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Functional Regulation of P2X6 Receptors by N-Linked Glycosylation: Identification of a Novel αβ-Methylene ATP-Sensitive Phenotype
Investigation of rat recombinant P2X 6 receptors has been limited because of the difficulty in obtaining functional expression in heterologous systems. In this study, we demonstrate glycosylation-dependent regulation of recombinant P2X 6 receptor function and associated conferral of a novel phenotyp...
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| Published in: | Molecular pharmacology 2004-04, Vol.65 (4), p.979 |
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| Main Authors: | , , , , , |
| Format: | Article |
| Language: | English |
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| container_issue | 4 |
| container_start_page | 979 |
| container_title | Molecular pharmacology |
| container_volume | 65 |
| creator | Clare A. Jones Catherine Vial Lynda A. Sellers Pat P. A. Humphrey Richard J. Evans Iain P. Chessell |
| description | Investigation of rat recombinant P2X 6 receptors has been limited because of the difficulty in obtaining functional expression in heterologous systems. In this
study, we demonstrate glycosylation-dependent regulation of recombinant P2X 6 receptor function and associated conferral of a novel phenotype that is sensitive to the P2X 1 and P2X 3 receptor agonist, αβ-methylene ATP. In cells functionally expressing P2X 6 receptors, ATP and αβ-methylene ATP evoked slowly desensitizing inward currents (EC 50 values, 0.5 and 0.6 μM, respectively) with slow kinetics of current decay on agonist washout. 2â²,3â²- O -(2,4,6-trinitrophenyl ATP) and iso-pyridoxalphosphate-6-azophenyl-2â²-5â²-disulfonate were effective antagonists (IC 50 values, 0.8 and 22 μM, respectively); however, suramin was relatively ineffective. Reverse transcription-polymerase chain
reaction analysis confirmed the absence of other P2X receptor subunits. Western analysis of membrane fractions from functional
and nonfunctional clones confirmed the presence of P2X 6 at the cell membrane but revealed a difference in apparent molecular mass of immunoreactive products (â¼70 and â¼60 kDa, respectively).
N -glycosidase F treatment of both functional and nonfunctional receptor cell membranes increased the electrophoretic mobilities
of immunoreactive products, with both proteins migrating at â¼55 kDa, demonstrating an increased level of glycosylation of
the P2X 6 receptor in functional compared with nonfunctional cells. This study demonstrates that nonfunctional rat recombinant P2X 6 receptors 1) are expressed on the membrane surface of human embryonic kidney cells and 2) are glycosylated. Expression of
the novel functional receptor phenotype is associated with further glycosylation, resulting in an apparently larger molecular
mass. These results suggest that P2X 6 receptor subunits contribute to αβ-methylene ATP sensitivity. |
| doi_str_mv | 10.1124/mol.65.4.979 |
| format | article |
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study, we demonstrate glycosylation-dependent regulation of recombinant P2X 6 receptor function and associated conferral of a novel phenotype that is sensitive to the P2X 1 and P2X 3 receptor agonist, αβ-methylene ATP. In cells functionally expressing P2X 6 receptors, ATP and αβ-methylene ATP evoked slowly desensitizing inward currents (EC 50 values, 0.5 and 0.6 μM, respectively) with slow kinetics of current decay on agonist washout. 2â²,3â²- O -(2,4,6-trinitrophenyl ATP) and iso-pyridoxalphosphate-6-azophenyl-2â²-5â²-disulfonate were effective antagonists (IC 50 values, 0.8 and 22 μM, respectively); however, suramin was relatively ineffective. Reverse transcription-polymerase chain
reaction analysis confirmed the absence of other P2X receptor subunits. Western analysis of membrane fractions from functional
and nonfunctional clones confirmed the presence of P2X 6 at the cell membrane but revealed a difference in apparent molecular mass of immunoreactive products (â¼70 and â¼60 kDa, respectively).
N -glycosidase F treatment of both functional and nonfunctional receptor cell membranes increased the electrophoretic mobilities
of immunoreactive products, with both proteins migrating at â¼55 kDa, demonstrating an increased level of glycosylation of
the P2X 6 receptor in functional compared with nonfunctional cells. This study demonstrates that nonfunctional rat recombinant P2X 6 receptors 1) are expressed on the membrane surface of human embryonic kidney cells and 2) are glycosylated. Expression of
the novel functional receptor phenotype is associated with further glycosylation, resulting in an apparently larger molecular
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study, we demonstrate glycosylation-dependent regulation of recombinant P2X 6 receptor function and associated conferral of a novel phenotype that is sensitive to the P2X 1 and P2X 3 receptor agonist, αβ-methylene ATP. In cells functionally expressing P2X 6 receptors, ATP and αβ-methylene ATP evoked slowly desensitizing inward currents (EC 50 values, 0.5 and 0.6 μM, respectively) with slow kinetics of current decay on agonist washout. 2â²,3â²- O -(2,4,6-trinitrophenyl ATP) and iso-pyridoxalphosphate-6-azophenyl-2â²-5â²-disulfonate were effective antagonists (IC 50 values, 0.8 and 22 μM, respectively); however, suramin was relatively ineffective. Reverse transcription-polymerase chain
reaction analysis confirmed the absence of other P2X receptor subunits. Western analysis of membrane fractions from functional
and nonfunctional clones confirmed the presence of P2X 6 at the cell membrane but revealed a difference in apparent molecular mass of immunoreactive products (â¼70 and â¼60 kDa, respectively).
N -glycosidase F treatment of both functional and nonfunctional receptor cell membranes increased the electrophoretic mobilities
of immunoreactive products, with both proteins migrating at â¼55 kDa, demonstrating an increased level of glycosylation of
the P2X 6 receptor in functional compared with nonfunctional cells. This study demonstrates that nonfunctional rat recombinant P2X 6 receptors 1) are expressed on the membrane surface of human embryonic kidney cells and 2) are glycosylated. Expression of
the novel functional receptor phenotype is associated with further glycosylation, resulting in an apparently larger molecular
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study, we demonstrate glycosylation-dependent regulation of recombinant P2X 6 receptor function and associated conferral of a novel phenotype that is sensitive to the P2X 1 and P2X 3 receptor agonist, αβ-methylene ATP. In cells functionally expressing P2X 6 receptors, ATP and αβ-methylene ATP evoked slowly desensitizing inward currents (EC 50 values, 0.5 and 0.6 μM, respectively) with slow kinetics of current decay on agonist washout. 2â²,3â²- O -(2,4,6-trinitrophenyl ATP) and iso-pyridoxalphosphate-6-azophenyl-2â²-5â²-disulfonate were effective antagonists (IC 50 values, 0.8 and 22 μM, respectively); however, suramin was relatively ineffective. Reverse transcription-polymerase chain
reaction analysis confirmed the absence of other P2X receptor subunits. Western analysis of membrane fractions from functional
and nonfunctional clones confirmed the presence of P2X 6 at the cell membrane but revealed a difference in apparent molecular mass of immunoreactive products (â¼70 and â¼60 kDa, respectively).
N -glycosidase F treatment of both functional and nonfunctional receptor cell membranes increased the electrophoretic mobilities
of immunoreactive products, with both proteins migrating at â¼55 kDa, demonstrating an increased level of glycosylation of
the P2X 6 receptor in functional compared with nonfunctional cells. This study demonstrates that nonfunctional rat recombinant P2X 6 receptors 1) are expressed on the membrane surface of human embryonic kidney cells and 2) are glycosylated. Expression of
the novel functional receptor phenotype is associated with further glycosylation, resulting in an apparently larger molecular
mass. These results suggest that P2X 6 receptor subunits contribute to αβ-methylene ATP sensitivity.</abstract><pub>American Society for Pharmacology and Experimental Therapeutics</pub><pmid>15044628</pmid><doi>10.1124/mol.65.4.979</doi></addata></record> |
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| ispartof | Molecular pharmacology, 2004-04, Vol.65 (4), p.979 |
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| language | eng |
| recordid | cdi_highwire_pharmacology_65_4_979 |
| source | Free Full-Text Journals in Chemistry |
| title | Functional Regulation of P2X6 Receptors by N-Linked Glycosylation: Identification of a Novel αβ-Methylene ATP-Sensitive Phenotype |
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