The interaction of a chimeric EGF containing the C-tail of TGFa with the EGF receptor reveals hidden ligand complexities
The interaction of a chimeric EGF containing the C-tail of TGFa with the EGF receptor reveals hidden ligand complexities
It has been assumed that substitution of homologous regions of TGFû into EGF can be used to probe ligand:receptor recognition without detrimental effects on ligand characteristics for the human EGFR. We show that a chimera of EGF in which the C-tail is substituted for that of TGFa results in complex features which belie this initial simplistic assumption. Comparison of EGF and the chimera in equilibrium binding assays showed that the relative binding affinity of the chimera was reduced 60 fold. Surprisingly, the chimera was more potent than EGF in mitogenesis assays using NR6/HER cells. This superagonist activity appeared to be due, in part, to choice of an EGFR overexpressing target cell where high receptor number compensated for the low affinity of the ligand. However, the enhanced mitogenic activity relative to EGF suggested a further unusual property of the chimera. Examination of EGFR tyrosine kinase activity showed that the chimera was at least as potent as EGF, despite its low affinity. Our results suggest a contextual requirement for EGFR recognition which is ligand specific. Further, the unpredictable responses to chimeric Hgands underlines the complex nature of the processes of ligand recognition, receptor activation and the ensuing cellular response.
A1376
Puddicombe, S.
124e2c4e-ab9a-46f3-855c-b54ed0b61cc4
Wood, L.
b7a3f367-e500-429f-adb4-38640e4b7ad4
Chamberlin, S.
65db4a68-a5ba-4110-b511-1a85f297c47a
Davies, D.
7de8fdc7-3640-4e3a-aa91-d0e03f990c38
1996
Puddicombe, S.
124e2c4e-ab9a-46f3-855c-b54ed0b61cc4
Wood, L.
b7a3f367-e500-429f-adb4-38640e4b7ad4
Chamberlin, S.
65db4a68-a5ba-4110-b511-1a85f297c47a
Davies, D.
7de8fdc7-3640-4e3a-aa91-d0e03f990c38
Puddicombe, S., Wood, L., Chamberlin, S. and Davies, D.
(1996)
The interaction of a chimeric EGF containing the C-tail of TGFa with the EGF receptor reveals hidden ligand complexities.
FASEB Journal, 10 (6), .
Abstract
It has been assumed that substitution of homologous regions of TGFû into EGF can be used to probe ligand:receptor recognition without detrimental effects on ligand characteristics for the human EGFR. We show that a chimera of EGF in which the C-tail is substituted for that of TGFa results in complex features which belie this initial simplistic assumption. Comparison of EGF and the chimera in equilibrium binding assays showed that the relative binding affinity of the chimera was reduced 60 fold. Surprisingly, the chimera was more potent than EGF in mitogenesis assays using NR6/HER cells. This superagonist activity appeared to be due, in part, to choice of an EGFR overexpressing target cell where high receptor number compensated for the low affinity of the ligand. However, the enhanced mitogenic activity relative to EGF suggested a further unusual property of the chimera. Examination of EGFR tyrosine kinase activity showed that the chimera was at least as potent as EGF, despite its low affinity. Our results suggest a contextual requirement for EGFR recognition which is ligand specific. Further, the unpredictable responses to chimeric Hgands underlines the complex nature of the processes of ligand recognition, receptor activation and the ensuing cellular response.
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Published date: 1996
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Local EPrints ID: 468613
URI: http://eprints.soton.ac.uk/id/eprint/468613
ISSN: 0892-6638
PURE UUID: cb94a517-194f-4841-a490-cafff6468157
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Date deposited: 18 Aug 2022 17:03
Last modified: 19 Aug 2022 01:31
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Author:
S. Puddicombe
Author:
L. Wood
Author:
S. Chamberlin
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