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Abstract
The effect of autophosphorylation on the tyrosine kinase activity of the epidermal growth factor receptor (EGFR) is not well understood. We previously demonstrated that phospholipase C-gamma physically associates with the EGF-activated EGFR, but not with a kinase-negative mutant of the EGFR, and, moreover, that only the tyrosine-phosphorylated EGFR is able to associate with phospholipase C-gamma. We have now investigated the effect of autophosphorylation on the tyrosine kinase activity of the EGFR by employing the purified kinase-active intracellular domain of the EGFR (EGFR-IC) produced by a baculovirus expression system. Synthetic peptides, including ones which contain the individual major tyrosine phosphorylation sites of phospholipase C-gamma, were used as substrates. We found that the extensively prephosphorylated EGFR-IC exhibited similar reaction kinetics to the unphosphorylated EGFR-IC when angiotensin II was used as a nonspecific substrate. In contrast there was a clear stimulation of kinase activity due to autophosphorylation of the EGFR-IC when peptides representing either the major autophosphorylation site of the EGFR or the EGFR phosphorylation sites of phospholipase C-gamma were used as substrates. However, the modes of stimulation for these peptides differed. The binding affinity (Km) for the unphosphorylated EGFR-IC for the peptide containing Tyr-771 of phospholipase C-gamma was relatively poor compared with other peptides, but improved 5-6-fold when the EGFR-IC was prephosphorylated. On the other hand, autophosphorylation improved the reaction velocity (Vm) of the phosphorylation of other peptides by 2-3-fold, with little or no increase in affinity. These results suggest that autophosphorylation of the EGFR may induce a conformational change of its kinase domain which enhances its kinase activity with exogenous substrates and may induce association with phospholipase C-gamma by increasing its affinity to a domain containing Tyr-771.
Highlights
The effect of autophosphorylation on the tyrosine domain within its cytoplasmic portion
The tyrosine kinase kinase activityof the epidermal growth factor receptaocrtivity is essential for receptor-related signal transduction (EGFR) is not well understood.We previously demon- as well asintracellularrouting of the receptor (1)
We found that of theEGFR is requiredfor its ability to associatewith the extensively prephosphorylated epidermal growth factor receptor (EGFR)-IC exhibited phospholipase C - r in a cell-free reaction (8).These results similar eactionkineticstotheunphosphorylated suggest that autophosphorylationof the EGFR may enhance
Summary
Sequences of phospholipase C-y peptides containing tyrosine of receptor autophosphorylation on its tyroskiinnease activity phosphovlation sites with various peptide substrates. Phe-Arg-Ile experiment, we used low levels of kinase (40 nM) and excess substrate (300 p ~ )T.he prephosphorylationreaction It has beensuggested (22, 25) that an important role of the autophosphorylation sitesof the EGFR is to compete with exogenous substrates and serve an intrinsic negative regulatory function in the phosphorylation of these exogenous substrates. The results reported in this study show that, in addition, autophosphorylation haas positive regulatory effect It increases either the binding affinity or the reaction velocity of the EGFR for different tyrosine phosphorylation sites of phospholipase The extent of phosphorylation of peptide K 1 by theP-EGFR-IC was -70%
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