On with signaling proteins (32). Earlier operate has shown that a synthetic peptide containing the ICAM-1 ITIM was able to bind to Shp2 CYP1 Inhibitor Purity & Documentation phosphatase and this interaction was phosphorylation dependent (32). Since Shp2 interacted with the GMR receptor upon GM-CSF stimulation (33), we tested no matter if GMR connected with ICAM-1 through the Shp2 adaptor molecule. We studied the affinity of a peptide containing the ICAM-1 ITIM (RKIKKpY485RLQ) as a potential GMR-associating molecule in eosinophils by coprecipitation. Biotin-tagged peptides have been incubated with eosinophil lysates and complexed molecules have been pulled down utilizing streptavidin immobilized on agarose beads. Affinity-bound complexes had been then analyzed by Western immunoblotting. Both phosphorylated and nonphosphorylated versions of your peptide have been applied. Working with this peptide affinity-binding process, we identified that Shp-2 bound only for the phosphorylated ITIM-containing peptide (Fig. 4A); no binding was detected when the nonphosphorylated peptide was made use of. In contrast, the interaction of Shp2 with the ICAM-1 peptide didn’t ETA Antagonist site demand Shp2 phosphorylation for the reason that incubation of lysates from each GM-CSF-stimulated (with phosphorylated Shp2) and nonstimulated cells (containing nonphosphorylated Shp2) offered equivalent binding to the phosphorylated ICAM-1 peptide. On the other hand, interaction of GMR and ADAP with phosphorylated ICAM-1-derived peptide was detected only when lysates from stimulated eosinophils were utilized, suggesting that the interaction of your GMR and ADAP with ICAM-1 essential phosphorylated Shp2 and/or phosphorylated GMR (Fig. 4, B and C). Taken collectively, these final results supported the view that the tyrosinephosphorylated fragment of ICAM-1 can transduce the interaction with GMR by means of phosphorylated Shp2 phosphatase and/or phosphorylated GMR. Blockade of ICAM-1 expression inhibits GM-CSF-induced intracellular signaling and cytokine release and prolongation of eosinophil survival The observation that ICAM-1 expression correlated with the GM-CSF-induced inhibition of eosinophil apoptosis plus the previously reported requirement of ICAM-1 for eosinophil degranulation (six) led us to investigate no matter whether ICAM-1 played a function in GMR-induced eosinophil activation. To address this question, we inhibited expression of ICAM-1 utilizing a certain antisense oligonucleotide and investigated the ability of eosinophils to express cmyc and c-fos, transcription aspects involved in the inhibition of apoptosis (34, 35). Pretreatment of eosinophils with all the phosphorothioated antisense oligonucleotide ISISJ Immunol. Author manuscript; out there in PMC 2015 June 14.Author Manuscript Author Manuscript Author Manuscript Author ManuscriptPazdrak et al.Pageat 50 nM for 1 h before GM-CSF stimulation effectively prevented the expression of ICAM-1 24 h later, whereas handle sense oligonucleotide had no impact on ICAM-1 upregulation (Fig. 5A). Reprobing the blots with anti-c-fos revealed significant inhibition of cfos expression in ISIS 2302-treated cells, suggesting the requirement of ICAM-1 for c-fos induction by GM-CSF. A related effect of ICAM-1 inhibition was observed with c-myc induction, whereas there was no effect of ICAM-1 inhibition on a number of other signaling molecules investigated, notably ERK1 and ERK2. Since phosphorylation and activation of MAPKs had been proposed to transduce “outside-in” signaling from adhesion molecules (9), we tested the time course of ERK phosphorylation and its modulation by ICAM-1 inhibition. Western.