This technique was developed by David J. Galas and Albert Schmitz at Geneva in 1977^[2]

References[edit]

^ Brenowitz M, Senear DF, Shea MA, Ackers GK (1986). "[9] Quantitative DNase footprint titration: A method for studying protein-DNA interactions". Quantitative DNase footprint titration: a method for studying protein-DNA interactions. Methods in Enzymology. Vol. 130. pp. 132–81. doi:10.1016/0076-6879(86)30011-9. ISBN 9780121820305. PMID 3773731.
^ Galas DJ, Schmitz A (Sep 1978). "DNAse footprinting: a simple method for the detection of protein-DNA binding specificity". Nucleic Acids Research. 5 (9): 3157–70. doi:10.1093/nar/5.9.3157. PMC 342238. PMID 212715.

[1] Brenowitz M, Senear DF, Shea MA, Ackers GK (1986). "[9] Quantitative DNase footprint titration: A method for studying protein-DNA interactions". Quantitative DNase footprint titration: a method for studying protein-DNA interactions. Methods in Enzymology. Vol. 130. pp. 132–81. doi:10.1016/0076-6879(86)30011-9. ISBN 9780121820305. PMID 3773731.

[2] Galas DJ, Schmitz A (Sep 1978). "DNAse footprinting: a simple method for the detection of protein-DNA binding specificity". Nucleic Acids Research. 5 (9): 3157–70. doi:10.1093/nar/5.9.3157. PMC 342238. PMID 212715.

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