包虫抗原 B 通过抑制 TAZ 促进 RANKL / NF-κB / TAK1 介导的破骨细胞发生 #br#

doi:10.3870/j.issn.1672-8009.2025.01.002

医学分子生物学杂志 ›› 2025, Vol. 22 ›› Issue (1): 8-15.doi: 10.3870/j.issn.1672-8009.2025.01.002

包虫抗原 B 通过抑制 TAZ 促进 RANKL / NF-κB / TAK1 介导的破骨细胞发生 #br#

新疆医科大学第一附属医院创伤骨科乌鲁木齐市, 830011

出版日期:2025-01-31 发布日期:2025-02-28
基金资助:
新疆维吾尔自治区自然科学基金 (No. 2021D01D19)

Hydatid Antigen B Promote RANKL / NF-κB / TAK1-mediated Osteoclastogenesis via Inhibition of TAZ #br#

Department of Trauma and Orthopedics, First Affiliated Hospital of Xinjiang Medical University, Urumqi, 830011, China

Online:2025-01-31 Published:2025-02-28

摘要/Abstract

摘要： 目的探讨包虫抗原 B (hydatid antigen-B, Hyd-B) 促进破骨细胞发生的分子机制。方法细胞实验分组-1: BMSCs 细胞分为 Control 组、 MCSF + RANKL 组和 MCSF + RANKL + Hyd-B 组; 使用巨噬细胞集落刺激因子 (macrophage colony-stimulating factor, MCSF) 联合可溶性核因子 κ B 受体激活配体 ( receptor activator of nuclear factor-κb ligand, RANKL), 外加/ 不加 Hyd-B 联合诱导骨髓间充质干细胞 ( bone marrow mesenchymal stem cells, BMSCs) 向破骨细胞分化。细胞实验分组-2: BMSCs 细胞分为 Ctrl 组和 Hyd-B 处理组 (Treat 组)。免疫共沉淀 (co-IP) 法测定 Hyd-B 对 TAZ (transcriptional coactivator with PDZ-binding motif)和 TAK1 (transforming growth factor β-activated kinase 1) 的直接相互作用的影响, 使用抗 TAK1 抗体进行 IP、IB 检测 TAZ 的表达。细胞实验分组-3: BMSCs 细胞分为 Control 组、 MCSF + RANKL 组、 MCSF + RANKL + Hyd-B 组、 MCSF + RANKL + Hyd-B + TAZ-OE 组和 MCSF + RANKL + Hyd-B + OE-vector 组。 BMSCs 转染腺病毒-TAZ OE 或腺病毒-OE vector 介导过表达 TAZ。 qPCR 法检测破骨细胞分化标志物 TRAP 和 Cathepsin K mRNA 相对表达水平。蛋白质印迹检测细胞核 p-P65、细胞质 P65、细胞核 NFATc1、 p-AKT、 AKT、 p-ERK1 / 2、 ERK 1 / 2、 p-TAZ、 TAZ 和 TAK1 的表达水平。结果与 Control 组比较, MCSF + RANKL 组和 MCSF +RANKL + Hyd-B 组细胞 TRAP 和 Cathepsin K mRNA 水平升高 (P< 0. 05); p-P65、 p-AKT、 p-ERK 1 / 2 水平升高 (P< 0. 05); 细胞核内 p-P65 和 NFATc1 的水平升高 (P< 0. 05)。与 MCSF + RANKL 组相比较, MCSF+ RANKL + Hyd-B 组细胞上述指标表达水平进一步升高 (P< 0. 05)。与 MCSF + RANKL + Hyd-B 组相比较,MCSF + RANKL + Hyd-B + TAZ OE 组细胞上述指标表达水平降低 ( P< 0. 05)。 Co-IP 结果, 与 Ctrl 组相比较, Treat 组中 TAZ 与 TAK1 的相互作用增加 (P< 0. 05)。与 Ctrl 组相比较, Treat 组中细胞质 p-TAZ 磷酸化水平增加 (P< 0. 05), TAZ 表达水平降低 ( P< 0. 05)。结论 Hyd-B 通过抑制 TAZ 上调 RANKL / NF-κB /TAK1 介导的破骨细胞发生。

关键词: 骨包虫病, 包虫抗原 B, RANKL / NF-κB / TAK1, TAZ, 破骨细胞分化

Abstract: Objective To investigate the molecular mechanisms of hydatid antigen-B (Hyd-B) in osteoclastogenesis. Methods Cell experiment group-1: Bone marrow mesenchymal stem cells(BMSCs) were divided into 3 groups (Control group, MCSF + RANKL group, MCSF + RANKL + Hyd-B group), cells in the MCSF + RANKL group and MCSF + RANKL + Hyd-B group were induced to differentiate into osteoclasts by using macrophage colony-stimulating factor (MCSF) combined with soluble receptor activator of nuclear factor-κb ligand (RANKL), and then treated with or without Hyd-B respectively. Cell experiment group-2: BMSCs were divided into Ctrl group and Hyd-B treatment group (Treat group), the effect of Hyd-B on the direct interaction between TAZ and TAK1 was determined by co-immunoprecipitation ( co-IP). IP was performed by using antiTAK1 antibody, and TAZ expression level was detected by IB. Cell experiment group-3: BMSCs were divided into 5 groups: Control group, MCSF + RANKL group, MCSF + RANKL + Hyd-B group, MCSF + RANKL + Hyd-B + TAZ-OE group and MCSF + RANKL + Hyd-B + OE-vector group. TAZ overexpression plasmid or vector plasmid was transfected to the BMSCs in the MCSF + RANKL + Hyd-B + TAZ-OE group and MCSF + RANKL + Hyd-B + OE-vector group respectively. qPCR was used to detect the mRNA expression levels of osteoclast differentiation markers of TRAP and Cathepsin K. Western blotting was used to detect the expression levels of nuclear p-P65, cytoplasmic P65, nuclear NFATc1, p-AKT, AKT, p-ERK 1 / 2, ERK 1 / 2, p-TAZ, TAZ and TAK1. Results Compared with those in the Control group, the TRAP and Cathepsin K mRNA expression levels in the MCSF + RANKL and MCSF + RANKL + Hyd-B groups were increased (P <0. 05); the expression levels of p-P65, p-AKT and p-ERK 1 / 2 were increased (P < 0. 05); theexpression levels of p-P65 and NFATc1 in nucleus were increased (P < 0. 05). The expression levels of the above indicators were further increased in the MCSF + RANKL + Hyd-B group when compared with those in the MCSF + RANKL group ( P < 0. 05). Compared with those in the MCSF +RANKL + Hyd-B group, the expression levels of the above indicators in MCSF + RANKL + Hyd-B +TAZ-OE group were all reduced (P < 0. 05). Co-IP results showed that Hyd-B treatment enhancedthe interaction between TAZ and TAK1 ( P < 0. 05). Compared with those in the Ctrl group, thephosphorylated level of cytoplasmic TAZ in Treat group was increased, the expression level of TAZwas reduced (P< 0. 05). Conclusion Hyd-B can promot the RANKL / NF-κB / TAK1-mediated osteoclastogenesis through inhibition of TAZ.

Key words:

bone cystic echinococcosis, hydatid antigen B, RANKL / NF-κB / TAK1, transcriptional coactivator with PDZ-binding motif, osteoclastogenesis

中图分类号:

R532. 32
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吾路汗· 马汗, 谢增如. 包虫抗原 B 通过抑制 TAZ 促进 RANKL / NF-κB / TAK1 介导的破骨细胞发生 #br#[J]. 医学分子生物学杂志, 2025, 22(1): 8-15.

Wuluhan Mahan, XIE Zengru. Hydatid Antigen B Promote RANKL / NF-κB / TAK1-mediated Osteoclastogenesis via Inhibition of TAZ #br#[J]. Journal of Medical Molecular Biology, 2025, 22(1): 8-15.

包虫抗原 B 通过抑制 TAZ 促进 RANKL / NF-κB / TAK1 介导的破骨细胞发生 #br#

Hydatid Antigen B Promote RANKL / NF-κB / TAK1-mediated Osteoclastogenesis via Inhibition of TAZ #br#

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