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气道平滑肌分泌的趋化因子诱导肥大细胞脱颗粒的单细胞分析。

Single-cell analysis of mast cell degranulation induced by airway smooth muscle-secreted chemokines.

作者信息

Manning Benjamin M, Meyer Audrey F, Gruba Sarah M, Haynes Christy L

机构信息

Department of Chemistry, University of Minnesota, Minneapolis, MN 55455, USA.

Department of Chemistry, University of Minnesota, Minneapolis, MN 55455, USA.

出版信息

Biochim Biophys Acta. 2015 Sep;1850(9):1862-8. doi: 10.1016/j.bbagen.2015.05.008. Epub 2015 May 15.

Abstract

BACKGROUND

Asthma is a chronic inflammatory disease characterized by narrowed airways, bronchial hyper-responsiveness, mucus hyper-secretion, and airway remodeling. Mast cell (MC) infiltration into airway smooth muscle (ASM) is a defining feature of asthma, and ASM regulates the inflammatory response by secreting chemokines, including CXCL10 and CCL5. Single cell analysis offers a unique approach to study specific cellular signaling interactions within large and complex signaling networks such as the inflammatory microenvironment in asthma.

METHODS

Carbon-fiber microelectrode amperometry was used to study the effects of ASM-secreted chemokines on mouse peritoneal MC degranulation.

RESULTS

MC degranulation in response to CXCL10 and CCL5 was monitored at the single cell level. Relative to IgE-mediated degranulation, CXCL10- and CCL5-stimulated MCs released a decreased amount of serotonin per granule with fewer release events per cell. Decreased serotonin release per granule was correlated with increased spike half-width and rise-time values.

CONCLUSIONS

MCs are directly activated by ASM-associated chemokines. CXCL10 and CCL5 induce less robust MC degranulation compared to IgE- and A23187-stimulation. The kinetics of MC degranulation are signaling pathway-dependent, suggesting a biophysical mechanism of regulated degranulation that incorporates control over granule trafficking, transport, and docking machinery.

GENERAL SIGNIFICANCE

The biophysical mechanisms, including variations in number of exocytotic release events, serotonin released per granule, and the membrane kinetics of exocytosis that underlie MC degranulation in response to CXCL10 and CCL5 were characterized at the single cell level. These findings clarify the function of ASM-derived chemokines as instigators of MC degranulation relative to classical mechanisms of MC stimulation.

摘要

背景

哮喘是一种慢性炎症性疾病,其特征为气道狭窄、支气管高反应性、黏液分泌过多以及气道重塑。肥大细胞(MC)浸润至气道平滑肌(ASM)是哮喘的一个决定性特征,并且ASM通过分泌趋化因子(包括CXCL10和CCL5)来调节炎症反应。单细胞分析为研究大型复杂信号网络(如哮喘炎症微环境)内特定细胞信号相互作用提供了一种独特方法。

方法

采用碳纤维微电极安培法研究ASM分泌的趋化因子对小鼠腹膜MC脱颗粒的影响。

结果

在单细胞水平监测了MC对CXCL10和CCL5的脱颗粒反应。相对于IgE介导的脱颗粒,CXCL10和CCL5刺激的MC每个颗粒释放的5-羟色胺量减少,每个细胞的释放事件也较少。每个颗粒5-羟色胺释放量的减少与峰值半宽度和上升时间值的增加相关。

结论

MC被ASM相关趋化因子直接激活。与IgE和A23187刺激相比,CXCL10和CCL5诱导的MC脱颗粒作用较弱。MC脱颗粒的动力学是信号通路依赖性的,提示了一种调节脱颗粒的生物物理机制,该机制涉及对颗粒运输、转运和对接机制的控制。

一般意义

在单细胞水平上表征了响应CXCL10和CCL5的MC脱颗粒的生物物理机制,包括胞吐释放事件的数量变化、每个颗粒释放的5-羟色胺以及胞吐作用的膜动力学。这些发现阐明了ASM衍生趋化因子相对于MC刺激经典机制作为MC脱颗粒激发剂的功能。

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