DNA extraction procedures meaningfully influence qPCR-based mtDNA copy number determination |
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| Authors: | Wen Guo Lan Jiang Shalender Bhasin Shaharyar M Khan Russell H Swerdlow |
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| Institution: | aDepartment of Internal Medicine, Boston University School of Medicine, Section of Endocrinology, Boston, MA 02118, United States;bGencia Corporation, University of Kansas School of Medicine, United States;cDepartments of Neurology, Molecular and Integrative Physiology, University of Kansas School of Medicine, United States |
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| Abstract: | Quantitative real time PCR (qPCR) is commonly used to determine cell mitochondrial DNA (mtDNA) copy number. This technique involves obtaining the ratio of an unknown variable (number of copies of an mtDNA gene) to a known parameter (number of copies of a nuclear DNA gene) within a genomic DNA sample. We considered the possibility that mtDNA:nuclear DNA (nDNA) ratio determinations could vary depending on the method of genomic DNA extraction used, and that these differences could substantively impact mtDNA copy number determination via qPCR. To test this we measured mtDNA:nDNA ratios in genomic DNA samples prepared using organic solvent (phenol–chloroform–isoamyl alcohol) extraction and two different silica-based column methods, and found mtDNA:nDNA ratio estimates were not uniform. We further evaluated whether different genomic DNA preparation methods could influence outcomes of experiments that use mtDNA:nDNA ratios as endpoints, and found the method of genomic DNA extraction can indeed alter experimental outcomes. We conclude genomic DNA sample preparation can meaningfully influence mtDNA copy number determination by qPCR. |
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| Keywords: | Mitochondrial DNA Phenol extraction Real-times PCR DNA isolation |
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