| Literature DB >> 24933424 |
Sebastian Marwitz1, Julia Kolarova2, Martin Reck3, Niels Reinmuth3, Christian Kugler3, Ines Schädlich2, Andrea Haake2, Peter Zabel4, Ekkehard Vollmer1, Reiner Siebert5, Torsten Goldmann1, Ole Ammerpohl5.
Abstract
Alterations in the DNA methylome are characteristic for numerous diseases and a typical hallmark of cancer. Therefore, DNA methylation is currently under investigation in research labs and has also entered diagnostics. Recently, protocols like the BeadChip technology have become commercially available to study DNA methylation in an array format and semiquantitative fashion. However, it is known that fixation of the sample material with formalin prior to BeadChip analysis can affect the results. In this study we compared the influence of fixation on the outcome of BeadChip analysis. From six patients each a lung cancer tissue sample and a corresponding tumor-free lung tissue sample were collected. The samples were separated into three pieces. One piece of each sample was fixed with formalin, another one by the non-cross-linking HOPE technique (Hepes-glutamic acid buffer mediated Organic solvent Protection Effect). Subsequently, both became paraffin embedded. As a reference, the remaining third piece was cryopreserved. In addition we used three adenocarcinoma cell lines (H838, A549, and H1650) to validate the results from patient tissues. We show that using the HOPE technique instead of formalin largely prevents the introduction of formalin-fixation related artifacts. An ANOVA analysis significantly separated HOPE- and cryopreserved from formalin-fixed samples (FDR<0.05), while differences in the methylation data obtained from HOPE-fixed and cryopreserved material were minor. Consequently, HOPE fixation is superior to formalin fixation if a subsequent BeadChip analysis of paraffin-embedded sample material is intended.Entities:
Mesh:
Substances:
Year: 2014 PMID: 24933424 DOI: 10.1038/labinvest.2014.79
Source DB: PubMed Journal: Lab Invest ISSN: 0023-6837 Impact factor: 5.662