Abstract

Biotin-labelled DNA probes, prepared by nick-translation in the presence of biotinylated analogs of TTP, are hybridized to DNA or RNA immobilized on nitrocellulose filters. After removal of residual probe, the filters are incubated for 2--5 min with a preformed complex made with avidin-DH (or streptavidin) and biotinylated polymers of intestinal alkaline phosphatase. The filters are then incubated with a mixture of 5-bromo-4-chloro-3-indolyl phosphate and nitro blue tetrazolium, which results in the deposition of a purple precipitate at the sites of hybridization. This procedure will detect target sequences in the 1- to 10-pg range after enzyme incubation periods of 1 hr or less. The incubation period can be extended up to 24 hr, if required, to increase the color intensity of the hybridization signal. Furthermore, at high probe concentrations (250--7560 ng/ml), biotin-labeled DNA exhibits lower nonspecific binding to nitrocellulose than does radiolabeled DNA, so hybridization times required for the analysis of unique mammalian gene sequences can be decreased to 1--2 hr. This nonradiographic method of probe detection should be of general utility for genetic studies using Southern, RNA, or dot-blot hybridization protocols.

Keywords

NitrocelluloseBiotinylationBiotinMolecular biologyDNAHybridization probeRNAAvidinDot blotCollodionDNA–DNA hybridizationSouthern blotStreptavidinBlotBiochemistryNucleic acid thermodynamicsChemistryOligonucleotideNucleic acidBiologyGeneMembrane

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Publication Info

Year
1983
Type
article
Volume
80
Issue
13
Pages
4045-4049
Citations
1064
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Jeffry J. Leary, David J. Brigati, David C. Ward (1983). Rapid and sensitive colorimetric method for visualizing biotin-labeled DNA probes hybridized to DNA or RNA immobilized on nitrocellulose: Bio-blots.. Proceedings of the National Academy of Sciences , 80 (13) , 4045-4049. https://doi.org/10.1073/pnas.80.13.4045

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DOI
10.1073/pnas.80.13.4045