Phosphorylation of Thr{sup 654} but not Thr{sup 669} within the juxtamembrane domain of the EGF receptor inhibits calmodulin binding

Phosphorylation of Thr{sup 654} but not Thr{sup 669} within the juxtamembrane domain of the EGF receptor inhibits calmodulin binding

Calcium-calmodulin (CaM) binding to the epidermal growth factor receptor (EGFR) has been shown to both inhibit and stimulate receptor activity. CaM binds to the intracellular juxtamembrane (JM) domain (Met{sup 645}-Phe{sup 688}) of EGFR. Protein kinase C (PKC) mediated phosphorylation of Thr{sup 654...

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Veröffentlicht in:Biochemical and biophysical research communications 2006-08, Vol.347 (2)
Hauptverfasser: Aifa, Sami, Centre of Biotechnology of Sfax, BP'K'3038 Sfax, Frikha, Fakher, Miled, Nabil, Johansen, Knut, Lundstroem, Ingemar, Svensson, Samuel P.S.
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60 APPLIED LIFE SCIENCES
CALCIUM
CALMODULIN
ESCHERICHIA COLI
GROWTH FACTORS
HYPOTHESIS
MUTANTS
PHOSPHORYLATION
RECEPTORS
THREONINE
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container_issue 2
container_start_page
container_title Biochemical and biophysical research communications
container_volume 347
creator Aifa, Sami
Centre of Biotechnology of Sfax, BP'K'3038 Sfax
Frikha, Fakher
Miled, Nabil
Johansen, Knut
Lundstroem, Ingemar
Svensson, Samuel P.S.
description Calcium-calmodulin (CaM) binding to the epidermal growth factor receptor (EGFR) has been shown to both inhibit and stimulate receptor activity. CaM binds to the intracellular juxtamembrane (JM) domain (Met{sup 645}-Phe{sup 688}) of EGFR. Protein kinase C (PKC) mediated phosphorylation of Thr{sup 654} occurs within this domain. CaM binding to the JM domain inhibits PKC phosphorylation and conversely PKC mediated phosphorylation of Thr{sup 654} or Glu substitution of Thr{sup 654} inhibits CaM binding. A second threonine residue (Thr{sup 669}) within the JM domain is phosphorylated by the mitogen-activated protein kinase (MAPK). Previous results have shown that CaM interferes with EGFR-induced MAPK activation. If and how phosphorylation of Thr{sup 669} affects CaM-EGFR interaction is however not known.In the present study we have used surface plasmon resonance (BIAcore) to study the influence of Thr{sup 669} phosphorylation on real time interactions between the intracellular juxtamembrane (JM) domain of EGFR and CaM. The EGFR-JM was expressed as GST fusion proteins in Escherichia coli and phosphorylation was mimicked by generating Glu substitutions of either Thr{sup 654} or Thr{sup 669}. Purified proteins were coupled to immobilized anti-GST antibodies at the sensor surface and increasing concentration of CaM was applied. When mutating Thr{sup 654} to Glu{sup 654} no specific CaM binding could be detected. However, neither single substitutions of Thr{sup 669} (Gly{sup 669} or Glu{sup 669}) nor double mutants Gly{sup 654}/Gly{sup 669} or Gly{sup 654}/Glu{sup 669} influenced the binding of CaM to the EGFR-JM. This clearly shows that PKC may regulate EGF-mediated CaM signalling through phosphorylation of Thr{sup 654} whereas phosphorylation of Thr{sup 669} seems to play a CaM independent regulatory role. The role of both residues in the EGFR-calmodulin interaction was also studied in silico. Our modelling work supports a scenario where Thr{sup 654} from the JM domain interacts with Glu{sup 12} in the calmodulin molecule. Phosphorylation of Thr{sup 654} or Glu{sup 654} substitution creates a repulsive electrostatic force that would diminish CaM binding to the JM domain. These results are in line with the Biacore experiments showing a weak binding of the CaM to the JM domain with Thr{sup 654} mutated to Glu. Furthermore, these results provide a hypothesis to how CaM binding to EGFR might both positively and negatively interfere with EGFR-activity.
doi_str_mv 10.1016/j.bbrc.2006.05.200
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CaM binds to the intracellular juxtamembrane (JM) domain (Met{sup 645}-Phe{sup 688}) of EGFR. Protein kinase C (PKC) mediated phosphorylation of Thr{sup 654} occurs within this domain. CaM binding to the JM domain inhibits PKC phosphorylation and conversely PKC mediated phosphorylation of Thr{sup 654} or Glu substitution of Thr{sup 654} inhibits CaM binding. A second threonine residue (Thr{sup 669}) within the JM domain is phosphorylated by the mitogen-activated protein kinase (MAPK). Previous results have shown that CaM interferes with EGFR-induced MAPK activation. If and how phosphorylation of Thr{sup 669} affects CaM-EGFR interaction is however not known.In the present study we have used surface plasmon resonance (BIAcore) to study the influence of Thr{sup 669} phosphorylation on real time interactions between the intracellular juxtamembrane (JM) domain of EGFR and CaM. The EGFR-JM was expressed as GST fusion proteins in Escherichia coli and phosphorylation was mimicked by generating Glu substitutions of either Thr{sup 654} or Thr{sup 669}. Purified proteins were coupled to immobilized anti-GST antibodies at the sensor surface and increasing concentration of CaM was applied. When mutating Thr{sup 654} to Glu{sup 654} no specific CaM binding could be detected. However, neither single substitutions of Thr{sup 669} (Gly{sup 669} or Glu{sup 669}) nor double mutants Gly{sup 654}/Gly{sup 669} or Gly{sup 654}/Glu{sup 669} influenced the binding of CaM to the EGFR-JM. This clearly shows that PKC may regulate EGF-mediated CaM signalling through phosphorylation of Thr{sup 654} whereas phosphorylation of Thr{sup 669} seems to play a CaM independent regulatory role. The role of both residues in the EGFR-calmodulin interaction was also studied in silico. Our modelling work supports a scenario where Thr{sup 654} from the JM domain interacts with Glu{sup 12} in the calmodulin molecule. Phosphorylation of Thr{sup 654} or Glu{sup 654} substitution creates a repulsive electrostatic force that would diminish CaM binding to the JM domain. These results are in line with the Biacore experiments showing a weak binding of the CaM to the JM domain with Thr{sup 654} mutated to Glu. 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CaM binds to the intracellular juxtamembrane (JM) domain (Met{sup 645}-Phe{sup 688}) of EGFR. Protein kinase C (PKC) mediated phosphorylation of Thr{sup 654} occurs within this domain. CaM binding to the JM domain inhibits PKC phosphorylation and conversely PKC mediated phosphorylation of Thr{sup 654} or Glu substitution of Thr{sup 654} inhibits CaM binding. A second threonine residue (Thr{sup 669}) within the JM domain is phosphorylated by the mitogen-activated protein kinase (MAPK). Previous results have shown that CaM interferes with EGFR-induced MAPK activation. If and how phosphorylation of Thr{sup 669} affects CaM-EGFR interaction is however not known.In the present study we have used surface plasmon resonance (BIAcore) to study the influence of Thr{sup 669} phosphorylation on real time interactions between the intracellular juxtamembrane (JM) domain of EGFR and CaM. The EGFR-JM was expressed as GST fusion proteins in Escherichia coli and phosphorylation was mimicked by generating Glu substitutions of either Thr{sup 654} or Thr{sup 669}. Purified proteins were coupled to immobilized anti-GST antibodies at the sensor surface and increasing concentration of CaM was applied. When mutating Thr{sup 654} to Glu{sup 654} no specific CaM binding could be detected. However, neither single substitutions of Thr{sup 669} (Gly{sup 669} or Glu{sup 669}) nor double mutants Gly{sup 654}/Gly{sup 669} or Gly{sup 654}/Glu{sup 669} influenced the binding of CaM to the EGFR-JM. This clearly shows that PKC may regulate EGF-mediated CaM signalling through phosphorylation of Thr{sup 654} whereas phosphorylation of Thr{sup 669} seems to play a CaM independent regulatory role. The role of both residues in the EGFR-calmodulin interaction was also studied in silico. Our modelling work supports a scenario where Thr{sup 654} from the JM domain interacts with Glu{sup 12} in the calmodulin molecule. Phosphorylation of Thr{sup 654} or Glu{sup 654} substitution creates a repulsive electrostatic force that would diminish CaM binding to the JM domain. These results are in line with the Biacore experiments showing a weak binding of the CaM to the JM domain with Thr{sup 654} mutated to Glu. 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CaM binds to the intracellular juxtamembrane (JM) domain (Met{sup 645}-Phe{sup 688}) of EGFR. Protein kinase C (PKC) mediated phosphorylation of Thr{sup 654} occurs within this domain. CaM binding to the JM domain inhibits PKC phosphorylation and conversely PKC mediated phosphorylation of Thr{sup 654} or Glu substitution of Thr{sup 654} inhibits CaM binding. A second threonine residue (Thr{sup 669}) within the JM domain is phosphorylated by the mitogen-activated protein kinase (MAPK). Previous results have shown that CaM interferes with EGFR-induced MAPK activation. If and how phosphorylation of Thr{sup 669} affects CaM-EGFR interaction is however not known.In the present study we have used surface plasmon resonance (BIAcore) to study the influence of Thr{sup 669} phosphorylation on real time interactions between the intracellular juxtamembrane (JM) domain of EGFR and CaM. The EGFR-JM was expressed as GST fusion proteins in Escherichia coli and phosphorylation was mimicked by generating Glu substitutions of either Thr{sup 654} or Thr{sup 669}. Purified proteins were coupled to immobilized anti-GST antibodies at the sensor surface and increasing concentration of CaM was applied. When mutating Thr{sup 654} to Glu{sup 654} no specific CaM binding could be detected. However, neither single substitutions of Thr{sup 669} (Gly{sup 669} or Glu{sup 669}) nor double mutants Gly{sup 654}/Gly{sup 669} or Gly{sup 654}/Glu{sup 669} influenced the binding of CaM to the EGFR-JM. This clearly shows that PKC may regulate EGF-mediated CaM signalling through phosphorylation of Thr{sup 654} whereas phosphorylation of Thr{sup 669} seems to play a CaM independent regulatory role. The role of both residues in the EGFR-calmodulin interaction was also studied in silico. Our modelling work supports a scenario where Thr{sup 654} from the JM domain interacts with Glu{sup 12} in the calmodulin molecule. Phosphorylation of Thr{sup 654} or Glu{sup 654} substitution creates a repulsive electrostatic force that would diminish CaM binding to the JM domain. These results are in line with the Biacore experiments showing a weak binding of the CaM to the JM domain with Thr{sup 654} mutated to Glu. Furthermore, these results provide a hypothesis to how CaM binding to EGFR might both positively and negatively interfere with EGFR-activity.</abstract><cop>United States</cop><doi>10.1016/j.bbrc.2006.05.200</doi></addata></record>
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subjects 60 APPLIED LIFE SCIENCES
CALCIUM
CALMODULIN
ESCHERICHIA COLI
GROWTH FACTORS
HYPOTHESIS
MUTANTS
PHOSPHORYLATION
RECEPTORS
THREONINE
title Phosphorylation of Thr{sup 654} but not Thr{sup 669} within the juxtamembrane domain of the EGF receptor inhibits calmodulin binding
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