Department of Orthopaedics, Chinese People's Liberation Army General Hospital, Beijing 100853, P.R. China.
Division of Infection and Immunity, Department of Electromagnetic and Laser Biology, Beijing Institute of Radiation Medicine, Beijing 100850, P.R. China.
Int J Mol Med. 2018 Feb;41(2):800-808. doi: 10.3892/ijmm.2017.3270. Epub 2017 Nov 17.
Autophagy may be a major mechanism by which osteoblasts (OBs) protect against the negative effects of chronic glucocorticoid (GC) usage. OBs are closely associated with the remodeling that occurs in GC‑induced osteoporosis (GIO). In osteocytes, in response to stress induced by GCs, several pathways are activated, including cell necrosis, apoptosis and autophagy. However, the role of autophagy in OBs following treatment with excess GCs has not been addressed. In the current study, confocal microscopy observation of green fluorescent protein‑microtubule‑associated protein 1 light chain 3β (LC3) punctuate, and western blotting for LC3Ⅱ and Beclin 1 were performed for detection of autophagy in the MC3T3‑E1 osteoblastic cell line. Flow cytometry and western blotting were used for the examination of apoptosis and expression of BAX apoptosis regulator (Bax)/apoptosis regulator Bcl‑2 (Bcl‑2). The expression of genes associated with osteoblastic function, runt‑related transcription factor 2, α‑1 type 1 collagen and osteocalcin, were measured by reverse transcription‑quantitative polymerase chain reaction. The results indicated that autophagy was induced in OBs during dexamethasone (Dex) treatment in a dose‑dependent manner. The level of autophagy did not continue to increase over time, but peaked at 48 h and then decreased gradually. Subsequently, flow cytometry was used to demonstrate that inhibition of autophagy induced apoptosis in OBs under Dex treatment, and was associated with the upregulation of Bax and the downregulation of Bcl‑2 protein expression. Furthermore, the data suggested that the inhibition of autophagy also suppressed the expression of osteoblastic genes. By contrast, the stimulation of autophagy maintained the gene expression level under Dex treatment. The data revealed that autophagy is an important regulator of osteoblastic apoptosis through its interaction with Bax/Bcl‑2, and maintains the osteoblastic function of MC3T3‑E1 cells following GC exposure. In addition, these results indicated that the suppression of autophagy in OBs under chronic GC therapy may increase the prevalence of GIO and fragility fractures.
自噬可能是成骨细胞(OBs)抵抗慢性糖皮质激素(GC)使用负面影响的主要机制。OBs 与 GC 诱导的骨质疏松症(GIO)发生的重塑密切相关。在骨细胞中,GC 诱导的应激会激活几种途径,包括细胞坏死、凋亡和自噬。然而,GC 过量处理后 OB 中的自噬作用尚未得到解决。在本研究中,通过共聚焦显微镜观察绿色荧光蛋白-微管相关蛋白 1 轻链 3β(LC3)点状结构,并通过 Western blot 检测 LC3Ⅱ和 Beclin 1,以检测 MC3T3-E1 成骨细胞系中的自噬作用。流式细胞术和 Western blot 用于检测细胞凋亡和 BAX 凋亡调节因子(Bax)/凋亡调节 Bcl-2(Bcl-2)的表达。通过逆转录-定量聚合酶链反应测量与成骨细胞功能相关的基因的表达,包括 runt 相关转录因子 2、α-1 型 1 胶原和骨钙素。结果表明,在 Dex 处理 OBs 时,自噬呈剂量依赖性诱导。自噬水平不会随着时间的推移继续增加,而是在 48 小时达到峰值,然后逐渐下降。随后,流式细胞术用于证明 Dex 处理下抑制自噬会诱导 OBs 凋亡,并与 Bax 上调和 Bcl-2 蛋白表达下调有关。此外,数据表明抑制自噬也会抑制成骨细胞基因的表达。相比之下,刺激自噬可维持 Dex 处理下的基因表达水平。数据表明,自噬通过与 Bax/Bcl-2 的相互作用,是成骨细胞凋亡的重要调节剂,并维持 MC3T3-E1 细胞在 GC 暴露后的成骨细胞功能。此外,这些结果表明,慢性 GC 治疗下 OB 中自噬的抑制可能会增加 GIO 和脆性骨折的发生率。
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