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PINK1 deficiency impairs osteoblast differentiation through aberrant mitochondrial homeostasis

DC Field Value Language
dc.contributor.authorLee, So-Young-
dc.contributor.authorAn, Hyun-Ju-
dc.contributor.authorKim, Jin Man-
dc.contributor.authorSung, Min-Ji-
dc.contributor.authorKim, Do Kyung-
dc.contributor.authorKim, Hyung Kyung-
dc.contributor.authorOh, Jongbeom-
dc.contributor.authorJeong, Hye Yun-
dc.contributor.authorLee, Yu Ho-
dc.contributor.authorYang, Taeyoung-
dc.contributor.authorKim, Jun Han-
dc.contributor.authorLim, Ha Jeong-
dc.contributor.authorLee, Soonchul-
dc.date.accessioned2022-03-16T04:49:47Z-
dc.date.available2022-03-16T13:57:51Z-
dc.date.issued2021-11-25-
dc.identifier.citationStem Cell Research & Therapy. 2021 Nov 25;12(1):589ko_KR
dc.identifier.issn1757-6512-
dc.identifier.urihttps://hdl.handle.net/10371/177016-
dc.description.abstractBackground
PTEN-induced kinase 1 (PINK1) is a serine/threonine-protein kinase in mitochondria that is critical for mitochondrial quality control. PINK1 triggers mitophagy, a selective autophagy of mitochondria, and is involved in mitochondrial regeneration. Although increments of mitochondrial biogenesis and activity are known to be crucial during differentiation, data regarding the specific role of PINK1 in osteogenic maturation and bone remodeling are limited.

Methods
We adopted an ovariectomy model in female wildtype and Pink1−/− mice. Ovariectomized mice were analyzed using micro-CT, H&E staining, Massons trichrome staining. RT-PCR, western blot, immunofluorescence, alkaline phosphatase, and alizarin red staining were performed to assess the expression of PINK1 and osteogenic markers in silencing of PINK1 MC3T3-E1 cells. Clinical relevance of PINK1 expression levels was determined via qRT-PCR analysis in normal and osteoporosis patients.

Results
A significant decrease in bone mass and collagen deposition was observed in the femurs of Pink1−/− mice after ovariectomy. Ex vivo, differentiation of osteoblasts was inhibited upon Pink1 downregulation, accompanied by impaired mitochondrial homeostasis, increased mitochondrial reactive oxygen species production, and defects in mitochondrial calcium handling. Furthermore, PINK1 expression was reduced in bones from patients with osteoporosis, which supports the practical role of PINK1 in human bone disease.

Conclusions
In this study, we demonstrated that activation of PINK1 is a requisite in osteoblasts during differentiation, which is related to mitochondrial quality control and low reactive oxygen species production. Enhancing PINK1 activity might be a possible treatment target in bone diseases as it can promote a healthy pool of functional mitochondria in osteoblasts.
ko_KR
dc.description.sponsorshipSo-Young Lee received National Research Foundation Grant of Korea (NRF2019R1A2C4070492), funded by the Korean government (https://www.nrf.re.kr) for this work. Soonchul Lee received National Research Foundation Grant of Korea (NRF-2019R1C1C1004017), funded by the Korean government (https://www.nrf.re.kr) for this work.ko_KR
dc.language.isoenko_KR
dc.publisherBMCko_KR
dc.subjectMitochondria-
dc.subjectOsteogenesis-
dc.subjectOsteoporosis-
dc.subjectPINK1-
dc.titlePINK1 deficiency impairs osteoblast differentiation through aberrant mitochondrial homeostasisko_KR
dc.typeArticleko_KR
dc.contributor.AlternativeAuthor이소영-
dc.contributor.AlternativeAuthor안현주-
dc.contributor.AlternativeAuthor김진만-
dc.contributor.AlternativeAuthor성민지-
dc.contributor.AlternativeAuthor김도경-
dc.contributor.AlternativeAuthor김형경-
dc.contributor.AlternativeAuthor오종범-
dc.contributor.AlternativeAuthor정혜윤-
dc.contributor.AlternativeAuthor이유호-
dc.contributor.AlternativeAuthor양태형-
dc.contributor.AlternativeAuthor김준한-
dc.contributor.AlternativeAuthor임하정-
dc.contributor.AlternativeAuthor이순철-
dc.identifier.doihttps://doi.org/10.1186/s13287-021-02656-4-
dc.citation.journaltitleStem Cell Research & Therapyko_KR
dc.language.rfc3066en-
dc.rights.holderThe Author(s)-
dc.date.updated2021-11-28T04:16:10Z-
dc.citation.number1ko_KR
dc.citation.startpage589ko_KR
dc.citation.volume12ko_KR
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