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Comparison of DNA Extraction Methods from Small Samples of Newborn Screening Cards Suitable for Retrospective Perinatal Viral Research
Authors:Gai L. McMichael  Amanda R. Highet  Catherine S. Gibson  Paul N. Goldwater  Michael E. O'Callaghan  Emily R. Alvino  Alastair H. MacLennan  for the South Australian Cerebral Palsy Research Group
Affiliation:The University of Adelaide, School of Paediatrics and Reproductive Health, Disciplines of 1.Obstetrics and Gynaecology and ;3.Paediatrics, and ;2.Department of Microbiology and Infectious Diseases, SA Pathology, Women''s and Children''s Hospital, Adelaide, Australia
Abstract:Reliable detection of viral DNA in stored newborn screening cards (NSC) would give important insight into possible silent infection during pregnancy and around birth. We sought a DNA extraction method with sufficient sensitivity to detect low copy numbers of viral DNA from small punch samples of NSC. Blank NSC were spotted with seronegative EDTA-blood and seropositive EBV EDTA-blood. DNA was extracted with commercial and noncommercial DNA extraction methods and quantified on a spectrofluorometer using a PicoGreen dsDNA quantification kit. Serial dilutions of purified viral DNA controls determined the sensitivity of the amplification protocol, and seropositive EBV EDTA-blood amplified by nested PCR (nPCR) validated the DNA extraction methods. There were considerable differences between the commercial and noncommercial DNA extraction methods (P=0.014; P=0.016). Commercial kits compared favorably, but the QIamp DNA micro kit with an added forensic filter step was marginally more sensitive. The mean DNA yield from this method was 3 ng/μl. The limit of detection was 10 viral genome copies in a 50-μl reaction. EBV nPCR detection in neat and 1:10 diluted DNA extracts could be replicated reliably. We conclude that the QIamp Micro DNA extraction method with the added forensic spin-filter step was suitable for retrospective DNA viral assays from NSC.
Keywords:nPCR   dried blood spots   cytomegalovirus
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