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通过改良的髓过氧化物酶测定法测量脑和肺组织中的中性粒细胞含量。

Measurement of neutrophil content in brain and lung tissue by a modified myeloperoxidase assay.

作者信息

Kuebler W M, Abels C, Schuerer L, Goetz A E

机构信息

Institute for Surgical Research, University of Munich, Germany.

出版信息

Int J Microcirc Clin Exp. 1996 Mar-Apr;16(2):89-97. doi: 10.1159/000179155.

Abstract

Myeloperoxidase (MPO) activity is assessed for the quantification of neutrophil accumulation in tissues. In particular, it may be used to support in vivo data on leukocyte kinetics obtained by intravital microscopy and to clarify whether phenomena observed on the organ surface reflect the situation of the whole organ microcirculation. Previous measurements of MPO activity were limited by interference with other peroxidases and by inhibition of MPO activity by specific enzymes. To circumvent these limitations, a modified assay was devised that combined a two-step tissue homogenization technique with heat incubation in a continuous photometric measurement. MPO activity was quantified in neutrophils isolated from rat and rabbit whole blood, rat brain and rabbit lung and compared with intravital microscopic data on leukocyte accumulation. The modified assay is characterized by high reproducibility, strong correlation of MPO activity with number of neutrophils and full recovery of neutrophils added to tissue homogenate. MPO activity per neutrophil was 342.9 +/- 11.7 mU/10(6) cells in rats and 40.3 +/- 0.8 mU/10(6) cells in rabbits. MPO activity in tissue was significantly lower in rat brains (18.9 +/- 29.7 mU/g) as compared to rabbit lungs (741 +/- 67 mU/g). Whereas global cerebral ischemia/reperfusion did not increase MPO activity in rat brain (18.1 +/- 26.1 mU/g), intravenous infusion of cobra venom factor (1,447 +/- 407 mU/g) or endotoxin (1,439 +/- 285 mU/g), enhanced MPO activity in rabbit lung. These results parallel microcirculatory data from the organ surface. Therefore they supplement the intravital microscopic observations by demonstrating that these are indeed representative of deeper parenchymal tissue areas.

摘要

髓过氧化物酶(MPO)活性用于评估组织中中性粒细胞的积聚情况。特别是,它可用于支持通过活体显微镜获得的关于白细胞动力学的体内数据,并阐明在器官表面观察到的现象是否反映了整个器官微循环的情况。先前对MPO活性的测量受到其他过氧化物酶的干扰以及特定酶对MPO活性的抑制作用的限制。为了克服这些限制,设计了一种改良的测定方法,该方法将两步组织匀浆技术与热孵育相结合,并进行连续光度测量。在从大鼠和兔全血、大鼠脑和兔肺中分离出的中性粒细胞中对MPO活性进行了定量,并与关于白细胞积聚的活体显微镜数据进行了比较。改良后的测定方法具有高重现性、MPO活性与中性粒细胞数量的强相关性以及添加到组织匀浆中的中性粒细胞的完全回收率等特点。大鼠每中性粒细胞的MPO活性为342.9±11.7 mU/10(6) 个细胞,兔子为40.3±0.8 mU/10(6) 个细胞。与兔肺(741±67 mU/g)相比,大鼠脑内组织中的MPO活性显著较低(18.9±29.7 mU/g)。虽然全脑缺血/再灌注并未增加大鼠脑内的MPO活性(18.1±26.1 mU/g),但静脉注射眼镜蛇毒因子(1,447±407 mU/g)或内毒素(1,439±285 mU/g)可增强兔肺中的MPO活性。这些结果与来自器官表面的微循环数据一致。因此,它们通过证明这些观察结果确实代表更深层实质组织区域,补充了活体显微镜观察结果。

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