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Derivation of human primary prostate epithelial cell lines by differentially targeting the locus along with expression of hTERT. | LitMetric

AI Article Synopsis

  • * The research focuses on creating normal prostate epithelial cell lines using a novel method that involves CRISPR to inactivate a key gene (exon 2) while also expressing a transgene, aiming to maintain genetic integrity.
  • * Two new cell lines were established, characterized by their ability to represent basal prostatic cells, with potential for further applications in developing new prostate cancer models due to the scarcity of existing cell lines.

Article Abstract

Prostate cancer (PCa) is the most common cancer diagnosed in men worldwide and the second leading cause of cancer-related deaths in US males in 2022. Prostate cancer also represents the second highest cancer mortality disparity between non-Hispanic blacks and whites. However, there is a relatively small number of prostate normal and cancer cell lines compared to other cancers. To identify the molecular basis of PCa progression, it is important to have prostate epithelial cell (PrEC) lines as karyotypically normal as possible. Our lab recently developed a novel methodology for the rapid and efficient immortalization of normal human PrEC that combines simultaneous CRISPR-directed inactivation of exon 2 (which directs expression of p16 and p14) and ectopic expression of an transgene. To optimize this methodology to generate immortalized lines with minimal genetic alterations, we sought to target exon 1α of the locus so that p16 expression is ablated while p14 expression remains unaltered. Here we describe the establishment of two cell lines: one with the above-mentioned p16 only loss, and a second line targeting both products in the locus. We characterize the potential lineage origin of these new cell lines along with our previously obtained clones, revealing distinct gene expression signatures. Based on the analyses of protein markers and RNA expression signatures, these cell lines are most closely related to a subpopulation of basal prostatic cells. Given the simplicity of this one-step methodology and the fact that it uses only the minimal genetic alterations necessary for immortalization, it should also be suitable for the establishment of cell lines from primary prostate tumor samples, an urgent need given the limited number of available prostate cancer cell lines.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11100872PMC
http://dx.doi.org/10.21203/rs.3.rs-4294058/v1DOI Listing

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