Testing effects of cell density on NGN2 iN transcriptom

We previously established a standard protocol for NGN2 iN produciton using iP11N iPSC line. Here we aim to explore whether plating density contributes to batch-to-batch variabilities in the transcriptome. Cells were plated at high (400K/cm2) or normal (150K/cm2 densities) and cultured according to the established protocol. Day 28 neurons were harvested and total RNA extracted for bulk RNA sequencing Overall design: 3 repeats of high density and regular density NGN2 iNs were plated in 6 well plates coated with PDL and iMatrix. Cells were maintained till differentiation day 28 before RNA extraction