Literature DB >> 17690213

DNA degradation test predicts success in whole-genome amplification from diverse clinical samples.

Fengfei Wang1, Lilin Wang, Christine Briggs, Ewa Sicinska, Sandra M Gaston, Harvey Mamon, Matthew H Kulke, Raffaella Zamponi, Massimo Loda, Elizabeth Maher, Shuji Ogino, Charles S Fuchs, Jin Li, Carlos Hader, G Mike Makrigiorgos.   

Abstract

The need to apply modern technologies to analyze DNA from diverse clinical samples often stumbles on suboptimal sample quality. We developed a simple approach to assess DNA fragmentation in minute clinical samples of widely different origin and the likelihood of success of degradation-tolerant whole genome amplification (restriction and circularization-aided rolling circle amplification, RCA-RCA) and subsequent polymerase chain reaction (PCR). A multiplex PCR amplification of four glyceraldehyde-3-phosphate dehydrogenase amplicons of varying sizes was performed using genomic DNA from clinical samples, followed by size discrimination on agarose gel or fluorescent denaturing high-performance liquid chromatography (dHPLC). RCA-RCA followed by real-time PCR was also performed, for correlation. Even minimal quantities of longer PCR fragments ( approximately 300 to 400 bp), visible via high-sensitivity fluorescent dHPLC or agarose gel, were essential for the success of RCA-RCA and subsequent PCR-based assays. dHPLC gave a more accurate correlation between DNA fragmentation and sample quality than agarose gel electrophoresis. Multiplex-PCR-dHPLC predicted correctly the likelihood of assay success in formalin-fixed, paraffin-embedded samples fixed under controlled conditions and of different ages, in laser capture microdissection samples, in tissue print micropeels, and plasma-circulating DNA. Estimates of the percent information retained relative to snap-frozen DNA are derived for real-time PCR analysis. The assay is rapid and convenient and can be used widely to characterize DNA from any clinical sample of unknown quality.

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Year:  2007        PMID: 17690213      PMCID: PMC1975106          DOI: 10.2353/jmoldx.2007.070004

Source DB:  PubMed          Journal:  J Mol Diagn        ISSN: 1525-1578            Impact factor:   5.568


  37 in total

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2.  Whole genome analysis of genetic alterations in small DNA samples using hyperbranched strand displacement amplification and array-CGH.

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4.  Degenerate oligonucleotide-primed PCR: general amplification of target DNA by a single degenerate primer.

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5.  Whole genome amplification from a single cell: implications for genetic analysis.

Authors:  L Zhang; X Cui; K Schmitt; R Hubert; W Navidi; N Arnheim
Journal:  Proc Natl Acad Sci U S A       Date:  1992-07-01       Impact factor: 11.205

6.  Real-time quantitative RT-PCR shows variable, assay-dependent sensitivity to formalin fixation: implications for direct comparison of transcript levels in paraffin-embedded tissues.

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7.  Towards fully automated genome-wide polymorphism screening.

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8.  Extraction of DNA from paraffin-embedded tissue for analysis by polymerase chain reaction: new tricks from an old friend.

Authors:  D Shibata
Journal:  Hum Pathol       Date:  1994-06       Impact factor: 3.466

9.  Microsatellite alterations in plasma DNA of small cell lung cancer patients.

Authors:  X Q Chen; M Stroun; J L Magnenat; L P Nicod; A M Kurt; J Lyautey; C Lederrey; P Anker
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10.  Whole genome amplification of DNA from laser capture-microdissected tissue for high-throughput single nucleotide polymorphism and short tandem repeat genotyping.

Authors:  Martha S Rook; Scott M Delach; Galina Deyneko; Andrew Worlock; Jia Liu Wolfe
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  27 in total

1.  National Cancer Institute Biospecimen Evidence-Based Practices: Harmonizing Procedures for Nucleic Acid Extraction from Formalin-Fixed, Paraffin-Embedded Tissue.

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Journal:  Biopreserv Biobank       Date:  2018-06-19       Impact factor: 2.300

Review 2.  Identification of evidence-based biospecimen quality-control tools: a report of the International Society for Biological and Environmental Repositories (ISBER) Biospecimen Science Working Group.

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3.  Detection of EGFR mutations in plasma DNA from lung cancer patients by mass spectrometry genotyping is predictive of tumor EGFR status and response to EGFR inhibitors.

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4.  Development of Novel Mutation-Specific Droplet Digital PCR Assays Detecting TERT Promoter Mutations in Tumor and Plasma Samples.

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5.  Nuclease-Assisted, Multiplexed Minor-Allele Enrichment: Application in Liquid Biopsy of Cancer.

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6.  Targeted KRAS mutation assessment on patient tumor histologic material in real time diagnostics.

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7.  Methylated eyes absent 4 (EYA4) gene promotor in non-neoplastic mucosa of ulcerative colitis patients with colorectal cancer: evidence for a field effect.

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8.  Performance of whole-genome amplified DNA isolated from serum and plasma on high-density single nucleotide polymorphism arrays.

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Journal:  J Mol Diagn       Date:  2008-04-10       Impact factor: 5.568

9.  Whole genome sequencing for lung cancer.

Authors:  Marissa Daniels; Felicia Goh; Casey M Wright; Krishna B Sriram; Vandana Relan; Belinda E Clarke; Edwina E Duhig; Rayleen V Bowman; Ian A Yang; Kwun M Fong
Journal:  J Thorac Dis       Date:  2012-04-01       Impact factor: 2.895

Review 10.  Clinical application of high-throughput genomic technologies for treatment selection in breast cancer.

Authors:  Aaron R Hansen; Philippe L Bedard
Journal:  Breast Cancer Res       Date:  2013       Impact factor: 6.466

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