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11R-VIVIT肽抑制实验设计诱导的颅骨骨溶解。

11R-VIVIT Peptide Inhibits Calvaria Osteolysis Induced by Experimental Design.

作者信息

Li Maoqiang, Zhu Liulong, Wang Xuepeng, Bian Zhenyu, Yao Wangxiang, He Qifang, Tian Fei

机构信息

Department of Orthopaedics, Hangzhou First People's Hospital, Nanjing Medical University, Hangzhou, China.

出版信息

J Craniofac Surg. 2017 Mar;28(2):570-573. doi: 10.1097/SCS.0000000000002975.

Abstract

Wear particles released from prosthetic implants can cause periprosthetic osteolysis, a major cause of implant loosening. The aim of this study was to investigate the effects of the 11R-VIVIT peptide on osteolysis induced by titanium (Ti) particles in vivo. Twenty-four C57BL/J6 mice were divided into 3 groups: sham operation, Ti group, and Ti/VIVIT group. A calvarial osteolysis model was established by implanting Ti particles into mouse calvaria of the Ti and Ti/VIVIT groups. After 2 weeks, 11R-VIVIT peptide (10 mg/kg/day) was intraperitoneally injected into the mice of the Ti/VIVIT group for 14 days. The other 2 groups received saline injection. The calvarial specimens were removed and stained with van Geison staining. The calvarial sagittal suture area was measured to observe bone resorption. The calvarial new bone area was measured to observe bone formation. Compared with the sham group, the area of calvarial new bone and calvarial sagittal suture were higher in the Ti group (P < 0.01). Compared with the Ti group, the area of calvarial new bone was higher and the area of calvarial sagittal suture was lower in the Ti/VIVIT group (P < 0.01). In conclusion, the 11R-VIVIT peptide inhibited bone resorption and enhanced bone formation. This may have contributed to lower wear particle-induced osteolysis. This method could eventually be used to prevent prosthesis loosening after joint replacement and to prolong the life of the prosthesis.

摘要

人工关节植入物释放的磨损颗粒可导致假体周围骨溶解,这是植入物松动的主要原因。本研究旨在探讨11R-VIVIT肽对钛(Ti)颗粒在体内诱导的骨溶解的影响。将24只C57BL/J6小鼠分为3组:假手术组、Ti组和Ti/VIVIT组。通过将Ti颗粒植入Ti组和Ti/VIVIT组小鼠的颅骨建立颅骨骨溶解模型。2周后,将11R-VIVIT肽(10 mg/kg/天)腹腔注射到Ti/VIVIT组小鼠体内,持续14天。另外2组接受生理盐水注射。取出颅骨标本,用凡吉森染色法染色。测量颅骨矢状缝面积以观察骨吸收情况。测量颅骨新骨面积以观察骨形成情况。与假手术组相比,Ti组颅骨新骨面积和颅骨矢状缝面积更高(P<0.01)。与Ti组相比,Ti/VIVIT组颅骨新骨面积更高,颅骨矢状缝面积更低(P<0.01)。综上所述,11R-VIVIT肽抑制骨吸收并增强骨形成。这可能有助于降低磨损颗粒诱导的骨溶解。该方法最终可用于预防关节置换术后假体松动并延长假体使用寿命。

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