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Fig. 1. Myc is a STAT3 target gene in ES cells. (A) LIF-maintained ES cells or
embryoid bodies (-LIF) generated from ES cells were harvested and mRNA
analysed by RT-PCR analysis using primers designed against Rex1, Oct4, Fgf5,
brachyury, Myc and ß-actin. (B) Chromatin immunoprecipitation (ChIP)
analysis with a FLAG monoclonal antibody was performed on crosslinked
chromatin from a cell line expressing FLAG-tagged STAT3
(STAT3FLAG). Immunoprecipitated chromatin was then used to
determine if STAT3FLAG bound the endogenous Myc promoter using a
specific primer pair that flanks an E2F/E-box in the Myc P2 promoter (left
panels). The same chromatin was used as a template in a PCR reaction using
primer for the CDK1 promoter that is not implicated as a STAT3 target gene
(right panel). Addition of FLAG antibody in ChIPs is as indicated (+). To
control for the amount of total chromatin in the ChIP assay, equivalent
amounts of total template (`input'), equivalent to 0.03% of total chromatin
DNA used in ChIP assays, were used in a parallel PCR reaction using Myc or
CDK1 specific primers. Immunoblot analysis: relative expression levels of
total STAT3 in the transfected cell line is shown relative to endogenous STAT3
levels (vector alone transfectant). (C) STAT3 trans-activates the Myc gene in
ES cells. LIF maintained STAT3-ER cells were deprived of LIF for 36 hours,
stimulated with 4OHT (10 nM) or LIF (1x103 units/ml) and
assayed 24 hours later by RT-PCR analysis.
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