4.7 Article

Size separation of circulatory DNA in maternal plasma permits ready detection of fetal DNA polymorphisms

Journal

CLINICAL CHEMISTRY
Volume 50, Issue 6, Pages 1002-1011

Publisher

OXFORD UNIV PRESS INC
DOI: 10.1373/clinchem.2003.029835

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Background: Analysis of fetal DNA in maternal plasma has recently been introduced as a new method for noninvasive prenatal diagnosis, particularly for the analysis of fetal genetic traits, which are absent from the maternal genome, e.g., RHD or Y-chromosome-specific sequences. To date, the analysis of other fetal genetic traits has been more problematic because of the overwhelming presence of maternal DNA sequences in the circulation. We examined whether different biochemical properties can be discerned between fetal and maternal circulatory DNA. Methods: Plasma DNA was examined by agarose gel electrophoresis. The fractions of fetal and maternal DNA in size-fractionated fragments were assayed by real-time PCR. The determination of paternally and maternally inherited fetal genetic traits was examined by use of highly polymorphic chromosome-21-specific microsatellite markers. Results: Size fractionation of circulatory DNA indicated that the major portion of cell-free fetal DNA had an approximate molecular size of <0.3 kb, whereas maternally derived sequences were, on average, considerably larger than 1 kb. Analysis of size-fractionated DNA (less than or equal to0.3 kb) from maternal plasma samples facilitated the ready detection of paternally and maternally inherited microsatellite markers. Conclusions: Circulatory fetal DNA can be enriched by size selection of fragment sizes less than similar to0.3kb. Such selection permits easier analysis of both paternally and maternally inherited DNA polymorphisms. (C) 2004 American Association for Clinical Chemistry.

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