AI Article Synopsis

  • - The study focuses on the role of demethylation in FOXP3-TSDR, which is crucial for the stable differentiation and function of regulatory T (Treg) cells.
  • - Researchers engineered plasmids to express a fusion protein that includes a nonfunctional Cas9 and a TET1 catalytic domain to target the FOXP3-TSDR segment in Jurkat T cells.
  • - Results showed that this approach significantly reduced FOXP3-TSDR methylation and increased Foxp3 mRNA levels in Jurkat cells, suggesting the potential for programming Treg cells in patients.

Article Abstract

Demethylation of FOXP3-TSDR (Treg specific demethylated region) is a hallmark of stable differentiation and suppressive function of regulatory T (Treg) cells. Previous protocols aiming at human naïve T cell differentiation failed to implement a Treg cell specific epigenetic signature. Ten-eleven translocation (TET) enzymes catalyze DNA demethylation. Plasmids towardexpression of a fusion protein encompassing nonfunctional Cas9, the catalytic domain of TET1, blue fluorescent protein, and encoding single guide RNAs (sgRNAs) targeting specific segments of the FOXP3-TSDR were engineered and transfected into Jurkat T cells. FOXP3-TSDR methylation was analyzed by deep-amplicon bisulfite sequencing while cellular Foxp3, Tbet, Gata3, and Rorgt mRNA levels were determined by real-time PCR. Overexpression of dCas9TET1 significantly decreased Jurkat cell FOXP3-TSDR methylation and increased Foxp3 mRNA expression while expressions of master transcription factor mRNAs of other major T cell lineages remained largely unaffected. dCas9-TET1 construct transfection mediated Treg programming of patients' primary T cells might be feasible.

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Source
http://dx.doi.org/10.1016/j.cellimm.2021.104471DOI Listing

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