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全血及纯化后中性粒细胞的功能:受体表达、氧化酶活性及对细胞因子反应性的变化

Neutrophil function in whole blood and after purification: changes in receptor expression, oxidase activity and responsiveness to cytokines.

作者信息

Watson F, Robinson J J, Edwards S W

机构信息

Dept. of Biochemistry, University of Liverpool.

出版信息

Biosci Rep. 1992 Apr;12(2):123-33. doi: 10.1007/BF02351217.

DOI:10.1007/BF02351217
PMID:1421055
Abstract

Neutrophil function and plasma membrane receptor expression was measured in cell suspensions isolated by two separate procedures and in unfractionated whole blood. When cells were prepared by a combined dextran/ficoll procedure, their ability to generate reactive oxidants in response to fMet-Leu-Phe was greater than in corresponding cells isolated by a one-step procedure on Mono-Poly Resolving Medium (M-PRM). Cells prepared by both methods could be primed in vitro by rGM-CSF, but the priming ratio was greater in cells prepared by the latter method. The ability of neutrophils in whole blood to generate reactive oxidants in response to fMet-Leu-Phe was extremely low, but this was increased by more than 10 fold if the blood was pre-incubated with rGM-CSF. Similarly, expression of CD 11b and CD 16 was very low (or undetectable) in neutrophils in whole blood, but this was rapidly increased upon priming. Activation by PMA resulted in a down regulation of CD 16 expression as the receptor was shed from the cell surface. Neutrophils isolated by either the dextran/ficoll or the M-PRM method showed increased expression of receptors compared with those in whole blood, although this expression was lower in cells isolated by the latter method. These data indicate that the isolation procedures used to obtain purified neutrophils prime both receptor expression and oxidase function, although these effects are minimalised in isolation procedures using M-PRM. Furthermore, as CD 16 expression on neutrophils in whole blood is rapidly up-regulated during priming, it seems likely that, as for complement receptors, rapidly-mobilisable intracellular stores of this receptor exist.

摘要

采用两种不同方法分离得到的细胞悬液以及未分离的全血中,均对中性粒细胞功能和质膜受体表达进行了检测。当通过葡聚糖/聚蔗糖联合法制备细胞时,其对甲酰甲硫氨酰-亮氨酰-苯丙氨酸(fMet-Leu-Phe)产生反应性氧化剂的能力,强于在单克隆-多聚分辨培养基(M-PRM)上通过一步法分离得到的相应细胞。两种方法制备的细胞均可在体外被重组粒细胞-巨噬细胞集落刺激因子(rGM-CSF)激活,但后一种方法制备的细胞激活率更高。全血中的中性粒细胞对fMet-Leu-Phe产生反应性氧化剂的能力极低,但如果血液预先与rGM-CSF孵育,该能力可提高10倍以上。同样,全血中性粒细胞中CD11b和CD16的表达非常低(或无法检测到),但激活后会迅速增加。佛波酯(PMA)激活会导致CD16表达下调,因为该受体从细胞表面脱落。与全血中的中性粒细胞相比,通过葡聚糖/聚蔗糖法或M-PRM法分离得到的中性粒细胞受体表达增加,尽管后一种方法分离的细胞中该表达较低。这些数据表明,用于获得纯化中性粒细胞的分离程序会引发受体表达和氧化酶功能的改变,尽管在使用M-PRM的分离程序中这些影响最小化。此外,由于全血中性粒细胞上的CD16表达在激活过程中迅速上调,因此与补体受体一样,这种受体似乎存在可快速动员的细胞内储存库。

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