2012
DOI: 10.1016/j.immuni.2012.02.017
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Critical Role of STAT5 Transcription Factor Tetramerization for Cytokine Responses and Normal Immune Function

Abstract: Summary Cytokine-activated STAT proteins dimerize and bind to high-affinity motifs, and N-terminal domain-mediated oligomerization of dimers allows tetramer formation and binding to low-affinity tandem motifs, but the functions of dimers versus tetramers are unknown. We generated Stat5a-Stat5b double knock-in (DKI) N-domain mutant mice that form dimers but not tetramers, identified cytokine-regulated genes whose expression required STAT5 tetramers, and defined dimer versus tetramer consensus motifs. Whereas St… Show more

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Cited by 165 publications
(201 citation statements)
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References 42 publications
(67 reference statements)
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“…RNA-Seq and ChIP-Seq were performed as reported (14,36). See SI Materials and Methods for more information.…”
Section: Materials Of Methodsmentioning
confidence: 99%
“…RNA-Seq and ChIP-Seq were performed as reported (14,36). See SI Materials and Methods for more information.…”
Section: Materials Of Methodsmentioning
confidence: 99%
“…16 A recent study elucidated the differences in DNA binding between phosphorylated STAT5 dimers and tetramers by generating STAT5A-STAT5B double knockin (DKI) ND mutant mice that lack P-STAT5 tetramers. 17 By studying IL-2-induced gene expression in DKI T cells vs. wild-type (WT) T cells and using ChIP-seq methodology to identify genome-wide binding sites for P-STAT5A/B dimer and tetramer, Lin et al have been able to establish the consensus binding motifs for P-STAT5A/B, including the optimal spacing between two GAS motifs located within 30 nucleotides for tetramer binding. 17 We re-analyzed the data set for GAS distribution at longer distances, 17 and also performed similar analysis of LIF-induced STAT3 binding to DNA, 18 to determine the optimal spacing between neighboring GAS sites using the CisGenome program 19 that is widely used for tiling array, ChIP-seq and genome analysis.…”
mentioning
confidence: 99%
“…17 By studying IL-2-induced gene expression in DKI T cells vs. wild-type (WT) T cells and using ChIP-seq methodology to identify genome-wide binding sites for P-STAT5A/B dimer and tetramer, Lin et al have been able to establish the consensus binding motifs for P-STAT5A/B, including the optimal spacing between two GAS motifs located within 30 nucleotides for tetramer binding. 17 We re-analyzed the data set for GAS distribution at longer distances, 17 and also performed similar analysis of LIF-induced STAT3 binding to DNA, 18 to determine the optimal spacing between neighboring GAS sites using the CisGenome program 19 that is widely used for tiling array, ChIP-seq and genome analysis. Since the profiles of ChIP-seq or ChIP-chip data are often noisy and diffusive, spanning regions ranging from short DNA fragments wrapped around several nucleosomes to large DNA domains covering multiple genes, we first narrowed down the diffusive regions to ChIPenriched sequences and then mapped out location of the GAS-like motif (T/C) (T/A)(C/T)(T/C)N(A/G/T)G(A/T)A in the ChIP-enriched data.…”
mentioning
confidence: 99%
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“…To date, cytokine-regulated genes, the expression of which requires STAT5 tetramers, have been identified using STAT5A-STAT5B double knock-in N-domain mutant mice with STAT5 proteins that form dimers and not tetramers. Of these, il-2r␣ was identified as one of the genes that was expressed through STAT5 tetramers (41). Among the STAT5 target genes analyzed, the expression pattern of il-2r␣ mRNA exhibited the closest relationship with the proliferation and tumorigenesis of cells expressing the JAK2 V617F mutant and EpoR mutants ( Fig.…”
Section: Discussionmentioning
confidence: 97%