TY - JOUR
T1 - PMEPA1 and NEDD4 control the proton production of osteoclasts by regulating vesicular trafficking
AU - Hirata, Hirohito
AU - Xu, Xianghe
AU - Nishioka, Kenichi
AU - Matsuhisa, Fumikazu
AU - Kitajima, Shuji
AU - Kukita, Toshio
AU - Murayama, Masatoshi
AU - Urano, Yasuteru
AU - Miyamoto, Hiroshi
AU - Mawatari, Masaaki
AU - Kukita, Akiko
N1 - Funding Information:
The authors thank Drs. Makoto Shiraki and Asana Kamohara for assistance, Dr Akemi Ito (Ito Bone Science Institute) for performing the histomorphometric analysis, Drs. Toshifumi Mawatari and Yoshiki Sato for assisting LEXT OLS4000 confocal microscope analysis, and Editage for English language editing. Analysis with LSM 880 confocal fluorescence microscopy was conducted at Analytical Research Center for Experimental Science, Saga University. µCT analysis of spines and LEXT OLS4000 confocal microscope analysis were the results of using research equipment shared in MEXT Project for promoting public utilization of advanced research infrastructure (Program for supporting introduction of the new sharing system) Grant Number JPMXS0422400020. The authors also thank Ms Kanae Mori and Ms Yuka Tokuyama of Analytical Research Center for their advice and help. This work was supported by Japan Society for the Promotion of Science Grants‐in‐Aid for Scientific Research (KAKENHI) (C) (15K11046 to A. K. and 16K10908 to M. Mawatari).
Funding Information:
MEXT Japan Society for the Promotion of Science, Grant/Award Number: 15K11046 and 16K10908 The authors thank Drs. Makoto Shiraki and Asana Kamohara for assistance, Dr Akemi Ito (Ito Bone Science Institute) for performing the histomorphometric analysis, Drs. Toshifumi Mawatari and Yoshiki Sato for assisting LEXT OLS4000 confocal microscope analysis, and Editage for English language editing. Analysis with LSM 880 confocal fluorescence microscopy was conducted at Analytical Research Center for Experimental Science, Saga University. ?CT analysis of spines and LEXT OLS4000 confocal microscope analysis were the results of using research equipment shared in MEXT Project for promoting public utilization of advanced research infrastructure (Program for supporting introduction of the new sharing system) Grant Number JPMXS0422400020. The authors also thank Ms Kanae Mori and Ms Yuka Tokuyama of Analytical Research Center for their advice and help. This work was supported by Japan Society for the Promotion of Science Grants-in-Aid for Scientific Research (KAKENHI) (C) (15K11046 to A. K. and 16K10908 to M. Mawatari).
Publisher Copyright:
© 2021 Federation of American Societies for Experimental Biology
PY - 2021/2
Y1 - 2021/2
N2 - Osteoclast bone resorption activity is critically regulated to maintain bone homeostasis. Osteoclasts resorb bone by producing protons and acid hydrolase via lysosomal secretion, however, a detailed mechanism remains elusive. PMEPA1 is a vesicular membrane protein, which binds to the NEDD4 family member of ubiquitin ligases. We have previously reported that Pmepa1 is highly expressed in bone resorbing osteoclasts, and regulates bone resorption. Here, we investigated the mechanism of bone resorption regulated by PMEPA1. Mutant mice lacking NEDD4-binding domains of PMEPA1 displayed enhanced bone volume, and reduced bone resorption activity in comparison with those of WT mice. Analysis with pH-sensitive fluorescence probe revealed that proton secretion from osteoclasts significantly decreased in Pmepa1 mutant osteoclasts. Immunofluorescence analysis revealed that PMEPA1 was colocalized with NEDD4, V0A3, and V0D2 subunits of vacuolar ATPase, which regulate the proton production of osteoclasts. In addition, Nedd4 knockdown reduced bone resorption and proton secretion of osteoclasts. Furthermore, Pmepa1 mutation and Nedd4 knockdown altered the cytoplasmic distribution of components of V-ATPase and expression of autophagy-related proteins, suggesting that lysosomal secretion is affected. Collectively, these findings indicate that PMEPA1 controls proton secretion from osteoclasts via NEDD4 by regulating vesicular trafficking, and NEDD4 is an important regulator of bone resorption.
AB - Osteoclast bone resorption activity is critically regulated to maintain bone homeostasis. Osteoclasts resorb bone by producing protons and acid hydrolase via lysosomal secretion, however, a detailed mechanism remains elusive. PMEPA1 is a vesicular membrane protein, which binds to the NEDD4 family member of ubiquitin ligases. We have previously reported that Pmepa1 is highly expressed in bone resorbing osteoclasts, and regulates bone resorption. Here, we investigated the mechanism of bone resorption regulated by PMEPA1. Mutant mice lacking NEDD4-binding domains of PMEPA1 displayed enhanced bone volume, and reduced bone resorption activity in comparison with those of WT mice. Analysis with pH-sensitive fluorescence probe revealed that proton secretion from osteoclasts significantly decreased in Pmepa1 mutant osteoclasts. Immunofluorescence analysis revealed that PMEPA1 was colocalized with NEDD4, V0A3, and V0D2 subunits of vacuolar ATPase, which regulate the proton production of osteoclasts. In addition, Nedd4 knockdown reduced bone resorption and proton secretion of osteoclasts. Furthermore, Pmepa1 mutation and Nedd4 knockdown altered the cytoplasmic distribution of components of V-ATPase and expression of autophagy-related proteins, suggesting that lysosomal secretion is affected. Collectively, these findings indicate that PMEPA1 controls proton secretion from osteoclasts via NEDD4 by regulating vesicular trafficking, and NEDD4 is an important regulator of bone resorption.
UR - http://www.scopus.com/inward/record.url?scp=85100326067&partnerID=8YFLogxK
UR - http://www.scopus.com/inward/citedby.url?scp=85100326067&partnerID=8YFLogxK
U2 - 10.1096/fj.202001795R
DO - 10.1096/fj.202001795R
M3 - Article
C2 - 33484199
AN - SCOPUS:85100326067
SN - 0892-6638
VL - 35
JO - FASEB Journal
JF - FASEB Journal
IS - 2
M1 - e21281
ER -