Human interleukin-3 (IL-3) induces disulfide-linked IL-3 receptor alpha- and beta-chain heterodimerization, which is required for receptor activation but not high-affinity binding
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Stomski, FC
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机构:INST MED & VET SCI,HANSON CTR CANC RES,ADELAIDE,SA 5000,AUSTRALIA
Stomski, FC
Sun, Q
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机构:INST MED & VET SCI,HANSON CTR CANC RES,ADELAIDE,SA 5000,AUSTRALIA
Sun, Q
Bagley, CJ
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机构:INST MED & VET SCI,HANSON CTR CANC RES,ADELAIDE,SA 5000,AUSTRALIA
Bagley, CJ
Woodcock, J
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机构:INST MED & VET SCI,HANSON CTR CANC RES,ADELAIDE,SA 5000,AUSTRALIA
Woodcock, J
Goodall, G
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机构:INST MED & VET SCI,HANSON CTR CANC RES,ADELAIDE,SA 5000,AUSTRALIA
Goodall, G
Andrews, RK
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Andrews, RK
Berndt, MC
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Berndt, MC
Lopez, AF
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Lopez, AF
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[1] INST MED & VET SCI,HANSON CTR CANC RES,ADELAIDE,SA 5000,AUSTRALIA
The human interleukin-3 receptor (IL-3R) is a heterodimer that comprises an IL-3-specific alpha chain (IL-3R alpha) and a common beta chain (beta(c)) that is shared with the receptors for granulocyte-macrophage colony-stimulating factor (GM-CSF) and IL-5. These receptors belong to the cytokine receptor superfamily, but they are structurally and functionally more related to each other and thus make up a distinct subfamily. Although activation of the normal receptor occurs only in the presence of ligand, the underlying mechanisms are not known. We show here that human IL-3 induces heterodimerization of IL-3R alpha and beta(c) and that disulfide linkage of these chains is involved in receptor activation but not high-affinity binding. Monoclonal antibodies (MAb) to IL-3R alpha and beta(c) were developed which immunoprecipitated, in the absence of IL-3, the respective chains from cells labelled with I-125 On the cell surface. However, in the presence of IL-3, each MAb immunoprecipitated both IL-3R alpha and beta(c). IL-3-induced receptor dimers were disulfide and nondisulfide linked and were dependent on IL-3 interacting with both IL-3R alpha add beta(c). In the presence of IL-3 and under nonreducing conditions, MAb to either IL-3R alpha or beta(c) immunoprecipitated complexes with apparent molecular weights of 215,000 and 245,000 and IL-3R alpha and beta(c) monomers. Preincubation with iodoacetamide prevented the formation of the two high-molecular-w eight complexes without affecting noncovalent dimer formation or high-affinity IL-3 binding. Two-dimensional gel electrophoresis and Western blotting (immunoblotting) demonstrated the presence of both IL-3R alpha and beta(c) in the disulfide-linked complexes. IL-3 could also be coimmunoprecipitated with anti-IL-3R alpha or anti-beta(c) MAb, but it was not covalently attached to the receptor. Following IL-3 stimulation, only the disulfide-linked heterodimers exhibited reactivity with antiphosphotyrosine antibodies, with beta(c) but not IL-3R alpha being the phosphorylated species. A model of IL-3R activation is proposed which may be also applicable to the related GM-CSF and IL-5 receptors.
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
SILLABER, C
GEISSLER, K
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
GEISSLER, K
SCHERRER, R
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
SCHERRER, R
KALTENBRUNNER, R
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
KALTENBRUNNER, R
BETTELHEIM, P
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
BETTELHEIM, P
LECHNER, K
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
LECHNER, K
VALENT, P
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UNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIAUNIV VIENNA, DEPT MED 1, DIV HEMATOL, LAZARETTGASSE 14, A-1090 VIENNA, AUSTRIA
机构:
Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia
Murphy, James M.
Soboleva, Tatiana A.
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Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia
Soboleva, Tatiana A.
Mirza, Shamaruh
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Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia
Mirza, Shamaruh
Ford, Sally C.
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Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia
Ford, Sally C.
Olsen, Jane E.
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Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia
Olsen, Jane E.
Chen, Jinglong
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Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia
Chen, Jinglong
Young, Ian G.
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Australian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, AustraliaAustralian Natl Univ, John Curtin Sch Med Res, Div Mol Biosci, Canberra, ACT 0200, Australia