RhoB plays a central role in hyperosmolarity‐induced cell shrinkage in renal cells

Author:

Centrone Mariangela1,Saltarella Ilaria2,D'Agostino Mariagrazia1,Ranieri Marianna1,Venneri Maria3,Di Mise Annarita1,Simone Laura4,Pisani Francesco1,Valenti Giovanna1,Frassanito Maria A.5,Tamma Grazia1ORCID

Affiliation:

1. Department of Biosciences Biotechnologies and Environment University of Bari Aldo Moro Bari Italy

2. Department of Precision and Regenerative Medicine and Ionian Area, Section of Pharmacology, School of Medicine University of Bari Aldo Moro Bari Italy

3. Istituti Clinici Scientifici Maugeri SPA SB IRCCS Bari Italy

4. Fondazione IRCCS Casa Sollievo della Sofferenza, Cancer Stem Cells Unit San Giovanni Rotondo Italy

5. Department of Precision and Regenerative Medicine and Ionian Area, Section of Clinical Pathology University of Bari Aldo Moro Bari Italy

Abstract

AbstractThe small Rho GTP‐binding proteins are important cell morphology, function, and apoptosis regulators. Unlike other Rho proteins, RhoB can be subjected to either geranylgeranylation (RhoB‐GG) or farnesylation (RhoB‐F), making that the only target of the farnesyltransferase inhibitor (FTI). Fluorescence resonance energy transfer experiments revealed that RhoB is activated by hyperosmolarity. By contrast, hyposmolarity did not affect RhoB activity. Interestingly, treatment with farnesyltransferase inhibitor‐277 (FTI‐277) decreased the cell size. To evaluate whether RhoB plays a role in volume reduction, renal collecting duct MCD4 cells and Human Kidney, HK‐2 were transiently transfected with RhoB‐wildtype‐Enhance Green Fluorescence Protein (RhoB‐wt‐EGFP) and RhoB‐CLLL‐EGFP which cannot undergo farnesylation. A calcein‐based fluorescent assay revealed that hyperosmolarity caused a significant reduction of cell volume in mock and RhoB‐wt‐EGFP‐expressing cells. By contrast, cells treated with FTI‐277 or expressing the RhoB‐CLLL‐EGFP mutant did not properly respond to hyperosmolarity with respect to mock and RhoB‐wt‐EGFP expressing cells. These findings were further confirmed by 3D‐LSCM showing that RhoB‐CLLL‐EGFP cells displayed a significant reduction in cell size compared to cells expressing RhoB‐wt‐EGFP. Moreover, flow cytometry analysis revealed that RhoB‐CLLL‐EGFP expressing cells as well as FTI‐277‐treated cells showed a significant increase in cell apoptosis. Together, these data suggested that: (i) RhoB is sensitive to hyperosmolarity and not to hyposmolarity; (ii) inhibition of RhoB farnesylation associates with an increase in cell apoptosis, likely suggesting that RhoB might be a paramount player controlling apoptosis by interfering with responses to cell volume change.

Publisher

Wiley

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