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肿瘤坏死因子抗体对注射内毒素的马前臂腕关节滑液细胞因子活性的影响。

Effect of tumor necrosis factor antibody on synovial fluid cytokine activities in equine antebrachiocarpal joints injected with endotoxin.

作者信息

Hawkins D L, Cargile J L, MacKay R J, Broome T A, Skelley L A

机构信息

Department of Large Animal Clinical Sciences, College of Veterinary Medicine, University of Florida, Gainesville 32610, USA.

出版信息

Am J Vet Res. 1995 Oct;56(10):1292-9.

PMID:8928945
Abstract

Six horses received intra-articular injections of a mixture of 1 micrograms of endotoxin/5 mg of equine tumor necrosis factor (eqTNF) monoclonal antibody in 1 antebrachiocarpal joint and an equal volume (2 ml) of 1 micrograms of endotoxin/5 mg of control antibody in the opposite joint. Synovial fluid sample collection (1 ml) was accomplished by use of an indwelling, intra-articular catheter at postinjection hours (PIH) 0, 1, 1.5, 2, 5, and 8, and by arthrocentesis at PIH 24. Joint fluid samples were analyzed for nucleated cell count, protein concentration, and TNF, interleukin 6 (IL-6), IL-1, and IL-1-inhibitory activities. To monitor local inflammation, each carpus was graded semiquantitatively for swelling prior to each sample collection. Tumor necrosis factor, IL-1, or IL-1-inhibitory activity was not detected in any synovial fluid sample collected before endotoxin/antibody was administered. However, low IL-6 activity (< 100 U/ml) was found in 2 of 12 preinjection samples. In joints injected with endotoxin/control antibody mixture, maximal mean +/- SEM activities for TNF (1,019 +/- 310 U/ml), IL-1 (173 +/- 102 U/ml), and IL-6 (10.8 +/- 3.1 x 10(4) U/ml) were observed at PIH 2, 5, and 8, respectively. Tumor necrosis factor and IL-1 activities returned to baseline values by PIH 8 and 24, respectively; however, IL-6 activity remained high. Interleukin 1 inhibitory activity (27.4 +/- 2.25 IU/ml) was detected in all PIH-24 samples from control joints, but was not detected at any other time in control joints (limit of detection, 20 IU/ml). Tumor necrosis factor activity was not detected in any synovial fluid sample from joints treated with endotoxin/eqTNF antibody. In contrast, endotoxin IL-1 inhibitory activity (PIH 24) was higher in eqTNF antibody-treated joints (41.0 +/- 7.7 IU/ml) than in control joints, but the difference was not significant. Mean WBC count and protein concentration in control and treated joints were maximal at PIH 8. The curves for mean values of WBC count and total protein concentration were not significantly different in treated versus control joints. Swelling in each treated joint was either less than or the same as that in the opposite control joint at even, time in the initial 8 PIH. There was significant (P = 0.043) difference between treated and control joints at PIH 5 and 8. These results describe a profile of synovial fluid TNF, IL-1, IL-6 bioactivities, and IL-1-inhibitory activity during the initial 24 hours of synovitis induced by intra-articular administration of endotoxin in horses. Our eqTNF monoclonal antibody was effective in neutralizing TNF activity in synovial fluid when administered intra-articularly with endotoxin in horses. The induction of IL-1, IL-1 inhibitory activity IL-6, WBC, and total protein concentration responses are largely independent of TNF activity in synovial fluid of horses receiving endotoxin intra-articularly.

摘要

6匹马的1个腕掌关节内注射1微克内毒素/5毫克马肿瘤坏死因子(eqTNF)单克隆抗体的混合物,对侧关节注射等体积(2毫升)的1微克内毒素/5毫克对照抗体。在注射后0、1、1.5、2、5和8小时,通过留置关节内导管采集滑膜液样本(1毫升),并在注射后24小时通过关节穿刺术采集。对关节液样本进行有核细胞计数、蛋白质浓度以及肿瘤坏死因子、白细胞介素6(IL-6)、白细胞介素1(IL-1)和IL-1抑制活性的分析。为监测局部炎症,在每次采集样本前对每个腕关节的肿胀程度进行半定量分级。在内毒素/抗体给药前采集的任何滑膜液样本中均未检测到肿瘤坏死因子、IL-1或IL-1抑制活性。然而,在12份注射前样本中的2份中发现低水平的IL-6活性(<100 U/ml)。在注射内毒素/对照抗体混合物的关节中,肿瘤坏死因子(1,019±310 U/ml)、IL-1(173±102 U/ml)和IL-6(10.8±3.1×10⁴ U/ml)的最大平均±标准误活性分别在注射后2、5和8小时观察到。肿瘤坏死因子和IL-1活性分别在注射后8小时和24小时恢复到基线值;然而,IL-6活性仍保持较高水平。在对照关节的所有注射后24小时样本中均检测到IL-1抑制活性(27.4±2.25 IU/ml),但在对照关节的其他任何时间均未检测到(检测限为20 IU/ml)。在用内毒素/eqTNF抗体处理的关节的任何滑膜液样本中均未检测到肿瘤坏死因子活性。相比之下,eqTNF抗体处理的关节中内毒素IL-1抑制活性(注射后24小时)(41.0±7.7 IU/ml)高于对照关节,但差异不显著。对照关节和处理关节中的平均白细胞计数和蛋白质浓度在注射后8小时达到最大值。处理关节与对照关节中白细胞计数和总蛋白质浓度平均值的曲线无显著差异。在最初注射后8小时的各个时间点,每个处理关节的肿胀程度均小于或等于对侧对照关节。在注射后5小时和8小时,处理关节与对照关节之间存在显著差异(P = 0.043)。这些结果描述了马关节内注射内毒素诱导滑膜炎最初24小时内滑膜液中肿瘤坏死因子、IL-1、IL-6生物活性以及IL-1抑制活性的情况。当与内毒素一起关节内给药时,我们的eqTNF单克隆抗体可有效中和马滑膜液中的肿瘤坏死因子活性。在关节内接受内毒素的马的滑膜液中,IL-1、IL-1抑制活性、IL-6、白细胞和总蛋白质浓度反应的诱导在很大程度上与肿瘤坏死因子活性无关。

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