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羟基磷灰石颗粒碎片对人成纤维细胞中细胞因子和蛋白酶产生的影响。

Effects of hydroxyapatite particulate debris on the production of cytokines and proteases in human fibroblasts.

作者信息

Ninomiya J T, Struve J A, Stelloh C T, Toth J M, Crosby K E

机构信息

Department of Orthopaedic Surgery, Medical College of Wisconsin, Milwaukee, USA.

出版信息

J Orthop Res. 2001 Jul;19(4):621-8. doi: 10.1016/S0736-0266(00)00061-9.

DOI:10.1016/S0736-0266(00)00061-9
PMID:11518271
Abstract

Cytokines and proteases are secreted by fibroblasts in response to particulate wear debris, and these proteins are felt to play an important role in the development of osteolysis and implant loosening. Although metallic and polyethlyene debris have been studied extensively, little is known about the cellular responses to hydroxyapatite, despite the wide clinical use of these materials. Therefore, the effects of hydroxyapatite (HA) and hydroxyapatite/beta-tricalciumphosphate (HA/TCP) on cellular proliferation, cytokine gene expression and protein secretion, protease synthesis, and gelatinolytic activity were investigated in human fibroblasts. HA and HA/TCP particles were synthesized, and their effects were compared to the responses elicited by titanium and cobalt chromium. Sample characterization by scanning electron microscopy and Coulter Counter demonstrated that the materials had a mean particle size of less than 10 microm, and all of the particles were compared using the same concentration ranges. Aliquots of particle suspensions were added to human fibroblasts maintained in tissue culture, and dose-response and time-course experiments were performed. Effects of the particles on fibroblast proliferation were assessed, and alterations in cytokine levels were determined by specific enzyme linked immunosorbent assays (ELISA). Cytokines that were evaluated included interleukin-1 (IL-1beta), interleukin-6 (IL-6), and tumor necrosis factor-alpha (TNF-alpha), all of which have been demonstrated to enhance bone resorption and are associated with osteolysis and implant loosening. Gene expression was determined using Northern blot analysis with cytokine-specific probes, while secretion of the proteases collagenase and stromelysin was determined by Western blot analysis. Functional gelatinolytic assay was assessed using zymogram gels. The particles were evaluated in a concentration range from 0.000021 to 0.021 vol%. All of the particles produced increases in cellular proliferation up to 0.0021 vol%, with the largest increases being seen at 0.021 vol% with HA/TCP and titanium. At the highest concentration, both cobalt chromium and HA samples decreased cellular proliferation relative to lower doses, possibly representing cytotoxicity. Hydroxyapatite particles yielded a 30-fold increase in interleukin-6 secretion compared to unstimulated controls, which was also greater than three times the levels produced by cobalt chromium, titanium, or HA/TCP. HA particles also tripled the secretion of IL-1beta at 0.00021 vol%, and doubled TNF-alpha secretion at 0.021 vol%. Addition of conditioned media prepared by incubation of the particles in culture medium in the absence of cells did not alter the secretion of any of the cytokines. Northern blot analysis using IL-6 probes also demonstrated strong increases with HA compared to the other materials, suggesting that the action of the HA particles was at the level of transcription. Secretion of the protease collagenase was increased by all of the samples including HA when compared to unstimulated controls. Stromelysin secretion into the culture medium was decreased by cobalt chromium, but increased by titanium, HA, and HA/TCP. All of the particles including HA increased the gelatinolytic activity of the fibroblasts. These findings demonstrate that HA and HA/TCP particles are capable of stimulating the expression and secretion of cytokines and proteases that enhance bone resorption, and suggest that particulate debris from implants using these coatings may also increase osteolysis and loosening.

摘要

成纤维细胞会响应颗粒磨损碎片而分泌细胞因子和蛋白酶,这些蛋白质被认为在骨溶解和植入物松动的发展中起重要作用。尽管对金属和聚乙烯碎片已进行了广泛研究,但尽管这些材料在临床上广泛使用,关于细胞对羟基磷灰石的反应却知之甚少。因此,研究了羟基磷灰石(HA)和羟基磷灰石/β-磷酸三钙(HA/TCP)对人成纤维细胞的细胞增殖、细胞因子基因表达和蛋白质分泌、蛋白酶合成以及明胶酶活性的影响。合成了HA和HA/TCP颗粒,并将它们的作用与钛和钴铬引发的反应进行比较。通过扫描电子显微镜和库尔特计数器对样品进行表征,结果表明这些材料的平均粒径小于10微米,并且所有颗粒都在相同的浓度范围内进行比较。将等分的颗粒悬浮液添加到组织培养中的人成纤维细胞中,并进行剂量反应和时间进程实验。评估颗粒对成纤维细胞增殖的影响,并通过特异性酶联免疫吸附测定(ELISA)确定细胞因子水平的变化。评估的细胞因子包括白细胞介素-1(IL-1β)、白细胞介素-6(IL-6)和肿瘤坏死因子-α(TNF-α),所有这些都已被证明可增强骨吸收并与骨溶解和植入物松动相关。使用细胞因子特异性探针通过Northern印迹分析确定基因表达,而通过Western印迹分析确定蛋白酶胶原酶和基质金属蛋白酶的分泌。使用酶谱凝胶评估功能性明胶酶活性。在0.000021至0.021体积%的浓度范围内评估颗粒。所有颗粒在浓度达到0.0021体积%时都会使细胞增殖增加,在HA/TCP和钛的0.021体积%时增加最大。在最高浓度下,钴铬和HA样品相对于较低剂量会降低细胞增殖,这可能代表细胞毒性。与未刺激的对照相比,羟基磷灰石颗粒使白细胞介素-6的分泌增加了30倍,这也比钴铬、钛或HA/TCP产生的水平高三倍以上。HA颗粒在0.00021体积%时也使IL-1β的分泌增加了两倍,在0.021体积%时使TNF-α的分泌增加了一倍。添加通过在无细胞的培养基中孵育颗粒制备的条件培养基不会改变任何细胞因子的分泌。使用IL-6探针的Northern印迹分析也表明,与其他材料相比,HA的增加很强,这表明HA颗粒的作用是在转录水平。与未刺激的对照相比,包括HA在内的所有样品都增加了蛋白酶胶原酶的分泌。钴铬会减少基质金属蛋白酶分泌到培养基中,但钛、HA和HA/TCP会增加。包括HA在内的所有颗粒都增加了成纤维细胞的明胶酶活性。这些发现表明,HA和HA/TCP颗粒能够刺激增强骨吸收的细胞因子和蛋白酶的表达和分泌,并表明使用这些涂层的植入物的颗粒碎片也可能增加骨溶解和松动。

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