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通过多孔盖试验测定标准和新型白三烯B4类似物对人中性粒细胞趋化性的影响。

Influence of standard and novel LTB4 analogs on human neutrophil chemotaxis measured by the multiwell cap assay.

作者信息

Psychoyos S, Uziel-Fusi S, Bhagwat S, Morrissey M M

机构信息

Research Department, Ciba-Geigy Corporation, Summit, NJ 07901.

出版信息

J Immunol Methods. 1989 Nov 30;124(2):189-96. doi: 10.1016/0022-1759(89)90352-9.

DOI:10.1016/0022-1759(89)90352-9
PMID:2557367
Abstract

Standard and novel LTB4 analogs were tested for neutrophil chemoattractant activity using the multiwell cap assay (Evans et al. (1986) Biosc. Rep. 6, 1041). The assay uses disposable equipment and measures chemotaxis by the number of cells able to migrate across the full thickness of cellulose nitrate filters. Under standard conditions (90 min incubation at 37 degrees C in buffer containing 2% bovine albumin), LTB4 and 6-cis-LTB1 had EC50 values of 3.5 and 15,000 nM, respectively. 20-hydroxy-LTB4 was equipotent with LTB4 and exhibited a similar biphasic chemotactic response, however, only one third of the number of cells migrated through the filter. 20-carboxy-LTB4 was inactive up to 1,000 nM. 5-desoxy-((6,7)-cis-cyclopropyl)-LTB2, (6,7)-benzo-LTB2 and 5-desoxy-(8,10)-LTB2 had EC50 values of 11,300, 50,000 and 84,000 nM, respectively. Checkerboard analysis indicated a chemokinetic component of 42% for LTB4 at a concentration causing peak chemotaxis. Reduction of albumin in the buffer to 0.5% increased the apparent potencies of LTB4 and 6-cis-LTB1 five-fold. Since LTB4 is a mediator of inflammation, various anti-inflammatory agents were tested at peak concentrations observed in vivo for in vitro inhibition of LTB4-stimulated chemotaxis in the presence of 0.5% albumin. Under the conditions of the assay, chloroquine diphosphate, dexamethasone, indomethacin, penicillamine, piroxicam and diclofenac sodium were inactive; gold sodium thiomalate was inhibitory (IC50 = 20 microM).

摘要

使用多孔盖试验(Evans等人,(1986) Biosc. Rep. 6, 1041)对标准和新型白三烯B4(LTB4)类似物的中性粒细胞趋化活性进行了测试。该试验使用一次性设备,并通过能够穿过硝酸纤维素滤膜全厚度迁移的细胞数量来测量趋化性。在标准条件下(于含有2%牛白蛋白的缓冲液中37℃孵育90分钟),LTB4和6-顺式-LTB1的半数有效浓度(EC50)值分别为3.5和15,000 nM。20-羟基-LTB4与LTB4效力相当,并表现出类似的双相趋化反应,然而,穿过滤膜迁移的细胞数量仅为其三分之一。20-羧基-LTB4在高达1,000 nM时无活性。5-脱氧-((6,7)-顺式-环丙基)-LTB2、(6,7)-苯并-LTB2和5-脱氧-(8,10)-LTB2的EC50值分别为11,300、50,000和84,000 nM。棋盘分析表明,在导致趋化峰值的浓度下,LTB4的化学动力学成分占42%。将缓冲液中的白蛋白浓度降至0.5%会使LTB4和6-顺式-LTB1的表观效力提高五倍。由于LTB4是一种炎症介质,因此测试了各种抗炎剂在体内观察到的峰值浓度下,在含有0.5%白蛋白的情况下对LTB4刺激的趋化作用的体外抑制能力。在该试验条件下,磷酸氯喹、地塞米松、吲哚美辛、青霉胺、吡罗昔康和双氯芬酸钠无活性;硫代苹果酸金钠具有抑制作用(半数抑制浓度(IC50)= 20 microM)。

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