Characterization of internalization, recycling and downregulation of muscarinic receptors

Muscarinic receptors mediate the responses elicited to the activation of the parasympathetic nervous system. Specifically, muscarinic receptors mediate exocrine glandular secretion, smooth muscle contraction and decreased heart rate and contractile force. Five subtypes of muscarinic receptors have been cloned and they undergo a process of agonist-dependent regulation, which involves desensitization, internalization, recycling and downregulation. This study was designed to characterize the kinetics and extent of internalization, recycling and downregulation of muscarinic receptors expressed individually in CHO cells and to identify subtype-specific differences in these processes. The mechanisms of downregulation of muscarinic receptors expressed in CHO cells were also investigated by using proteasomal and lysosomal inhibitors. Additionally, deletion mutations were made in the third intracellular loop and C-terminal tail region of the muscarinic M1 receptor to identify regions responsible for recycling or downregulation.;There are subtype-specific differences in the internalization, recycling and downregulation of muscarinic receptors. The rank order for carbachol-induced internalization was M2 > M4 = M5 > M 3 = M1. Unlike M2 receptors, M1, M 3, M4 and M5 receptors recycled back to the plasma membrane following 1 h carbachol treatment. M1 receptor downregulated to a greater extent compared to other subtypes. The downregulation of M1, M3, M4 and M5 receptors was affected by proteasomal inhibitors, while lysosomal inhibitors affected the downregulation of M2 and M4 receptors. The M 1 deletion mutants (M1 del 276-282 and M1 del 447-459) signaled through activation of phospholipase C activation and were able to bind to [3H]NMS. Additionally, the internalization of M1 deletion mutants was indifferent from those of the wild-type M1 receptor. However, both deletion mutants had an impaired recycling and downregulation. The C-terminal deletion (K447-Q459) significantly affected the downregulation of M1 receptor, suggesting a role of this domain in mediating M1 receptor downregulation.