Dimerization of GPCRs: Novel insight into the role of FLNA and SSAs regulating SST2 and SST5 homo- and hetero-dimer formation

Donatella Treppiedi; Giusy Marra; Genesio Di Muro; Rosa Catalano; Federica Mangili; Emanuela Esposito; Davide Calebiro; Maura Arosio; Erika Peverelli; Giovanna Mantovani

doi:10.3389/fendo.2022.892668

Dimerization of GPCRs: Novel insight into the role of FLNA and SSAs regulating SST₂ and SST₅ homo- and hetero-dimer formation

Front Endocrinol (Lausanne). 2022 Aug 5:13:892668. doi: 10.3389/fendo.2022.892668. eCollection 2022.

Authors

Donatella Treppiedi¹, Giusy Marra¹, Genesio Di Muro^{1

2}, Rosa Catalano¹, Federica Mangili¹, Emanuela Esposito¹, Davide Calebiro^{3

4}, Maura Arosio^{1

5}, Erika Peverelli¹, Giovanna Mantovani^{1

5}

Affiliations

¹ Department of Clinical Sciences and Community Health, University of Milan, Milan, Italy.
² University Sapienza of Rome, Rome, Italy.
³ Institute of Metabolism and Systems Research, University of Birmingham, Birmingham, United Kingdom.
⁴ Centre of Membrane Proteins and Receptors, Universities of Birmingham and Nottingham, Birmingham, United Kingdom.
⁵ Endocrinology Unit, Fondazione Istituto di Ricovero e Cura a Carattere Scientifico (IRCCS) Ca' Granda Ospedale Maggiore Policlinico, Milan, Italy.

Abstract

The process of GPCR dimerization can have profound effects on GPCR activation, signaling, and intracellular trafficking. Somatostatin receptors (SSTs) are class A GPCRs abundantly expressed in pituitary tumors where they represent the main pharmacological targets of somatostatin analogs (SSAs), thanks to their antisecretory and antiproliferative actions. The cytoskeletal protein filamin A (FLNA) directly interacts with both somatostatin receptor type 2 (SST₂) and 5 (SST₅) and regulates their expression and signaling in pituitary tumoral cells. So far, the existence and physiological relevance of SSTs homo- and hetero-dimerization in the pituitary have not been explored. Moreover, whether octreotide or pasireotide may play modulatory effects and whether FLNA may participate to this level of receptor organization have remained elusive. Here, we used a proximity ligation assay (PLA)-based approach for the in situ visualization and quantification of SST₂/SST₅ dimerization in rat GH3 as well as in human melanoma cells either expressing (A7) or lacking (M2) FLNA. First, we observed the formation of endogenous SST₅ homo-dimers in GH3, A7, and M2 cells. Using the PLA approach combined with epitope tagging, we detected homo-dimers of human SST₂ in GH3, A7, and M2 cells transiently co-expressing HA- and SNAP-tagged SST₂. SST₂ and SST₅ can also form endogenous hetero-dimers in these cells. Interestingly, FLNA absence reduced the basal number of hetero-dimers (-36.8 ± 6.3% reduction of PLA events in M2, P < 0.05 vs. A7), and octreotide but not pasireotide promoted hetero-dimerization in both A7 and M2 (+20.0 ± 11.8% and +44.1 ± 16.3% increase of PLA events in A7 and M2, respectively, P < 0.05 vs. basal). Finally, immunofluorescence data showed that SST₂ and SST₅ recruitment at the plasma membrane and internalization are similarly induced by octreotide and pasireotide in GH3 and A7 cells. On the contrary, in M2 cells, octreotide failed to internalize both receptors whereas pasireotide promoted robust receptor internalization at shorter times than in A7 cells. In conclusion, we demonstrated that in GH3 cells SST₂ and SST₅ can form both homo- and hetero-dimers and that FLNA plays a role in the formation of SST₂/SST₅ hetero-dimers. Moreover, we showed that FLNA regulates SST₂ and SST₅ intracellular trafficking induced by octreotide and pasireotide.

Keywords: FLNA; GPCR dimerization; SST2; SST5; in situ PLA; somatostatin analogs.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Dimerization
Filamins / metabolism
Humans
Octreotide* / metabolism
Octreotide* / pharmacology
Pituitary Neoplasms* / pathology
Rats
Somatostatin

Substances

FLNA protein, human
Filamins
Somatostatin
Octreotide