Institute of Orthopaedics and Traumatology, The First Affiliated Hospital of Zhejiang Chinese Medical University (Zhejiang Provincial Hospital of Chinese Medicine), Hangzhou, 310053, People's Republic of China.
School of Pharmaceutical Sciences, Zhejiang Chinese Medical University, Hangzhou, 310053, People's Republic of China.
Int J Nanomedicine. 2024 Nov 21;19:12389-12407. doi: 10.2147/IJN.S483621. eCollection 2024.
Infected bone defects pose a challenging clinical issue due to an imbalance of osteoclasts (OC) and osteoblasts (OB). Exosomes are crucial for intercellular signaling of OC and OB in bone repair. Icariin, has been shown to regulate the balance between OC and OB. However, the specific mechanisms by which icariin influences exosomes derived from osteoclasts, and subsequently impacts osteoblast activity, remain unclear. This study aims to investigate the effects of icariin-treated osteoclast-derived exosomes (ICA-OC-Exo) on osteoblast function and bone repair in cases of infected bone defects.
We investigated the exosome profile and localization of multivesicular bodies (MVB) and quantification of intraluminal vesicles (ILVs) in osteoclasts by using transmission electron microscopy. Additionally, the expressions of Rab27A and MITF, which are associated with exosome release, were determined through immunofluorescence staining and Western blot. The profiling of exosomal miRNA expression was conducted via miRNA-sequencing. The effects of ICA-OC-Exo on osteoblast differentiation were determined using RT-qPCR, Western blot, alkaline phosphatase staining. Additionally, ICA-OC-Exo was administered into the localized bone defect of the infected bone rat models, and bone formation was assessed using Micro-CT.
Icariin increased the presence of MVBs in the cytoplasm through modulation of the MITF/Rab27A signaling pathway, resulting in higher number of ICA-OC-Exo compared to OC-Exo. Additionally, miR-331-3p expression in ICA-OC-Exo was found to be elevated compared to OC-Exo. ICA-OC-Exo was observed to stimulate osteoblast function by targeting FGF23, reducing DKK1, and subsequently upregulating ALP. In the in vivo study, ICA-OC-Exo exhibited the capacity to enhance bone healing at the site of a local bone defect following anti-infection treatment.
Icariin enhanced the quantification of OC-Exo and the expression of miRNA-331-3p in OC-Exo, leading to the regulation of osteoblast function via activation of the miRNA-331-3p/FGF23/DKK1 pathway. ICA-OC-Exo demonstrated potential clinical applicability in bone repair of infected bone defects.
感染性骨缺损是一个具有挑战性的临床问题,其涉及到破骨细胞(OC)和成骨细胞(OB)之间的失衡。外泌体在骨修复过程中对于 OC 和 OB 的细胞间信号传递至关重要。淫羊藿苷已被证明可以调节 OC 和 OB 之间的平衡。然而,淫羊藿苷影响破骨细胞衍生的外泌体(ICA-OC-Exo),进而影响成骨细胞活性的具体机制尚不清楚。本研究旨在探讨淫羊藿苷处理的破骨细胞衍生外泌体(ICA-OC-Exo)对感染性骨缺损中骨修复的成骨细胞功能的影响。
我们通过透射电子显微镜观察骨细胞中外泌体的特征和多泡体(MVB)的定位,以及对腔内小泡(ILVs)的定量。此外,通过免疫荧光染色和 Western blot 确定与外泌体释放相关的 Rab27A 和 MITF 的表达。通过 miRNA-seq 对外泌体 miRNA 表达谱进行分析。通过 RT-qPCR、Western blot、碱性磷酸酶染色来确定 ICA-OC-Exo 对成骨细胞分化的影响。此外,将 ICA-OC-Exo 注入感染性骨大鼠模型的局部骨缺损部位,并通过 Micro-CT 评估骨形成。
淫羊藿苷通过调节 MITF/Rab27A 信号通路增加了细胞质中 MVB 的存在,导致 ICA-OC-Exo 数量多于 OC-Exo。此外,ICA-OC-Exo 中的 miR-331-3p 表达高于 OC-Exo。ICA-OC-Exo 通过靶向 FGF23 刺激成骨细胞功能,降低 DKK1,从而上调 ALP。在体内研究中,ICA-OC-Exo 在抗感染治疗后局部骨缺损部位表现出增强骨愈合的能力。
淫羊藿苷增强了 OC-Exo 的定量和 OC-Exo 中 miRNA-331-3p 的表达,通过激活 miRNA-331-3p/FGF23/DKK1 通路调节成骨细胞功能。ICA-OC-Exo 在感染性骨缺损的骨修复中具有潜在的临床应用价值。
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