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In vitro effects of alendronate on fibroblasts of the human rotator cuff tendonopen access

Authors
Sung, Chang-MeenKim, Ra JeongHah, Young-SoolGwark, Ji-YongPark, Hyung Bin
Issue Date
11-Jan-2020
Publisher
BMC
Keywords
Human rotator cuff tendon fibroblasts; Alendronate; Wound healing
Citation
BMC MUSCULOSKELETAL DISORDERS, v.21, no.1
Indexed
SCIE
SCOPUS
Journal Title
BMC MUSCULOSKELETAL DISORDERS
Volume
21
Number
1
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/7013
DOI
10.1186/s12891-019-3014-1
ISSN
1471-2474
1471-2474
Abstract
Background Bone mineral density of the humeral head is an independent determining factor for postoperative rotator cuff tendon healing. Bisphosphonates, which are commonly used to treat osteoporosis, have raised concerns regarding their relationships to osteonecrosis of the jaw and to atypical fracture of the femur. In view of the prevalence of rotator cuff tear in osteoporotic elderly people, it is important to determine whether bisphosphonates affect rotator cuff tendon healing. However, no studies have investigated bisphosphonates' cytotoxicity to human rotator cuff tendon fibroblasts (HRFs) or bisphosphonates' effects on rotator cuff tendon healing. The purpose of this study was to evaluate the cytotoxicity of alendronate (Ald), a bisphosphonate, and its effects on HRF wound healing. Methods HRFs were obtained from human supraspinatus tendons, using primary cell cultures. The experimental groups were control, 0.1 mu M Ald, 1 mu M Ald, 10 mu M Ald, and 100 mu M Ald. Alendronate exposure was for 48 h, except during a cell viability analysis with durations from 1 day to 6 days. The experimental groups were evaluated for cell viability, cell cycle and cell proliferation, type of cell death, caspase activity, and wound-healing ability. Results The following findings regarding the 100 mu M Ald group contrasted with those for all the other experimental groups: a significantly lower rate of live cells (p < 0.01), a higher rate of subG1 population, a lower rate of Ki-67 positive cells, higher rates of apoptosis and necrosis, a higher number of cells with DNA fragmentation, higher caspase-3/7 activity (p < 0.001), and a higher number of caspase-3 positive staining cells. In scratch-wound healing analyses of all the experimental groups, all the wounds healed within 48 h, except in the 100 mu M Ald group (p < 0.001). Conclusions Low concentrations of alendronate appear to have little effect on HRF viability, proliferation, migration, and wound healing. However, high concentrations are significantly cytotoxic, impairing cellular proliferation, cellular migration, and wound healing in vitro.
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