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HERO ID
6213796
Reference Type
Book/Book Chapter
Title
[28] DNA extraction from archived specimens by sonication
Author(s)
Heller, MJ; Robinson, RA
Year
1995
Publisher
Academic Press
Book Title
Methods in Neurosciences
Volume
26
Page Numbers
431-443
DOI
10.1016/S1043-9471(06)80106-0
URL
http://www.sciencedirect.com/science/article/pii/S1043947106801060
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Abstract
Publisher Summary The analysis of DNA from archived tissues is an important clinical research and diagnostic tool. The analyses of these preserved tissues that are most commonly formalin-fixed and paraffin-embedded allow for the retrospective study of a variety of genetic changes, or even the presence of infectious agents. Prior to polymerase chain reaction (PCR), the genetic analyses of fixed tissues were carried out using in situ hybridization, dot-blot hybridization, or Southern blotting. These methodologies have traditionally provided some degree of success, but are sometimes limited in sensitivity, involve complex procedures, or cannot detect degraded DNA, which is found in old-fixed tissues. PCR analysis provides a simple and sensitive method for the analysis of DNA from fixed tissues. A number of methods exist for isolating DNA from formalin-fixed, paraffin-embedded tissues, but the best procedures in terms of reliably releasing DNA involve a large number of solvent extractions, centrifugations, and long digestion periods with enzyme buffers. A method has been developed that quickly and efficiently extracts DNA from paraffin-embedded tissue. This method utilizes a sonicating water bath to disrupt the tissue samples and such samples can be prepared in less than 30 min with only solvent extraction in a minimum of steps.
Editor(s)
Sarkar, Gobinda
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