Evaluation of automated techniques for extraction of circulating cell-free DNA for implementation in standardized high-throughput workflows

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Sarah Lehle
Julius Emons
Carolin C. Hack
Felix Heindl
Alexander Hein
Caroline Preuß
Katharina Seitz
Anna L. Zahn
Matthias W. Beckmann
Peter A. Fasching
Matthias Ruebner
Hanna Huebner
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[1] Erlangen University Hospital,Department of Gynecology and Obstetrics, Comprehensive Cancer Center Erlangen
[2] Friedrich-Alexander-Universität Erlangen-Nürnberg (FAU),EMN
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Analysis of circulating cell-free DNA (ccfDNA) is a suitable tool for detecting somatic mutations for the purpose of making decisions on treatment, monitoring treatment response, and predicting survival. High-throughput techniques for ccfDNA extraction are essential to implementing ccfDNA testing in the clinical setting. We set out to compare two automated techniques with regard to hands-on time, ccfDNA output and integrity, and circulating mitochondrial DNA (mtDNA). CcfDNA was isolated using the EZ1&2 ccfDNA field test kit (EZ2 kit, QIAGEN) and the Maxwell RSC ccfDNA plasma kit (Maxwell kit, Promega). DNA was extracted from plasma of 30 breast cancer patients enrolled in the iMODE-B (#325_19B; 12.10.2020) study. Real-time PCR, fluorescence-based detection and automated electrophoresis were used to assess ccfDNA concentrations. The ccfDNA yield was significantly higher when extracted with the EZ2 kit. The EZ2 kit enabled the isolation of a higher proportion of short fragments and a lower proportion of long fragments, resulting in lower DNA integrity. Significantly lower mtDNA quantities were detected in the Maxwell eluate than in the EZ2 eluate. Thus, decisions on which extraction method to use should proceed on the basis of the required input for downstream applications, the anticipated fragment size and minimum hands-on time.
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