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小鼠的急性炎症反应:脂皮质素1免疫中和作用导致炎症加剧。

Acute inflammatory response in the mouse: exacerbation by immunoneutralization of lipocortin 1.

作者信息

Perretti M, Ahluwalia A, Harris J G, Harris H J, Wheller S K, Flower R J

机构信息

Department of Biochemical Pharmacology, Medical College of St. Bartholomew's Hospital, London.

出版信息

Br J Pharmacol. 1996 Mar;117(6):1145-54. doi: 10.1111/j.1476-5381.1996.tb16709.x.

DOI:10.1111/j.1476-5381.1996.tb16709.x
PMID:8882609
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1909779/
Abstract
  1. An immuno-neutralization strategy was employed to investigate the role of endogenous lipocortin 1 (LC1) in acute inflammation in the mouse. 2. Mice were treated subcutaneously with phosphate-buffered solution (PBS), non-immune sheep serum (NSS) or with one of two sheep antisera raised against LC1 (LCS3), or its N-terminal peptide (LCPS1), three times over a period of seven days. Twenty four hours after the last injection several parameters of acute inflammation were measured including zymosan-induced inflammation in 6-day-old air-pouches, zymosan-activated serum (ZAS)-induced oedema in the skin, platelet-activating factor (PAF)-induced neutrophilia and interleukin-1 beta (IL-1 beta)-induced corticosterone (CCS) release. 3. At the 4 h time-point of the zymosan inflamed air-pouch model, treatment with LCS3 did not modify the number of polymorphonuclear leucocytes (PMN) recruited: 7.84 +/- 1.01 and 7.00 +/- 0.77 x 10(6) PMN per mouse for NSS- and LCS3 group, n = 7. However, several other parameters of cell activation including myeloperoxidase (MPO) and elastase activities were increased (2.2 fold, P < 0.05, and 6.5 fold, P < 0.05, respectively) in the lavage fluids of these mice. Similarly, a significant increase in the amount of immunoreactive prostaglandin E2 (PGE2; 1.81 fold, P < 0.05) and IL-1 alpha (2.75 fold, P < 0.05), but not tumour necrosis factor-alpha (TNF-alpha), was also observed in LCS3-treated mice. 4. The recruitment of PMN into the zymosan inflamed air-pouches by 24 h had declined substantially (4.13 +/- 0.61 x 10(6) PMN per mouse, n = 12) in the NSS-treated mice, whereas high values were still measured in those treated with LCS3 (9.35 +/- 1.20 x 10(6) PMN per mouse, n = 12, P < 0.05). A similar effect was also found following sub-chronic treatment of mice with LCPS1: 6.48 +/- 0.10 x 10(6) PMN per mouse, vs. 2.77 +/- 1.20 and 2.64 +/- 0.49 x 10(6) PMN per mouse for PBS- and NSS-treated groups (n = 7, P < 0.05). Most markers of inflammation were also increased in the lavage fluids of LCS3-treated mice: MPO and elastase showed a 2.47 fold and 17 fold increase, respectively (P < 0.05 in both cases); TNF-alpha showed a 11.1 fold increase (P < 0.05) whereas the IL-1 alpha levels were not significantly modified. PGE2 was still detectable in most (5 out of 7) of the mice treated with LCS3 but only in 2 out of 7 of the NSS-treated mice. 5. Intradermal injection of 50% ZAS caused a significant increase in the 2 hoedema formation in the skin of LCS3-treated mice in comparison to PBS- and NSS-treated animals: 16.7 +/- 1.5 microliters vs. 10.8 +/- 1.2 microliters and 10.2 +/- 1.0 microliters, respectively (n = 14 mice per group, P < 0.05). ZAS-induced oedema had subsided by 24 h in control animals but a residual significant amount of extravasation was still detectable in LCS3-treated mice: 4.4 +/- 0.8 microliters (P < 0.05). 6. A recently described model driven by endogenous glucocorticoids is the blood neutrophilia observed following administration of PAF. In our experimental conditions, a single bolus of PAF (100 ng, i.v.) provoked a marked neutrophilia at 2 h (2.43 and 2.01 fold) in NSS- and PBS-treated mice (n = 11), respectively, which was significantly attenuated in the animals treated with LCS3: 1.26 fold increase in circulating PMN (n = 11, P < 0.01 vs. NSS- and PBS-groups). 7. Intraperitoneal injection of IL-1 beta (5 micrograms kg-1) caused a marked increase in circulating plasma CCS by 2 h, to a similar extent in all experimental groups. In contrast, measurement of CCS levels in the plasma of mice bearing air-pouches inflamed with zymosan revealed significant differences between LCS3 and NSS-treated mice at the 4 h time-point: 198 +/- 26 ng ml-1 vs. 110 +/- 31 ng ml-1 (n = 8, P < 0.05). 8. In conclusion, we found a remarkable exacerbation of the inflammatory process with respect to both humoral and cellular components in mice passively immunised agains
摘要
  1. 采用免疫中和策略研究内源性脂皮质素1(LC1)在小鼠急性炎症中的作用。2. 小鼠在7天内皮下注射3次磷酸盐缓冲溶液(PBS)、非免疫羊血清(NSS)或两种抗LC1的羊抗血清之一(LCS3),或其N端肽(LCPS1)。末次注射24小时后,测量急性炎症的几个参数,包括6日龄气袋中酵母聚糖诱导的炎症、酵母聚糖激活血清(ZAS)诱导的皮肤水肿、血小板活化因子(PAF)诱导的中性粒细胞增多以及白细胞介素-1β(IL-1β)诱导的皮质酮(CCS)释放。3. 在酵母聚糖诱发炎症的气袋模型的4小时时间点,LCS3处理并未改变募集的多形核白细胞(PMN)数量:NSS组和LCS3组每只小鼠分别为7.84±1.01和7.00±0.77×10⁶个PMN,n = 7。然而,这些小鼠灌洗液中其他几个细胞活化参数,包括髓过氧化物酶(MPO)和弹性蛋白酶活性增加(分别为2.2倍,P < 0.05,和6.5倍,P < 0.05)。同样,在LCS3处理的小鼠中也观察到免疫反应性前列腺素E2(PGE2;1.81倍,P < 0.05)和IL-1α(2.75倍,P < 0.05)的量显著增加,但肿瘤坏死因子-α(TNF-α)未增加。4. 24小时时,NSS处理的小鼠中PMN向酵母聚糖诱发炎症的气袋中的募集显著下降(每只小鼠4.13±0.61×10⁶个PMN,n = 12),而LCS3处理的小鼠中仍测量到高值(每只小鼠9.35±1.20×10⁶个PMN,n = 12,P < 0.05)。用LCPS1对小鼠进行亚慢性处理后也发现了类似的效果:每只小鼠6.48±0.10×10⁶个PMN,而PBS和NSS处理组每只小鼠分别为2.77±1.20和2.64±0.49×10⁶个PMN(n = 7,P < 0.05)。LCS3处理的小鼠灌洗液中大多数炎症标志物也增加:MPO和弹性蛋白酶分别增加2.47倍和17倍(两者均P < 0.05);TNF-α增加11.1倍(P < 0.05),而IL-1α水平无显著改变。PGE2在大多数(7只中的5只)LCS3处理的小鼠中仍可检测到,但在7只NSS处理的小鼠中只有2只可检测到。5. 与PBS和NSS处理的动物相比,皮内注射50% ZAS导致LCS3处理的小鼠皮肤在2小时时水肿形成显著增加:分别为16.7±1.5微升,而PBS和NSS处理组分别为10.8±1.2微升和10.2±1.0微升(每组14只小鼠,P < 0.05)。ZAS诱导的水肿在对照动物中24小时时消退,但在LCS3处理的小鼠中仍可检测到残留的显著渗出量:4.4±0.8微升(P < 0.05)。6. 最近描述的由内源性糖皮质激素驱动的模型是PAF给药后观察到的血液中性粒细胞增多。在我们的实验条件下,单次推注PAF(100 ng,静脉注射)在2小时时在NSS和PBS处理的小鼠(n = 11)中分别引起显著的中性粒细胞增多(2.43倍和2.01倍),在用LCS3处理的动物中显著减弱:循环PMN增加1.26倍(n = 11,与NSS和PBS组相比P < 0.01)。7. 腹腔注射IL-1β(5微克/千克)在2小时时导致循环血浆CCS显著增加,在所有实验组中程度相似。相反,测量酵母聚糖诱发炎症的气袋小鼠血浆中CCS水平发现,在4小时时间点LCS3和NSS处理的小鼠之间存在显著差异:198±26纳克/毫升对110±31纳克/毫升(n = 8,P < 0.05)。8. 总之,我们发现被动免疫的小鼠在体液和细胞成分方面炎症过程均有显著加剧。

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