The Separation of Antler Polypeptide and Its Effects on the Proliferation and Osteogenetic Differentiation of Bone Marrow Mesenchymal Stem Cells

Author:

Wang Ping12,Sun Tie-Feng2,Li Gang1,Zhang Hui-Min2,Liu Fan-jie3,Gao Zhi-hui24,Cao Sheng-nan3,Sun Guo-dong5,Du Hai-tao4,Wang Cong-an3,Wang Dan-dan3ORCID,Shi Bin3ORCID,Lin Ling1ORCID

Affiliation:

1. State Key Laboratory of Precision Measurement Technology and Instruments, Tianjin University, Tianjin 300072, China

2. Shandong Academy of Chinese Medicine, Jinan 250014, China

3. Bone Biomechanics Engineering Laboratory of Shandong Province, Key Laboratory for Biotech-Drugs of National Health Commission, Neck-Shoulder and Lumbocrural Pain Hospital of Shandong First Medical University, Shandong Medicinal Biotechnology Center, Shandong First Medical University and Shandong Academy of Medical Sciences, Jinan 250062, China

4. School of Pharmaceutical Sciences, Shandong University of Traditional Chinese Medicine, Jinan 250355, China

5. Department of Traditional Chinese Medicine Orthopedics, The Third Affiliated Hospital of Shandong First Medical University, Shandong First Medical University and Shandong Academy of Medical Sciences, Jinan 250062, China

Abstract

Background. Colla Cornus Cervi (CCC) has been used as a traditional Chinese medicine in the treatment of osteoporosis and osteonecrosis of the femoral head. However, the bioavailability of CCC is seriously limited owing to its large molecular weight and complex ingredients. In the present study, antler polypeptide was separated from CCC, and the effects of antler polypeptide on rat bone marrow mesenchymal stem cells (BMSCs) were investigated. Methods. Antler polypeptide was separated from Colla Cornus Cervi by ultrafiltration into different samples according to the molecular weight. The total peptide content of these samples was determined by the biuret method. The content of antler polypeptide in different samples was quantified by high-performance liquid chromatography (HPLC). The effects of antler polypeptide at different concentrations on the proliferation, cell cycle, alkaline phosphatase activity, and BMP7 expression of BMSCs were investigated. Results. Antler polypeptide was separated by ultrafiltration into different samples: A (molecular weight <800 Da), B (molecular weight 800–1500 Da), and C (molecular weight >1500 Da). The total peptide contents of A, B, and C were 0.602 mg/mL, 8.976 mg/mL, and 38.88 mg/mL. Antler polypeptide B eluted at 14.279∼15.351 min showed that the content of antler polypeptide was significantly higher than that of A and C with a peak area of 933.80927. The BMSCs proliferation rate (84.66%) of polypeptide B was the highest at the concentration of 1.578 × 10−2 g/mL. Antler polypeptide B significantly promoted the proliferation of BMSCs with a proliferation index of 38.68%, which was significantly higher than that of the other groups. Antler polypeptide B significantly enhanced the activity of alkaline phosphatase in BMSCs compared to that of the blank group ( P < 0.001 ). Antler polypeptide B increased the BMP7 protein expression in BMSCs. Conclusions. Results suggested that antler polypeptide may promote the proliferation and osteogenic differentiation of BMSCs. Our study lays an experimental foundation for the further development and application of antler polypeptide in medicine.

Funder

Major Science and Technology Innovation Projects of Shandong Province

Publisher

Hindawi Limited

Subject

Complementary and alternative medicine

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