DNA damage promotes jumping between templates during enzymatic amplification.

Pairs of templates and primers were designed so that only recombination events would lead to amplification via the polymerase chain reaction. This approach reveals that lesions such as breaks, apurinic sites, and UV damage in a DNA template can cause the extending primer to jump to another template during the polymerase chain reaction. By comparing sequences of amplification products that were determined directly or via bacterial cloning, it was shown that when the thermostable Thermus aquaticus DNA polymerase encounters the end of a template molecule, it sometimes inserts an adenosine residue; the prematurely terminated product then jumps to another template and polymerization continues, creating an in vitro recombination product. Consequently, amplification products from damaged templates such as archaeological DNA are made up of a high proportion of chimeric molecules. The illegitimate adenosine and thymidine residues in these molecules are detected when cloned molecules are sequenced, but are generally averaged out when the amplification product is sequenced directly. However, if site-specific lesions exist in template DNA or if the amplification is initiated from very few copies, direct sequencing also may yield incorrect sequences. The phenomenon of the "jumping polymerase chain reaction" can be exploited to assess the frequency and location of lesions in nucleic acids.

• Publication year

  1990

• Venue

  Journal of Biological Chemistry

• Publication date

  1990-03-15

• Fields of study

  Biology, Medicine, Chemistry

• Identifiers
  DOI 10.1016/s0021-9258(19)39621-8PMID 2307682
• External record

  Open on Semantic Scholar

• Source metadata

  Semantic Scholar, PubMed

• When lesions are site-specific or the starting template copy number is very low, direct sequencing of PCR products can also produce incorrect sequences.

  Confidence 0.89

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• Amplification of damaged templates such as archaeological DNA yields many chimeric molecules, so cloned products can reveal illegitimate bases that are often averaged out by direct sequencing.

  Confidence 0.96

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• At template ends, Thermus aquaticus DNA polymerase sometimes adds an adenosine residue, and the truncated product can jump to another template before extension continues.

  Confidence 0.93

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• DNA damage can promote template switching during PCR, producing recombination across templates.

  Confidence 0.97

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review

• archaeological dna

  molecule, sample type

  Highly degraded DNA recovered from archaeological material and used here as an example of damaged template DNA.

  Aliases: ancient DNA

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• bacterial cloning

  method, technique

  Propagation of individual PCR products in bacteria before sequencing so that separate molecules can be read one at a time.

  Aliases: cloning

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• chimeric molecule

  molecule, product

  A DNA molecule composed of sequence segments derived from more than one template.

  Aliases: chimera, recombinant molecule

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• direct sequencing

  method, technique

  Sequencing of a pooled amplification product without prior cloning of individual molecules.

  Aliases: bulk sequencing

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• dna damage

  molecule, phenomenon

  Any lesion in a DNA template, including breaks, apurinic sites, and UV-induced damage, that can affect amplification behavior.

  Aliases: damaged DNA, lesions

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• jumping polymerase chain reaction

  method, assay

  A PCR-based assay in which recombination events between templates generate the amplification product.

  Aliases: jumping PCR

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• template end adenosine insertion

  molecular event, process

  The addition of an adenosine residue by DNA polymerase when synthesis reaches the end of a template molecule.

  Aliases: terminal A addition, A addition at template ends

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• template switching

  process, phenomenon

  A PCR event in which an extending primer leaves one DNA template and resumes synthesis on another template.

  Aliases: jumping between templates, primer jumping

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review
• thermus aquaticus dna polymerase

  enzyme, reagent

  The thermostable bacterial DNA polymerase used for PCR amplification in this work.

  Aliases: Taq polymerase, Taq DNA polymerase

  박진우 (dztg5apj7m) extractionB (s683577b42) reviewAnonymous (12632b8b5f) review

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