Development of Assay-ready iPSCs-derived CD34+ Cells, Monocytes, and Mesenchymal Stem Cells

There is an unmet need for highly characterized and reproducible cell models for a wide range of applications including mechanisms of action, drug development, and toxicity testing. Human induced pluripotent stem cells (iPSCs) have the potential to differentiate into all somatic cell types and therefore hold great promise for development into cell models for variety of toxicity applications. Herein, we have developed processes for the scalable generation of iPSCs-derived CD34+ cells, monocytes, and mesenchymal stem cells (MSCs). It is well documented that starting cell types and donor background play an important role in the efficiency of iPSCs to terminally differentiated cells. We screened four iPSC lines, three from bone marrow CD34+ cells and one foreskin fibroblasts-derived iPSC line, for differentiation into CD34+, monocytes, or MSCs. All CD34+ cells-derived iPSC lines exhibited high efficiency for differentiation into CD34+ cells and MSCs, while the fibroblasts-derived iPSC line favored differentiation into monocytes. To assess the differentiation potential of the iPSCs-derived cells, we demonstrated that CD34+ cells could be differentiated into erythroid cells, myeloid cells, and megakaryocytes while monocytes were capable of differentiating into dendritic cells and functionally active macrophages. Compared to primary MSCs, iPSCs-derived MSCs exhibited similar immunophenotypes and T-cell suppression property as well as the ability to differentiate into adipocytes, osteoblasts, and chondrocytes. It can be problematic to obtain sufficient quantities of certain cell types, including CD34+ cells, for high throughput drug screenings. To address cell availability and donor variation issues, we have developed processes for the scalable and reproducible generation of highly pure, functionally active, assay-ready iPSCs-derived CD34+ cells, monocytes, and MSCs. Furthermore, we have validated iPSC-derived monocytes for conducting the monocyte activation assay, which can be used as an alternative to the rabbit pyrogen test for biologic drugs. Utilization of CFU-GM assays for myelotoxicity screening is hampered by the low throughput of the assay. We have explored the potential of using iPSCs-derived CD34+ for in vitro assessment of anticancer drug-induced myelotoxicity. This assay further enhances the wide variety of applications these highly characterized iPSCs-derived cells provide as powerful tools for drug screening and toxicity testing.