Improving specificity of DNA hybridization-based methods

doi:10.1093/nar/gnh125

Nucleic Acids Research 2004 32(16):e130; doi:10.1093/nar/gnh125

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Published online 15 September 2004

Improving specificity of DNA hybridization-based methods

Tatyana Chalaya, Elena Gogvadze, Anton Buzdin^*, Elena Kovalskaya and Eugene D. Sverdlov

Shemyakin–Ovchinnikov Institute of Bioorganic Chemistry, Moscow 117871, Russia

^* To whom correspondence should be addressed. Tel: +7 095 3306329; Fax: +7 095 3306538; Email: anton{at}humgen.siobc.ras.ru
The authors wish it to be known that, in their opinion, the first two authors should be regarded as joint First Authors
⁺AY688954–AY688956

Received July 21, 2004; Revised and Accepted August 19, 2004

Methods based on DNA reassociation in solution with the subsequentPCR amplification of certain hybrid molecules, such as coincidencecloning and subtractive hybridization, all suffer from a commonimperfection: cross-hybridization between various types of paralogousrepetitive DNA fragments. Although the situation can be slightlyimproved by the addition of repeat-specific competitor DNA intothe hybridization mixture, the cross-hybridization outcome isa significant number of background chimeric clones in resultingDNA libraries. In order to overcome this challenge, we developeda technique called mispaired DNA rejection (MDR), which utilizesa treatment of resulting reassociated DNA with mismatch-specificnucleases. We examined the MDR efficiency using cross-hybridizationof complex, whole genomic mixtures derived from human and chimpanzeegenomes, digested with frequent-cutter restriction enzyme. Weshow here that both single-stranded DNA-specific and mismatcheddouble-stranded DNA-specific nucleases can be used for MDR separatelyor in combination, reducing the background level from 60 to4% or lower. The technique presented here is of universal usefulnessand can be applied to both cDNA and genomic DNA subtractionsof very complex DNA mixtures. MDR is also useful for the genome-widerecovery of highly conserved DNA sequences, as we demonstrateby comparing human and pygmy marmoset genomes.

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