抗炎治疗对人髓核细胞的炎症动力学及疗效
Inflammatory Kinetics and Efficacy of Anti-inflammatory Treatments on Human Nucleus Pulposus Cells.
作者信息
Walter Benjamin A, Purmessur Devina, Likhitpanichkul Morakot, Weinberg Alan, Cho Samuel K, Qureshi Sheeraz A, Hecht Andrew C, Iatridis James C
机构信息
*Leni and Peter W. May Department of Orthopaedics at the Icahn School of Medicine at Mount Sinai, New York, NY †Department of Biomedical Engineering, The City College of New York, New York, NY; and ‡Department of Population Health Science and Policy, Icahn School of Medicine at Mount Sinai, New York, NY.
出版信息
Spine (Phila Pa 1976). 2015 Jul 1;40(13):955-63. doi: 10.1097/BRS.0000000000000932.
STUDY DESIGN
Human nucleus pulposus (NP) cell culture study investigating response to tumor necrosis factor-α (TNFα), effectiveness of clinically available anti-inflammatory drugs, and interactions between proinflammatory cytokines.
OBJECTIVE
To characterize the kinetic response of proinflammatory cytokines released by human NP cells to TNFα stimulation and the effectiveness of multiple anti-inflammatories with 3 substudies: Timecourse, Same-time blocking, Delayed blocking.
SUMMARY OF BACKGROUND DATA
Chronic inflammation is a key component of painful intervertebral disc degeneration. Improved efficacy of anti-inflammatories requires better understanding of how quickly NP cells produce proinflammatory cytokines and which proinflammatory mediators are most therapeutically advantageous to target.
METHODS
Degenerated human NP cells (n = 10) were cultured in alginate with or without TNFα (10 ng/mL). Cells were incubated with 1 of 4 anti-inflammatories (anti-IL-6 receptor/atlizumab, IL-1 receptor anatagonist, anti-TNFα/infliximab and sodium pentosan polysulfate/PPS) in 2 blocking-studies designed to determine how intervention timing influences drug efficacy. Cell viability, protein, and gene expression for IL-1β, IL-6, and IL-8 were assessed.
RESULTS
Timecourse: TNFα substantially increased the amount of IL-6, IL-8, and IL-1β, with IL-1β and IL-8 reaching equilibrium within ∼72 hours (IL-1β: 111 ± 40 pg/mL, IL-8: 8478 ± 957 pg/mL), and IL-6 not reaching steady state after 144 hours (1570 ± 435 pg/mL). Anti-TNFα treatment was most effective at reducing the expression of all cytokines measured when added at the same time as TNFα stimulation. Similar trends were observed when drugs were added 72 hours after TNFα stimulation, however, no anti-inflammatories significantly reduced cytokine levels compared with TNF control.
CONCLUSION
IL-1β, IL-6, and IL-8 were expressed at different rates and magnitudes suggesting different roles for these cytokines in disease. Autocrine signaling of IL-6 or IL-1β did not contribute to the expression of any proinflammatory cytokines measured in this study. Anti-inflammatory treatments were most effective when applied early in the inflammatory process, when targeting the source of the inflammation.
LEVEL OF EVIDENCE
N/A.
研究设计
人髓核(NP)细胞培养研究,旨在探究对肿瘤坏死因子-α(TNFα)的反应、临床可用抗炎药物的有效性以及促炎细胞因子之间的相互作用。
目的
通过三项子研究(时间进程、同时阻断、延迟阻断)来描述人NP细胞释放的促炎细胞因子对TNFα刺激的动力学反应以及多种抗炎药物的有效性。
背景数据总结
慢性炎症是疼痛性椎间盘退变的关键组成部分。提高抗炎药物的疗效需要更好地了解NP细胞产生促炎细胞因子的速度以及哪些促炎介质是最具治疗优势的靶点。
方法
将退变的人NP细胞(n = 10)在有或无TNFα(10 ng/mL)的情况下于藻酸盐中培养。在两项旨在确定干预时机如何影响药物疗效的阻断研究中,将细胞与4种抗炎药物之一(抗IL-6受体/阿特珠单抗、IL-1受体拮抗剂、抗TNFα/英夫利昔单抗和戊聚糖多硫酸钠/PPS)孵育。评估细胞活力、蛋白质以及IL-1β、IL-6和IL-8的基因表达。
结果
时间进程:TNFα显著增加了IL-6、IL-8和IL-1β的量,IL-1β和IL-8在约72小时内达到平衡(IL-1β:111±40 pg/mL,IL-8:8478±957 pg/mL),而IL-6在144小时后未达到稳态(1570±435 pg/mL)。抗TNFα治疗在与TNFα刺激同时添加时,对降低所有检测细胞因子的表达最有效。当在TNFα刺激72小时后添加药物时也观察到类似趋势,然而,与TNF对照组相比,没有抗炎药物能显著降低细胞因子水平。
结论
IL-1β、IL-6和IL-8以不同的速率和幅度表达,表明这些细胞因子在疾病中具有不同作用。IL-6或IL-1β的自分泌信号传导对本研究中检测的任何促炎细胞因子的表达均无贡献。抗炎治疗在炎症过程早期针对炎症源时最有效。
证据水平
无。
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