Optimized Real-Time Quantitative PCR Measurement of Male Fetal DNA in Maternal Plasma

Author:

Zimmermann Bernhard1,El-Sheikhah Ahmad2,Nicolaides Kypros2,Holzgreve Wolfgang1,Hahn Sinuhe1

Affiliation:

1. University Women’s Hospital/Department of Research, University Hospital Basel, Basel, Switzerland

2. Harris Birthright Research Centre for Fetal Medicine, King’s College Hospital, London, United Kingdom

Abstract

Abstract Background: Circulating fetal DNA (cfDNA) in maternal plasma has been measured to investigate its possible relationship with pregnancy-related disorders, including fetal trisomy 21 and preeclampsia. The circulating concentrations of single-copy fetal genes, however, are close to the detection limits of PCR methods. Methods: We optimized a protocol for the real-time quantitative PCR amplification of the multicopy sequence DYS14 on the Y-chromosome. This was compared with an established real-time PCR assay for the single-copy SRY gene. Results: By probit regression analysis, the measurements of male DNA by the DYS14 assay had a 10-fold lower detection limit (0.4 genome equivalents) than did measurements of SRY. For plasma samples from women in the first trimester of pregnancy, imprecision (CV) was 2%–22% when amplifying DYS14 compared with 26%–140% for SRY. Conclusions: The low copy numbers of fetal DNA in plasma of women in the first trimester of pregnancy cannot be measured precisely when targeting single-copy sequences. Better results are obtained by amplifying a sequence that is present in multiple copies per male genome.

Publisher

Oxford University Press (OUP)

Subject

Biochemistry (medical),Clinical Biochemistry

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