Figure 4.

Validation of transcript abundance estimation for endogenous transcripts. qPCR primer sets were designed for selected genes so that amplicons were upstream of 60-mer oligonucleotide probes when possible, or less than 650 bp downstream, and copy number was estimated using serial dilutions of RNA, in vitro transcribed from mouse cDNAs, at known copy numbers as standards. Error bars represent one standard deviation across three replicate samples for each tissue. Dotted diagonal lines represent five- and tenfold differences between the two datasets. Each gene's official symbol, along with the unique identifier for the 60-mer oligonucleotide probe it was measured with, are listed in the key. Data was normalized to Gapd expression for both methods. EM = E12.5 embryo, PL = E12.5 placenta, ES = embryonic stem cells, TS = trophoblast stem cells.