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不同富血小板血浆方法对人体肌肉、骨骼和肌腱细胞的积极影响。

The positive effects of different platelet-rich plasma methods on human muscle, bone, and tendon cells.

机构信息

University of Connecticut, Department of Orthopaedic Surgery, 263 Farmington Ave, MARB 4th Floor, Farmington, CT 06034, USA.

出版信息

Am J Sports Med. 2012 Aug;40(8):1742-9. doi: 10.1177/0363546512452713. Epub 2012 Jul 16.

Abstract

BACKGROUND

Clinical application of platelet-rich plasma (PRP) in the realm of orthopaedic sports medicine has yielded variable results. Differences in separation methods and variability of the individual may contribute to these variable results.

PURPOSE

To compare the effects of different PRP separation methods on human bone, muscle, and tendon cells in an in vitro model.

STUDY DESIGN

Controlled laboratory study.

METHODS

Blood collected from 8 participants (mean ± SD age 31.6 ± 10.9 years) was used to obtain PRP preparations. Three different PRP separation methods were used: a single-spin process yielding a lower platelet concentration (PRP(LP)), a single-spin process yielding high platelet and white blood cell concentrations (PRP(HP)), and a double-spin that produces a higher platelet concentration and lower white blood cell concentration (PRP(DS)). Human bone, muscle, and tendon cells obtained from discarded tissue samples during shoulder surgery were placed into culture and treated with the 3 PRP preparations, control media (2% fetal bovine serum [FBS] and 10% FBS), and native blood. Radioactive thymidine assays were obtained to examine cell proliferation, and testing with enzyme-linked immunosorbent assay was used to determine growth factor concentrations.

RESULTS

Addition of PRP(LP) to osteocytes, myocytes, and tenocytes significantly increased cell proliferation (P ≤ .05) compared with the controls. Adding PRP(DS) to osteoblasts and tenocytes increased cell proliferation significantly (P ≤ .05), but no significance was shown for its addition to myocytes. The addition of PRP(HP) significantly increased cell proliferation compared with the controls only when added to tenocytes (P ≤ .05). Osteoblasts: Proliferation was significantly increased by addition of PRP(LP) compared with all controls (2% FBS, 10% FBS, native blood) (P ≤ .05). Addition of PRP(DS) led to significantly increased proliferation compared with all controls, native blood, and PRP(HP) (P ≤ .05). Proliferation was significantly less when PRP(HP) was added compared with PRP(DS) (P ≤ .05). Myocytes: Proliferation was significantly increased by addition of PRP(LP) compared with native blood (P ≤ .05). Adding PRP(HP) or PRP(DS) to myocytes showed no significant increase in proliferation compared with the controls or the other separations. Tenocytes: Proliferation was significantly increased by addition of PRP(LP) compared with all controls (2% FBS, 10% FBS, native blood) (P ≤ .05). Addition of PRP(DS) showed a significant increase compared with the controls and native blood. For tenocytes, there was a significant increase (P ≤ .05) seen when PRP(HP) was added compared with the controls and native blood but not compared with the other separations.

CONCLUSION

The primary findings of this study suggest the application of different PRP separations may result in a potential beneficial effect on the clinically relevant target cells in vitro. However, it is unclear which platelet concentration or PRP preparation may be optimal for the treatment of various cell types. In addition, a "more is better" theory for the use of higher platelet concentrations cannot be supported. This study was not intended to prove efficacy but to provide a platform for future research to be built upon.

CLINICAL RELEVANCE

The utilization of different PRP separations may result in a potentially beneficial effect on the clinically relevant target cells in vitro, but it is unclear which platelet concentration or PRP preparation may be optimal for the treatment of various cell types.

摘要

背景

富血小板血浆(PRP)在运动医学领域的临床应用效果不一。不同的分离方法和个体差异可能是导致这些结果差异的原因。

目的

比较不同 PRP 分离方法对体外人骨、肌肉和肌腱细胞的影响。

研究设计

对照实验室研究。

方法

从 8 名参与者(平均年龄 31.6±10.9 岁)采集血液,用于获得 PRP 制剂。使用三种不同的 PRP 分离方法:一种产生较低血小板浓度的单旋过程(PRP(LP))、一种产生高血小板和白细胞浓度的单旋过程(PRP(HP))和一种产生更高血小板浓度和更低白细胞浓度的双旋过程(PRP(DS))。从肩关节手术中废弃的组织样本中获得人骨、肌肉和肌腱细胞,放入培养物中,并分别用 3 种 PRP 制剂、对照培养基(2%胎牛血清[FBS]和 10% FBS)和天然血液进行处理。通过放射性胸腺嘧啶测定法检测细胞增殖,酶联免疫吸附测定法检测生长因子浓度。

结果

与对照组相比,添加 PRP(LP)到成骨细胞、肌细胞和肌腱细胞中可显著增加细胞增殖(P≤.05)。向成骨细胞和肌腱细胞中添加 PRP(DS)可显著增加细胞增殖(P≤.05),但对肌细胞没有明显影响。与对照组相比,添加 PRP(HP)仅能显著增加肌腱细胞的细胞增殖(P≤.05)。成骨细胞:与所有对照组(2% FBS、10% FBS、天然血液)相比,添加 PRP(LP)可显著增加增殖(P≤.05)。与所有对照组、天然血液和 PRP(HP)相比,添加 PRP(DS)可导致显著增加的增殖(P≤.05)。与 PRP(DS)相比,添加 PRP(HP)时增殖明显减少(P≤.05)。肌细胞:与天然血液相比,添加 PRP(LP)可显著增加增殖(P≤.05)。向肌细胞中添加 PRP(HP)或 PRP(DS)与对照组或其他分离物相比,增殖没有显著增加。肌腱细胞:与所有对照组(2% FBS、10% FBS、天然血液)相比,添加 PRP(LP)可显著增加增殖(P≤.05)。与对照组和天然血液相比,添加 PRP(DS)可显著增加增殖。与对照组和天然血液相比,添加 PRP(HP)可显著增加增殖(P≤.05),但与其他分离物相比没有显著增加。

结论

本研究的主要发现表明,应用不同的 PRP 分离方法可能会对体外临床相关靶细胞产生潜在的有益影响。然而,目前尚不清楚哪种血小板浓度或 PRP 制剂可能是治疗各种细胞类型的最佳选择。此外,较高血小板浓度的“越多越好”理论不能得到支持。本研究并非旨在证明疗效,而是为未来的研究提供一个平台。

临床相关性

不同的 PRP 分离方法的应用可能会对体外临床相关靶细胞产生潜在的有益影响,但尚不清楚哪种血小板浓度或 PRP 制剂可能是治疗各种细胞类型的最佳选择。

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