2017
DOI: 10.4049/jimmunol.1602033
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Integration of Kinase and Calcium Signaling at the Level of Chromatin Underlies Inducible Gene Activation in T Cells

Abstract: TCR signaling pathways cooperate to activate the inducible transcription factors NF-κB, NFAT, and AP-1. In this study, using the calcium ionophore ionomycin and/or PMA on Jurkat T cells, we show that the gene expression program associated with activation of TCR signaling is closely related to specific chromatin landscapes. We find that calcium and kinase signaling cooperate to induce chromatin remodeling at ∼2100 chromatin regions, which demonstrate enriched binding motifs for inducible factors and correlate w… Show more

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Cited by 60 publications
(53 citation statements)
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“…RAW264.7:Gp65 cells also expressed an H2B-mCherry nuclear marker (38). NF-B transcriptional activity was monitored with a lentiviral construct (B-NLSluc), which includes a 5× B consensus promoter regulating a sensitive and destabilized firefly luciferase reporter gene as previously described (61). Knockdown of TNFR1 abundance was achieved with the pGFP-TNFRSF1a-B lentiviral shRNA vector (OriGene).…”
Section: Transduced and Primary Cellsmentioning
confidence: 99%
“…RAW264.7:Gp65 cells also expressed an H2B-mCherry nuclear marker (38). NF-B transcriptional activity was monitored with a lentiviral construct (B-NLSluc), which includes a 5× B consensus promoter regulating a sensitive and destabilized firefly luciferase reporter gene as previously described (61). Knockdown of TNFR1 abundance was achieved with the pGFP-TNFRSF1a-B lentiviral shRNA vector (OriGene).…”
Section: Transduced and Primary Cellsmentioning
confidence: 99%
“…After retrieval, cells were collected and cultured off chip for three hours to permit potential alterations by the DEP field or the fluidic forces to be represented transcriptionally. Input cells that were solely cultured served as negative control (Input), whilst cells cultured for three hours under Phorbol-12-myristate 13-acetate and Ionomycin activation (PMA/Iono), globally activating transcription based on protein kinase C (PKC) activation and calcium ion influx [34], served as positive control for global T-cell. Due to the low number of maximally 400 cells per sample and the high volume of up to 100 µl of cell culture medium, we employed mRNA capture beads to obtain the mRNA of the lysed cells and detected over 7600 genes across the experimental conditions (Figure 5a).…”
Section: Transcriptional Profiling Of Miparc Processed Cells Reveals mentioning
confidence: 99%
“…were constructed to express a low resolution luminescence reporter and a high resolution fluorescence reporter. The luminescence reporter was constructed of destabilized firefly luciferase (pGL4.24-luc2P, Promega) (Li et al, 1998;Suter et al, 2011) open reading frame controlled by a DNA cassette containing five tandem repeats of the NF-B transcriptional response element (pLNT-minP-5B-luc2P) (Brignall et al, 2017). The fluorescence reporter was constructed of human p65 N-terminal fusion with tagRFP reporter (pLNT-UbC-tagRFP-p65).…”
Section: Plasmids and Recombinant Virusesmentioning
confidence: 99%