4.6 Article

Establishment of reporter cells that respond to glucocorticoids by a transposon-mediated promoter-trapping system

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ELSEVIER
DOI: 10.1016/j.ejps.2021.105819

Keywords

Glucocorticoid receptor; Glucocorticoids; Gene reporter assay; Transposon; Trap vector

Funding

  1. Fukushima Prefecture

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By screening reporter cells under specific conditions, the study identified PKP2 as a novel gene responding to glucocorticoids, potentially supplementing the current GRE-based reporter systems. Due to differences in responses to steroids among different clones, using these clones can provide more information.
Previously, we had established a highly sensitive trap vector system for the efficient isolation of reporter cells for a certain condition of interest. In this study, we used this system to screen reporter cells that express the luciferase and enhanced green fluorescent protein genes in response to dexamethasone, a glucocorticoid receptor agonist to facilitate glucocorticoid signaling research. In total, 10 clones were isolated. The insertion sites of the trap vector were analyzed using 5 ' rapid amplification of cDNA ends (5 ' RACE), whereupon LPIN1, PKP2, and FKBP5 were identified as genes that were upregulated by the dexamethasone treatment. Specifically, PKP2 has not previously been focused as a gene that responds to glucocorticoids. The PKP2 mRNA was analyzed and induction of the endogenous gene was confirmed by real-time polymerase chain reaction. Given that PKP2 does not appear to have a consensus glucocorticoid response element (GRE) sequence, this reporter clone could supplement the current GRE-based reporter systems that are prevalently used. Because different clones showed different responses to glucocorticoids, these clones should provide more information than analysis with a single reporter clone. This paper demonstrates that the previously developed trap vector technology can contribute to the rapid construction of drug evaluation systems.

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