A simple modification to improve the accuracy of methylation-sensitive restriction enzyme quantitative polymerase chain reaction |
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| Authors: | Magdalena Krygier Justyna Podolak-Popinigis Janusz Limon Paweł Sachadyn Anna Stanisławska-Sachadyn |
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| Affiliation: | 1. Department of Biology and Genetics, Medical University of Gdańsk, 80-210 Gdańsk, Poland;2. Department of Molecular Biotechnology and Microbiology, Gdańsk University of Technology, 80-233 Gdańsk, Poland |
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| Abstract: | DNA digestion with endonucleases sensitive to CpG methylation such as HpaII followed by polymerase chain reaction (PCR) quantitation is commonly used in molecular studies as a simple and inexpensive solution for assessment of region-specific DNA methylation. We observed that the results of such analyses were highly overestimated if mock-digested samples were applied as the reference. We determined DNA methylation levels in several promoter regions in two setups implementing different references: mock-digested and treated with a restriction enzyme that has no recognition sites within examined amplicons. Fragmentation of reference templates allowed removing the overestimation effect, thereby improving measurement accuracy. |
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| Keywords: | Methylation-sensitive restriction enzyme MSRE&ndash qPCR Methylation Assay Validation |
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