Development and validation of a 4-color multiplexing spinal muscular atrophy (SMA) genotyping assay on a novel integrated digital PCR instrument

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作者
Lingxia Jiang
Robert Lin
Steve Gallagher
Andrew Zayac
Matthew E. R. Butchbach
Paul Hung
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[1] Combinati Inc.,Center for Applied Clinical Genomics
[2] Nemours Biomedical Research,Center for Pediatric Research
[3] Nemours Alfred I. duPont Hospital for Children,Department of Pediatrics
[4] Nemours Biomedical Research,Department of Biological Sciences
[5] Nemours Alfred I. duPont Hospital for Children,undefined
[6] Sidney Kimmel College of Medicine,undefined
[7] Thomas Jefferson University,undefined
[8] University of Delaware,undefined
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Digital PCR (dPCR) technology has been proven to be highly sensitive and accurate in detecting copy number variations (CNV). However, a higher-order multiplexing dPCR assay for measuring SMN1 and SMN2 copy numbers in spinal muscular atrophy (SMA) samples has not been reported. Described here is a rapid multiplex SMA dPCR genotyping assay run on a fully integrated dPCR instrument with five optical channels. The hydrolysis probe-based multiplex dPCR assay quantifies SMN1, SMN2, and the total SMN (SMN1 + SMN2) while using RPPH1 gene as an internal reference control. The quadruplex assay was evaluated with characterized control DNA samples and validated with 15 blinded clinical samples from a previously published study. SMN1 and SMN2 copy numbers were completely concordant with previous results for both the control and blinded samples. The dPCR-based SMA copy number determination was accomplished in 90 min with a walk-away workflow identical to real-time quantitative PCR (qPCR). In summary, presented here is a simple higher-order multiplexing solution on a novel digital PCR platform to meet the growing demand for SMA genotyping and prognostics.
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