Endocrine cell ER stress conservation

Endocrine cells are dedicated to the production and processing of hormones, from peptides to small molecules, to regulate key physiological processes including glucose homeostasis and metabolism. Because of this relatively high productivity, endocrine cells must handle a variety of stresses from oxidative stress to the unfolded protein response of the endoplasmic reticulum (UPRER). While much is known about the major pathways regulating the UPRER, the roles of endocrine cell type-specific, context-dependent, and time-dependent transcriptional changes are not well explored. To identify unique and shared responses to the UPRER across a subset of endocrine cell types, we tested representative lines for β-cells (insulin), α-cells (glucagon), δ-cells (somatostatin), X/A-cells (ghrelin), L-cells (glucagon-like peptide 1 (GLP1)), and thyrotropes (thyroid hormone and thyroglobulin). We exposed each cell type to the canonical ER stressor thapsigargin for 6 and 24 h, or vehicle (DMSO 0.1%) for 24 h and performed mRNA sequencing. Analysis of the data showed all lines responded to thapsigargin. Comparisons of up- and down-regulated genes between each line revealed both shared and unique transcriptional signatures. These data represent a valuable mineable set of candidate genes which may have cell type-specific functions during the UPRER, and have the potential to lead to new understanding about how different endocrine cells mitigate or succumb to ER stress. All cell lines were plated in 6 well tissue culture dishes until >75% confluent. Cells were treated with DMSO (0.1%) for 24 h or thapsigargin (100nM: MIN6, QGP-1, MGN3-1, GLUTag, PTH-C1; 500nM: αTC1-6 and PCCL3) for 6 and 24 h. RNA was isolated and 100ng of RNA used for RNAseq. MIN6 RNAseq data included in the processed data file is from GSE194200 for the DMSO 24 h and thapsigargin 6 h and 24 h.