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酵母聚糖可增强猪肺泡巨噬细胞对白三烯D4的代谢。

Zymosan enhances leukotriene D4 metabolism by porcine alveolar macrophages.

作者信息

Paterson N A, McIver D J, Schurch S

出版信息

Immunology. 1985 Sep;56(1):153-9.

Abstract

Porcine alveolar macrophages (AM) metabolize leukotriene D4 (LTD4) to leukotriene E4 (LTE4). In the present study, the ability of a fluid-phase AM stimulus (A23187) and a phagocytic stimulus (opsonized zymosan) to augment LTD4 metabolism was examined. Both stimuli increased the release of superoxide (O-2) anions. However, whereas zymosan caused a consistent reduction in surface free energy, the effect of A23187 was variable. Similarly, zymosan induced release of the lysosomal enzymes N-acetyl-beta-D-glucosaminidase and arylsulphatase (mean net release, 14.9% and 12.0%, respectively), whereas release induced by A23187 was smaller (mean net release 1.42% and 1.31%, respectively) and of marginal statistical significance. Zymosan, but not A23187, caused a significant (P less than 0.005) augmentation of LTD4 inactivation: from 93 +/- 7 pM/10(7) cells (69 +/- 5% of added LTD4) at 60 min by control AM, to 117 +/- 3 pM/10(7) cells (88 +/- 2% of added LTD4) at 60 min by zymosan-treated AM. Zymosan also induced the release of LTD4 inactivating capacity (128 +/- 21 pM LTD4/10(7) AM/60 min) into the supernatant. Conversion of LTD4 to LTE4 by zymosan-treated AM and their supernatants was confirmed chromatographically. In addition, LTD4 inactivation by AM and their supernatants was inhibited by 10 mM L-cysteine. These data suggest that zymosan released a dipeptidase, possibly of lysosomal origin, which catalysed the conversion of LTD4 to LTE4.

摘要

猪肺泡巨噬细胞(AM)可将白三烯D4(LTD4)代谢为白三烯E4(LTE4)。在本研究中,检测了液相AM刺激物(A23187)和吞噬刺激物(调理酵母聚糖)增强LTD4代谢的能力。两种刺激均增加了超氧阴离子(O-2)的释放。然而,酵母聚糖导致表面自由能持续降低,而A23187的作用则存在差异。同样,酵母聚糖诱导溶酶体酶N-乙酰-β-D-氨基葡萄糖苷酶和芳基硫酸酯酶释放(平均净释放率分别为14.9%和12.0%),而A23187诱导的释放量较小(平均净释放率分别为1.42%和1.31%),且具有边缘统计学意义。酵母聚糖而非A23187导致LTD4失活显著增强(P<0.005):对照AM在60分钟时为93±7 pM/10(7) 个细胞(占添加LTD4的69±5%),经酵母聚糖处理的AM在60分钟时为117±3 pM/10(7) 个细胞(占添加LTD4的88±2%)。酵母聚糖还诱导LTD4失活能力(128±21 pM LTD4/10(7) AM/60分钟)释放到上清液中。经酵母聚糖处理的AM及其上清液将LTD4转化为LTE4通过色谱法得到证实。此外,AM及其上清液对LTD4的失活受到10 mM L-半胱氨酸的抑制。这些数据表明,酵母聚糖释放了一种二肽酶,可能来源于溶酶体,它催化LTD4转化为LTE4。

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