TaqMan qPCR efficiency for quantifying DGAT family mRNA in tung seeds, leaves and flowers.

TaqMan qPCR reaction mixtures contained variable amounts of RNA-equivalent cDNAs from tung seed (2.5, 5, 12.5 and 25 ng), the optimized concentrations of each primer and probe (200 nM) and Absolute QPCR Mix. The amplification efficiency of qPCR assay is calculated according to the equation E = (10−1/slope −1)×100.