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用[(99m)Tc] - 锡胶体锝标记中性粒细胞是由补体受体3介导的,并增强了中性粒细胞对脂多糖的预激反应。

Neutrophil labeling with [(99m)Tc]-technetium stannous colloid is complement receptor 3-mediated and increases the neutrophil priming response to lipopolysaccharide.

作者信息

Gallagher Hayley, Ramsay Stuart C, Barnes Jodie, Maggs Jacqueline, Cassidy Nathan, Ketheesan Natkunam

机构信息

School of Veterinary and Biomedical Sciences, James Cook University, Townsville, Queensland 4811, Australia.

出版信息

Nucl Med Biol. 2006 Apr;33(3):433-9. doi: 10.1016/j.nucmedbio.2005.12.014. Epub 2006 Mar 9.

DOI:10.1016/j.nucmedbio.2005.12.014
PMID:16631093
Abstract

INTRODUCTION

[(99m)Tc]-technetium stannous colloid (TcSnC)-labeled white cells are used to image inflammation. Neutrophil labeling with TcSnC is probably phagocytic, but the phagocytic receptor involved is not known. We hypothesised that complement receptor 3 (CR3) plays a key role. Phagocytic labeling could theoretically result in neutrophil activation or priming, affecting the behaviour of labeled cells. Fluorescence-activated cell sorter (FACS) analysis side scatter measurements can assess neutrophil activation and priming.

METHODS

We tested whether TcSnC neutrophil labeling is CR3-mediated by assessing if neutrophil uptake of TcSnC was inhibited by a monoclonal antibody (mAb) directed at the CD11b component of CR3. We tested if TcSnC-labeled neutrophils show altered activation or priming status, comparing FACS side scatter in labeled and unlabeled neutrophils and examining the effect of lipopolysaccharide (LPS), a known priming agent.

RESULTS

Anti-CD11b mAb reduced neutrophil uptake of TcSnC in a dose-dependent fashion. Labeled neutrophils did not show significantly increased side scatter compared to controls. LPS significantly increased side scatter in control cells and labeled neutrophils. However, the increase was significantly greater in labeled neutrophils than unlabeled cells.

CONCLUSIONS

Neutrophil labeling with TcSnC is related to the function of CR3, a receptor which plays a central role in phagocytosis. TcSnC labeling did not significantly activate or prime neutrophils. However, labeled neutrophils showed a greater priming response to LPS. This could result in labeled neutrophils demonstrating increased adhesion on activated endothelium at sites of infection.

摘要

引言

[(99m)Tc] - 锝锡胶体(TcSnC)标记的白细胞用于炎症成像。用TcSnC标记中性粒细胞可能是通过吞噬作用,但涉及的吞噬受体尚不清楚。我们假设补体受体3(CR3)起关键作用。理论上,吞噬标记可能导致中性粒细胞活化或致敏,从而影响标记细胞的行为。荧光激活细胞分选仪(FACS)分析侧向散射测量可以评估中性粒细胞的活化和致敏情况。

方法

我们通过评估针对CR3的CD11b成分的单克隆抗体(mAb)是否抑制中性粒细胞对TcSnC的摄取,来测试TcSnC对中性粒细胞的标记是否由CR3介导。我们通过比较标记和未标记中性粒细胞的FACS侧向散射,并检查已知的致敏剂脂多糖(LPS)的作用,来测试TcSnC标记的中性粒细胞是否显示出改变的活化或致敏状态。

结果

抗CD11b mAb以剂量依赖方式减少中性粒细胞对TcSnC的摄取。与对照组相比,标记的中性粒细胞侧向散射没有显著增加。LPS显著增加了对照细胞和标记中性粒细胞的侧向散射。然而,标记中性粒细胞的增加显著大于未标记细胞。

结论

用TcSnC标记中性粒细胞与CR3的功能有关,CR3是一种在吞噬作用中起核心作用的受体。TcSnC标记没有显著激活或致敏中性粒细胞。然而,标记的中性粒细胞对LPS表现出更大的致敏反应。这可能导致标记的中性粒细胞在感染部位的活化内皮上表现出增加的粘附。

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