TRIM33 protects osteoblasts from oxidative stress‐induced apoptosis in osteoporosis by inhibiting FOXO3a ubiquitylation and degradation

TRIM33 protects osteoblasts from oxidative stress‐induced apoptosis in osteoporosis by inhibiting FOXO3a ubiquitylation and degradation

This study aimed to probe into the effect of TRIM33 on oxidative stress‐induced apoptosis of osteoblasts in osteoporosis and to probe into the underlying mechanism. The apoptosis of osteoblasts was induced by H2O2 treatment and tested by flow cytometry. A mouse osteoporosis model was conducted by ov...

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Veröffentlicht in:Aging cell 2021-07, Vol.20 (7), p.e13367-n/a, Article 13367
Hauptverfasser: Zou, De‐bo, Mou, Zongyou, Wu, Wenliang, Liu, Haichun
Format: Artikel
Sprache:eng
Schlagworte:
3T3 Cells
Acetylation
Animals
Apoptosis
Apoptosis - physiology
Bone mineral density
Cell Biology
Degradation
Experiments
Female
Flow cytometry
Forkhead Box Protein O3 - antagonists & inhibitors
Forkhead Box Protein O3 - metabolism
FOXO3 protein
FOXO3a
Geriatrics & Gerontology
Humans
Hydrogen peroxide
Immunoprecipitation
Life Sciences & Biomedicine
Mice
Original
Osteoblasts
Osteoblasts - metabolism
Osteoblasts - pathology
Osteoporosis
Osteoporosis - metabolism
Osteoporosis - pathology
Ovariectomy
Oxidative stress
Oxidative Stress - physiology
Patients
Science & Technology
Transcription Factors - metabolism
Transfection
TRIM33
Ubiquitin
Ubiquitination
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Zusammenfassung:This study aimed to probe into the effect of TRIM33 on oxidative stress‐induced apoptosis of osteoblasts in osteoporosis and to probe into the underlying mechanism. The apoptosis of osteoblasts was induced by H2O2 treatment and tested by flow cytometry. A mouse osteoporosis model was conducted by ovariectomy (OVX). The function of TRIM33 was assessed by in vitro and in vivo experiments. The mechanism of TRIM33 was determined by immunoprecipitation, immunofluorescent staining and co‐transfection experiments. Here, we found that TRIM33 expression was lessened in the osteoblasts of patients with osteoporosis and was positively correlated with the bone mineral density of these patients. FOXO3a and TRIM33 were co‐localized in the osteoblasts nuclei. TRIM33 silence boosted FOXO3a degradation in normal osteoblasts, while TRIM33 overexpression restrained FOXO3a degradation in H2O2‐treated osteoblasts. The binding of TRIM33 to CBP and its overexpression restrained CBP‐mediated FOXO3a acetylation, thereby attenuating FOXO3a ubiquitylation. The H2O2‐induced apoptosis of osteoblasts was restrained by TRIM33 overexpression, while the FOXO3a knockdown reversed this trend. The in vivo experiments corroborated that TRIM33 overexpression attenuated the OVX‐driven impacts in mice. In general, our findings expounded that TRIM33 protected osteoblasts against oxidative stress‐induced apoptosis in osteoporosis and that the underlying mechanism was the restraint of FOXO3a ubiquitylation and degradation. The mechanism flow diagram to a better understanding of the pivotal role of TRIM33. In the presence of oxidative stress, the expression of TRIM33 in osteoblasts was lessened and the lessened TRIM33 further boosted the acetylation modification of FOXO3a by CBP, thereby boosting the ubiquitination and degradation of FOXO3a protein, and boosting the oxidative stress and apoptosis of osteoblasts and aggravating osteoporosis.
ISSN:1474-9718
1474-9726
DOI:10.1111/acel.13367