Identification of a Critical Ligand Binding Determinant of the Human Erythropoietin Receptor

Middleton, Steven A.; Johnson, Dana L.; Jin, Renzhe; McMahon, Frank J.; Collins, Alexander; Tullai, Jennifer; Gruninger, Robert H.; Jolliffe, Linda K.; Mulcahy, Linda S.

doi:10.1074/jbc.271.24.14045

Cited by 50 publications

(56 citation statements)

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“…The W40A mutation was then expressed as a full-length EPOR in COS cells and failed to bind EPO in the whole cell binding assay (Table I). Further investigation of this mutant full-length receptor utilizing a radiolabeled antibody cell surface detection method (15) revealed no detectable cell surface expression of the W40A full-length receptor (data not shown). These data suggest that W40A is a critical structural determinant of the EPOR.…”

Section: Resultsmentioning

confidence: 99%

“…Generally, our approach was to screen for mutations resulting in decreased EPO binding activity by testing crude preparations of the mutant EBPs in a high performance-size exclusion chromatography (HP-SEC) assay (16). Although not quantitative, the HP-SEC assay does not require purification of the mutant proteins, is quick and easy to perform, and is capable of identifying mutations resulting in large reductions in EPO binding (15,16). This assay was successful in identifying an EBP mutant with a 1,000-fold increased IC 50 for EPO (15); however, it may not be sensitive enough to detect less dramatic effects on EPO binding, since an EBP mutant (L96A-EBP) with a 200-fold increased IC 50 for EPO still showed EPO binding.…”

Section: Resultsmentioning

confidence: 99%

“…Although not quantitative, the HP-SEC assay does not require purification of the mutant proteins, is quick and easy to perform, and is capable of identifying mutations resulting in large reductions in EPO binding (15,16). This assay was successful in identifying an EBP mutant with a 1,000-fold increased IC 50 for EPO (15); however, it may not be sensitive enough to detect less dramatic effects on EPO binding, since an EBP mutant (L96A-EBP) with a 200-fold increased IC 50 for EPO still showed EPO binding. Following HP-SEC analysis, selected mutant proteins were purified and analyzed in competition binding assays or expressed and characterized as full-length receptor on the surface of COS cells.…”

Section: Resultsmentioning

confidence: 99%

“…Detection of EPOR on the surface of COS cells was performed using an anti-EBP monoclonal antibody in a modification of the receptor binding assay described above. This procedure for cell surface detection has been described previously (15).…”

Section: Methodsmentioning

confidence: 99%

“…Previously, we reported that a single residue, Phe 93 , is a critical ligand binding determinant of the EPOR (15). Here, in a more extensive mutagenesis analysis of the 225-amino acid extracellular domain of the EPOR, we report the effect on EPO binding of single amino acid substitutions created by sitespecific mutagenesis.…”

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confidence: 87%

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Mutagenesis Studies of the Human Erythropoietin Receptor

Barbone¹,

Middleton²,

Johnson³

et al. 1997

Journal of Biological Chemistry

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Mutagenesis of the erythropoietin receptor (EPOR)permits analysis of the contribution that individual amino acid residues make to erythropoietin (EPO) binding. We employed both random and site-specific mutagenesis to determine the function of amino acid residues in the extracellular domain (referred to as EPO binding protein, EBP) of the EPOR. Residues were chosen for site-specific alanine substitution based on the results of the random mutagenesis or on their homology to residues that are conserved or have been reported to be involved in ligand binding in other receptors of the cytokine receptor family. Site-specific mutants were expressed in Escherichia coli as soluble EBP and analyzed for EPO binding in several different assay formats. In addition, selected mutant proteins were expressed as full-length EPOR on the surface of COS cells and analyzed for 125 I-EPO binding in receptor binding assays. Using these methods, we have identified residues that appear to be involved in EPO binding as well as other residues, most of which are conserved in receptors of the cytokine receptor family, that appear to be necessary for the proper folding and/or stability of the EPOR. We present correlations between these mutagenesis data and the recently solved crystal structure of the EBP with a peptide ligand.Erythropoietin (EPO) 1 is a glycoprotein hormone that functions as the primary regulator of erythropoiesis by binding a specific receptor (EPOR) on the surface of erythrocyte precursor cells, signaling their proliferation and differentiation into mature red blood cells (reviewed in Ref. 1). The human EPOR is a 484-amino acid glycoprotein comprised of extracellular and cytoplasmic domains of nearly equal size and a single transmembrane domain (2). The extracellular domain of the EPOR contains a 225-amino acid region referred to as the cytokine receptor homology (CRH) domain that shares conserved features with an expanding family of cytokine and growth factor receptors (3, 4) including the receptors for many interleukins (IL), colony stimulating factors, growth hormone (GH), thrombopoietin, leptin, interferons (IFN), and tissue factor among others. The CRH domains consist of two motifs of approximately 100 amino acids each that are structurally related to fibronectin type III domains. Based on this homology, Bazan (3, 4) proposed that the CRH domains consist of two motifs of seven ␤-strands each which adopt ␤-sheet structures with fibronectin type III-like or immunoglobulin (Ig)-like folds. These structural predictions have been confirmed by the solution of the crystal structures of the ligand-bound extracellular domains of the GH receptor and IFN-␥ receptor ␣ (IFN-␥R␣), the GH bound extracellular domain of the prolactin receptor, the extracellular domain of tissue factor, and most recently, the extracellular domain of the EPOR with a peptide ligand (5-10). Alignment of the CRH domains of this family of receptors based on their predicted ␤-strand secondary structural elements reveals several conserved characteristics (3, 4,...

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Section: Resultsmentioning

confidence: 99%