identification of factors contributing to variability in a blood-based gene expression test识别的因素变化blood-based基因表达检测.pdfVIP
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identification of factors contributing to variability in a blood-based gene expression test识别的因素变化blood-based基因表达检测
Identification of Factors Contributing to Variability in a
Blood-Based Gene Expression Test
Michael R. Elashoff, Rachel Nuttall, Philip Beineke, Michael H. Doctolero, Mark Dickson,
Andrea M. Johnson, Susan E. Daniels, Steven Rosenberg, James A. Wingrove*
CardioDx, Inc., Palo Alto, California, United States of America
Abstract
Background: Corus CAD is a clinically validated test based on age, sex, and expression levels of 23 genes in whole blood
that provides a score (1–40 points) proportional to the likelihood of obstructive coronary disease. Clinical laboratory process
variability was examined using whole blood controls across a 24 month period: Intra-batch variability was assessed using
sample replicates; inter-batch variability examined as a function of laboratory personnel, equipment, and reagent lots.
Methods/Results: To assess intra-batch variability, five batches of 132 whole blood controls were processed; inter-batch
variability was estimated using 895 whole blood control samples. ANOVA was used to examine inter-batch variability at 4
process steps: RNA extraction, cDNA synthesis, cDNA addition to assay plates, and qRT-PCR. Operator, machine, and reagent
lots were assessed as variables for all stages if possible, for a total of 11 variables. Intra- and inter-batch variations were
estimated to be 0.092 and 0.059 Cp units respectively (SD); total laboratory variation was estimated to be 0.11 Cp units (SD).
In a regression model including all 11 laboratory variables, assay plate lot and cDNA kit lot contributed the most to
variability (p = 0.045; 0.009 respectively). Overall, reagent lots for RNA extraction, cDNA synthesis, and qRT-PCR contributed
the most to inter-batch variance (52.3%), followed by operators and machines (18.9% and 9.2% respectively), leaving 19.6%
of the variance unexplained.
Conclusion: Intra-batch variability inherent to the PCR
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