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High elastic modulus nanoparticles: a novel tool for subfailure connective tissue matrix damage.
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Comparative effectiveness of injection therapies in lateral epicondylitis: a systematic review and network meta-analysis of randomized controlled trials.注射治疗外侧肱骨上髁炎的疗效比较:随机对照试验的系统评价和网络荟萃分析。
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Tendon healing: repair and regeneration.肌腱愈合:修复与再生。
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Rheumatology (Oxford). 2012 Jul;51(7):1161-5. doi: 10.1093/rheumatology/kes002. Epub 2012 Feb 15.
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Effect of prolotherapy on cellular proliferation and collagen deposition in MC3T3-E1 and patellar tendon fibroblast populations.富血小板血浆疗法对 MC3T3-E1 细胞和髌腱成纤维细胞群体的细胞增殖和胶原沉积的影响。
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注射疗法在体外诱导人肌腱细胞产生炎症反应。

Prolotherapy Induces an Inflammatory Response in Human Tenocytes In Vitro.

作者信息

Ekwueme Emmanuel C, Mohiuddin Mahir, Yarborough Jazmin A, Brolinson P Gunnar, Docheva Denitsa, Fernandes Hugo A M, Freeman Joseph W

机构信息

Department of Biomedical Engineering, Rutgers University, 599 Taylor Road, Piscataway, NJ, 08854, USA.

Edward Via Virginia College of Osteopathic Medicine, Blacksburg, VA, USA.

出版信息

Clin Orthop Relat Res. 2017 Aug;475(8):2117-2127. doi: 10.1007/s11999-017-5370-1. Epub 2017 Apr 27.

DOI:10.1007/s11999-017-5370-1
PMID:28451864
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5498388/
Abstract

BACKGROUND

Proliferative therapy, or prolotherapy, is a controversial treatment method for many connective tissue injuries and disorders. It involves the injection of a proliferant, or irritant solution, into the site of injury, which causes small-scale cell death. This therapeutic trauma is theorized to initiate the body's wound-healing cascade, perhaps leading to tissue repair. The immediate effects of many of these proliferants are poorly characterized, as are the cellular responses to them; here, we sought to evaluate the immediate effects of two common proliferants (dextrose and P2G, a combination of phenol, glucose, and glycerin) on the cellular response of human tenocytes, and begin to explicate the mechanisms with which each proliferant functions.

QUESTIONS/PURPOSES: We asked: What are the effects of treating cultured tenocytes with proliferative treatment agents on their (1) cellular metabolic activity, (2) RNA expression, (3) protein secretion, and (4) cell migration?

METHODS

Using human hamstring and Achilles tendon cells, we attempted to answer our research questions. We used a colorimetric metabolic assay to assess the effect of dextrose and P2G proliferant treatment on cell mitochondrial activity compared with nontreated tenocytes. Next, using quantitative PCR, ELISA, and a reporter cell line, we assessed the expression of several key markers involved in tendon development and inflammation. In addition, we used a scratch wound-healing assay to evaluate the effect of proliferant treatment on tenocyte migration.

RESULTS

Results showed that exposure to both solutions led to decreased metabolic activity of tenocytes, with P2G having the more pronounced effect (75% ± 7% versus 95% ± 7% of untreated control cell metabolic levels) (ANOVA; p < 0.01; mean difference, 0.202; 95% CI, 0.052-0.35). Next, gene expression analysis confirmed that treatment led to the upregulation of key proinflammatory markers including interleukin-8 and cyclooxygenase-2 and downregulation of the matrix marker collagen type I. Furthermore, using a reporter cell line for transforming growth factor-β (TGF-β), a prominent antiinflammatory marker, we showed that treatments led to decreased TGF-β bioactivity. Analysis of soluble proteins using ELISA revealed elevated levels of soluble prostaglandin E2 (PGE2), a prominent inducer of inflammation. Finally, both solutions led to decreased cellular migration in the tenocytes.

CONCLUSIONS

Taken together, these results suggest that prolotherapy, more so with P2G, may work by decreasing cellular function and eliciting an inflammatory response in tenocytes. Additional studies are needed to confirm the cellular signaling mechanisms involved and the resulting immediate response in vivo.

CLINICAL RELEVANCE

If these preliminary in vitro findings can be confirmed in an in vivo model, they may provide clues for a possible cellular mechanism of a common alternative treatment method currently used for certain soft tissue injuries.

摘要

背景

增殖疗法,即注射增殖剂疗法,是一种针对多种结缔组织损伤和病症的具有争议性的治疗方法。它涉及将一种增殖剂或刺激性溶液注射到损伤部位,这会导致小规模的细胞死亡。从理论上讲,这种治疗性创伤会启动人体的伤口愈合级联反应,可能会导致组织修复。许多此类增殖剂的即时效应以及细胞对它们的反应都尚未得到充分描述;在此,我们试图评估两种常见增殖剂(葡萄糖和P2G,一种苯酚、葡萄糖和甘油的混合物)对人肌腱细胞的细胞反应的即时效应,并开始阐明每种增殖剂发挥作用的机制。

问题/目的:我们提出以下问题:用增殖治疗剂处理培养的肌腱细胞对其(1)细胞代谢活性、(2)RNA表达、(3)蛋白质分泌和(4)细胞迁移有何影响?

方法

我们使用人绳肌和跟腱细胞来尝试回答我们的研究问题。我们使用比色代谢测定法来评估葡萄糖和P2G增殖剂处理与未处理的肌腱细胞相比对细胞线粒体活性的影响。接下来,我们使用定量PCR、酶联免疫吸附测定(ELISA)和一个报告细胞系来评估参与肌腱发育和炎症的几种关键标志物的表达。此外,我们使用划痕伤口愈合测定法来评估增殖剂处理对肌腱细胞迁移的影响。

结果

结果表明,两种溶液处理均导致肌腱细胞的代谢活性降低,其中P2G的影响更为显著(分别为未处理对照细胞代谢水平的75%±7%和95%±7%)(方差分析;p<0.01;平均差异为0.202;95%置信区间为0.052 - 0.35)。接下来,基因表达分析证实,处理导致关键促炎标志物上调,包括白细胞介素 - 8和环氧化酶 - 2,同时基质标志物I型胶原蛋白下调。此外,使用转化生长因子 - β(TGF - β,一种突出的抗炎标志物)的报告细胞系,我们发现处理导致TGF - β生物活性降低。使用ELISA对可溶性蛋白质进行分析显示,可溶性前列腺素E2(PGE2,一种突出的炎症诱导剂)水平升高。最后,两种溶液均导致肌腱细胞的细胞迁移减少。

结论

综上所述,这些结果表明,注射增殖剂疗法,尤其是P2G,可能是通过降低细胞功能并引发肌腱细胞的炎症反应来发挥作用的。需要进一步的研究来确认其中涉及的细胞信号传导机制以及在体内产生的即时反应。

临床意义

如果这些初步的体外研究结果能够在体内模型中得到证实,它们可能为目前用于某些软组织损伤的一种常见替代治疗方法的可能细胞机制提供线索。