应用流式细胞术鉴定和表征自然杀伤细胞上的瞬时受体电位 melastatin 2 和 CD38 通道。

Identification and characterisation of transient receptor potential melastatin 2 and CD38 channels on natural killer cells using the novel application of flow cytometry.

机构信息

School of Medical Science, Griffith University, Gold Coast, QLD, Australia.

The National Centre for Neuroimmunology and Emerging Diseases, Menzies Health Institute Queensland, Griffith University, Gold Coast, Southport, QLD, 4222, Australia.

出版信息

BMC Immunol. 2019 May 10;20(1):14. doi: 10.1186/s12865-019-0293-0.

DOI:10.1186/s12865-019-0293-0

PMID:31077146

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6509826/

Abstract

BACKGROUND

Natural Killer (NK) cells are effector lymphocytes of the innate immune system and are subclassed into CD56CD16 and CD56CD16 NK cells. Intracellular calcium (Ca) is fundamental to regulate a number of intracellular signalling pathways and functions in NK cells, which are essential in mediating their natural cytotoxic function. Transient receptor potential melastatin 2 (TRPM2) is a Ca-permeable non-selective cation channel that possesses a critical role in calcium-dependent cell signalling to maintain cellular homeostasis. TRPM2 and CD38 protein surface expression has yet to be determined on NK cells using flow cytometry. Characterisation of TRPM2 has been previously identified by in vivo models, primarily using methods such as genetic remodification, immunohistochemistry and whole cell electrophysiology. The aim of this study was to develop an in vitro methodology to characterise TRPM2 and CD38 surface expression on NK cell subsets using an antibody that has not been previously applied using flow cytometry.

RESULTS

At 2 h/1 h, TRPM2 (Fig. 2 A, B, p < 0.05) and TRPM2/CD38 (Fig. 3A, B, p < 0.05) surface expression significantly increased between 1:300 and 1:50 at 2 h/1 h. TRPM2/CD38 surface expression furthermore increased between 1:100 and 1:50 at 2 h/1 h (Fig. 3A, p < 0.05). Interestingly, TRPM2/CD38 surface expression significantly decreased from 1:50 to 1:5 on CD56CD16 NK cells. These consistent findings highlight that 1:50 is the optimal antibody dilution and threshold to measure TRPM2 and TRPM2/CD38 surface expression on NK subsets. 2 h/1 h was determined as the optimal incubation period to ensure a sufficient timeframe for maximal antibody binding and surface expression.

CONCLUSION

For the first time, we describe an in vitro methodology to characterise TRPM2 and CD38 surface expression on NK cells in healthy participants. Finally, using an antibody that has not been previously applied in flow cytometry, we determined an antibody concentration and incubation time that is robust, rapid and sensitive for the application of flow cytometry.

摘要

背景

自然杀伤 (NK) 细胞是先天免疫系统的效应淋巴细胞，可分为 CD56CD16 和 CD56CD16 NK 细胞。细胞内钙离子 (Ca) 是调节 NK 细胞内许多信号通路和功能的基础，这些功能对于介导其天然细胞毒性功能至关重要。瞬时受体电位 melastatin 2 (TRPM2) 是一种 Ca 通透性非选择性阳离子通道，在维持细胞内稳态的 Ca 依赖性细胞信号转导中具有关键作用。使用流式细胞术尚未确定 NK 细胞上的 TRPM2 和 CD38 蛋白表面表达。TRPM2 的特征以前已经通过体内模型确定，主要使用遗传重塑、免疫组织化学和全细胞电生理学等方法。本研究的目的是开发一种使用尚未通过流式细胞术应用的抗体来表征 NK 细胞亚群上的 TRPM2 和 CD38 表面表达的体外方法。

结果

在 2 小时/1 小时时，TRPM2（图 2A、B，p<0.05）和 TRPM2/CD38（图 3A、B，p<0.05）表面表达在 2 小时/1 小时时在 1:300 和 1:50 之间显著增加。TRPM2/CD38 表面表达在 2 小时/1 小时时也在 1:100 和 1:50 之间增加（图 3A，p<0.05）。有趣的是，CD56CD16 NK 细胞上的 TRPM2/CD38 表面表达从 1:50 减少到 1:5。这些一致的发现强调，1:50 是测量 NK 亚群上的 TRPM2 和 TRPM2/CD38 表面表达的最佳抗体稀释度和阈值。确定 2 小时/1 小时是最佳孵育期，以确保有足够的时间进行最大的抗体结合和表面表达。