AI Article Synopsis

  • Cancer stem-like cells (CSCs), especially glioblastoma stem-like cells, drive cancer growth, treatment resistance, and metastasis due to their self-renewal abilities.
  • A study found that four transcription factors (SOX2, SALL2, OLIG2, and POU3F2) are essential for reprogramming differentiated glioblastoma cells into a stem-like state, with FOSL1 identified as a potential regulator of these factors.
  • Experiments using NTERA-2 and HEK293T cells showed that FOSL1 can directly influence the four transcription factors, alter stemness markers, and affect the cells' ability to form aggregates, indicating its role in stemness reprogram

Article Abstract

Cancer stem-like cells (CSCs) have self-renewal abilities responsible for cancer progression, therapy resistance, and metastatic growth. The glioblastoma stem-like cells are the most studied among CSC populations. A recent study identified four transcription factors (SOX2, SALL2, OLIG2, and POU3F2) as the minimal core sufficient to reprogram differentiated glioblastoma (GBM) cells into stem-like cells. Transcriptomic data of GBM tissues and cell lines from two different datasets were then analyzed by the SWItch Miner (SWIM), a network-based software, and FOSL1 was identified as a putative regulator of the previously identified minimal core. Herein, we selected NTERA-2 and HEK293T cells to perform an in vitro study to investigate the role of FOSL1 in the reprogramming mechanisms. We transfected the two cell lines with a constitutive FOSL1 cDNA plasmid. We demonstrated that FOSL1 directly regulates the four transcription factors binding their promoter regions, is involved in the deregulation of several stemness markers, and reduces the cells' ability to generate aggregates increasing the extracellular matrix component FN1. Although further experiments are necessary, our data suggest that FOSL1 reprograms the stemness by regulating the core of the four transcription factors.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC8290037PMC
http://dx.doi.org/10.1038/s41598-021-94072-0DOI Listing

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