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单个肺泡巨噬细胞超氧化物释放的测量

Measurement of superoxide release from single pulmonary alveolar macrophages.

作者信息

DiGregorio K A, Cilento E V, Lantz R C

出版信息

Am J Physiol. 1987 Jun;252(6 Pt 1):C677-83. doi: 10.1152/ajpcell.1987.252.6.C677.

Abstract

An electrooptical method was developed to quantify superoxide (O2-) release from single rat pulmonary alveolar macrophages (PAM) during adherence to the bottom of a culture dish. This was done by measuring the reduction of nitro blue tetrazolium (NBT) to a diformazan precipitate at 550 nm from videorecorded images of individual cells. Temporal changes in cell optical density, which are proportional to the mass of diformazan produced, were calculated from videophotometric measurements of the change in light intensity over individual cells. Total diformazan produced increased 78 and 126% with an increase in NBT from 0.5 to 1.0 and 2.0 mg/ml, respectively. Total diformazan produced and maximum rate of production among individual PAM varied two- to threefold providing strong evidence for heterogeneity in O2- production. Specific inhibition of O2- production by superoxide dismutase, iodoacetate, and chlorpromazine significantly reduced the total diformazan produced and maximum rate of diformazan production. Hydrogen peroxide was not involved in NBT reduction, since catalase alone did not significantly change diformazan production. This novel method to quantify O2- release from single PAM should be valuable in analyzing heterogeneity and single cell kinetics of O2- production, in assessing the effects of exposure of cells to particulates on O2- release, and in relating release to electrophysiological measurements.

摘要

开发了一种电光方法,用于量化单个大鼠肺泡巨噬细胞(PAM)在贴附于培养皿底部时超氧化物(O2-)的释放。这是通过从单个细胞的视频记录图像中测量在550nm处硝基蓝四唑(NBT)还原为双甲臜沉淀来实现的。根据对单个细胞上光强度变化的视频光度测量,计算出与产生的双甲臜质量成比例的细胞光密度的时间变化。随着NBT从0.5增加到1.0和2.0mg/ml,产生的双甲臜总量分别增加了78%和126%。单个PAM中产生的双甲臜总量和最大产生速率变化了两到三倍,这为O2-产生的异质性提供了有力证据。超氧化物歧化酶、碘乙酸盐和氯丙嗪对O2-产生的特异性抑制显著降低了产生的双甲臜总量和双甲臜产生的最大速率。过氧化氢不参与NBT的还原,因为单独的过氧化氢酶并没有显著改变双甲臜的产生。这种量化单个PAM中O2-释放的新方法在分析O2-产生的异质性和单细胞动力学、评估细胞暴露于颗粒物对O2-释放的影响以及将释放与电生理测量相关联方面应该是有价值的。

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