Bradykinin-induced Internalization of the Human B2Receptor Requires Phosphorylation of Three Serine and Two Threonine Residues at Its Carboxyl Tail

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RESEARCH PRODUCT

Bradykinin-induced Internalization of the Human B2Receptor Requires Phosphorylation of Three Serine and Two Threonine Residues at Its Carboxyl Tail

François Alhenc-gelas Werner Müller-esterl Anne Pizard Andree Blaukat Rabary M. Rajerison

subject

Threonine Receptor Bradykinin B2 media_common.quotation_subject Molecular Sequence Data CHO Cells Biology Bradykinin Transfection Biochemistry Cell Line Serine Cricetinae Serine Animals Humans 5-HT5A receptor Amino Acid Sequence Phosphorylation Internalization Receptor Molecular Biology Peptide sequence DNA Primers media_common Base Sequence Receptors Bradykinin Coated Pits Cell-Membrane Cell Biology Interleukin-13 receptor Clathrin Endocytosis Recombinant Proteins Cell biology Kinetics Biochemistry COS Cells Phosphorylation Signal transduction

description

The binding of bradykinin (BK) to B2 receptor triggers the internalization of the agonist-receptor complex. To investigate the mechanisms and the receptor structures involved in this fundamental process of receptor regulation, the human B2 receptor was mutated within its cytoplasmic tail by complementary strategies of truncation, deletion, and amino acid substitution. Ligand binding, signal transduction, internalization as well as phosphorylation were studied for the mutated receptors expressed in COS, CHO, and HEK 293 cells. Truncation of 44 out of 55 amino acid residues of the receptor's cytoplasmic tail corresponding to positions 321-364 did not alter the kinetics of BK binding and the receptor coupling to phospholipase C and phospholipase A2. By contrast, truncations after positions 320 and 334, deletions within the segment covering positions 335-351, as well as alanine substitution of serine and threonine residues within segment 335-351 diminished the internalization capacity of the mutant receptors. Mutants with a markedly reduced internalization potential failed to produce BK-induced receptor phosphorylation suggesting that phosphorylation may be involved in receptor internalization. The mutagenesis approaches converged at the conclusion that three serines in positions 339, 346, and 348 and two threonines in positions 342 and 345, contained in a sequence segment that is highly conserved between species, have a critical role in the ligand-dependent internalization and phosphorylation of kinin receptors and can intervene in these processes in an alternative manner. However, mutants lacking these residues were still sensitive to dominant-negative forms of beta-arrestin and dynamin, suggesting the existence of additional receptor structure(s) involved in the receptor sequestration through clathrin-coated vesicles.

year	journal	country	edition	language
1999-04-23	Journal of Biological Chemistry

https://doi.org/10.1074/jbc.274.18.12738