Literature DB >> 9016676

Effect of highly fragmented DNA on PCR.

E M Golenberg1, A Bickel, P Weihs.   

Abstract

We characterized the behavior of polymerase chain reactions (PCR) using degraded DNA as a template. We first demonstrated that fragments larger than the initial template fragments can be amplified if overlapping fragments are allowed to anneal and extend prior to routine PCR. Amplification products increase when degraded genomic DNA is pretreated by polymerization in the absence of specific primers. Secondly, we measured nucleotide uptake as a function of template DNA degradation. dNTP incorporation initially increases with increasing DNA fragmentation and then declines when the DNA becomes highly degraded. We demonstrated that dNTP uptake continues for >10 polymerization cycles and is affected by the quality and quantity of template DNA and by the amount of substrate dNTP. These results suggest that although reconstruction of degraded DNA may allow amplification of large fragments, reconstructive polymerization and amplification polymerization may compete. This was confirmed in PCR where the addition of degraded DNA reduced the resultant product. Because terminal deoxynucleotidyl transferase activity of Taq polymerase may inhibit 3' annealing and restrict the length of template reconstruction, we suggest modified PCR techniques which separate reconstructive and amplification polymerization reactions.

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Year:  1996        PMID: 9016676      PMCID: PMC146324          DOI: 10.1093/nar/24.24.5026

Source DB:  PubMed          Journal:  Nucleic Acids Res        ISSN: 0305-1048            Impact factor:   16.971


  17 in total

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3.  Postmortem stability of DNA.

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5.  Extraction, evaluation, and amplification of DNA from decalcified and undecalcified United States Civil War bone.

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Journal:  J Forensic Sci       Date:  1993-01       Impact factor: 1.832

6.  Sex identification by polymerase chain reaction of alpha-satellite in aged tissue samples.

Authors:  P Fattorini; S Cacció; S Gustincih; F Florian; B M Altamura; G Graziosi
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7.  Purification of forensic specimens for the polymerase chain reaction (PCR) analysis.

Authors:  A Akane; H Shiono; K Matsubara; H Nakamura; M Hasegawa; M Kagawa
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8.  Guidelines for internal validation of the HLA-DQ alpha DNA typing system.

Authors:  R B Wilson; J L Ferrara; H J Baum; R C Shaler
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9.  Rate of depurination of native deoxyribonucleic acid.

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Authors:  V W Campbell; D A Jackson
Journal:  J Biol Chem       Date:  1980-04-25       Impact factor: 5.157

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  21 in total

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2.  A validation study of the Qiagen Investigator DIPplex® kit; an INDEL-based assay for human identification.

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3.  Forensic performance of two insertion-deletion marker assays.

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4.  Assessment of the role of DNA repair in damaged forensic samples.

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5.  Sensitive Identification of Bacterial DNA in Clinical Specimens by Broad-Range 16S rRNA Gene Enrichment.

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6.  Evaluating the Feasibility of DNA Methylation Analyses Using Long-Term Archived Brain Formalin-Fixed Paraffin-Embedded Samples.

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7.  A novel method to compensate for different amplification efficiencies between patient DNA samples in quantitative real-time PCR.

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8.  Modeling of 5' nuclease real-time responses for optimization of a high-throughput enrichment PCR procedure for Salmonella enterica.

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Review 9.  Current genetic methodologies in the identification of disaster victims and in forensic analysis.

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Journal:  BMC Bioinformatics       Date:  2007-04-20       Impact factor: 3.169

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