使用具有耗散功能的石英晶体微天平对纳米颗粒诱导的血小板微聚集进行药理学表征:与光聚集法的比较。
Pharmacological characterization of nanoparticle-induced platelet microaggregation using quartz crystal microbalance with dissipation: comparison with light aggregometry.
作者信息
Santos-Martinez Maria J, Tomaszewski Krzysztof A, Medina Carlos, Bazou Despina, Gilmer John F, Radomski Marek W
机构信息
School of Pharmacy and Pharmaceutical Sciences and Trinity Biomedical Sciences Institute, University of Dublin, Dublin, Ireland ; School of Medicine, Trinity College Dublin, University of Dublin, Dublin, Ireland.
School of Pharmacy and Pharmaceutical Sciences and Trinity Biomedical Sciences Institute, University of Dublin, Dublin, Ireland ; Department of Anatomy, Jagiellonian University Medical College, Krakow, Poland.
出版信息
Int J Nanomedicine. 2015 Aug 13;10:5107-19. doi: 10.2147/IJN.S84305. eCollection 2015.
BACKGROUND
Engineered nanoparticles (NPs) can induce platelet activation and aggregation, but the mechanisms underlying these interactions are not well understood. This could be due in part to use of devices that study platelet function under quasi-static conditions with low sensitivity to measure platelet microaggregation. Therefore, in this study we investigated the pharmacological pathways and regulators of NP-induced platelet microaggregation under flow conditions at nanoscale using quartz crystal microbalance with dissipation (QCM-D) and compared the data thus obtained with those generated by light aggregometry.
METHODS
Blood was collected from healthy volunteers, and platelet-rich plasma was obtained. Thrombin receptor-activating peptide, a potent stimulator of platelet function, and pharmacological inhibitors were used to modulate platelet microaggregation in the presence/absence of silica (10 nm and 50 nm) and polystyrene (23 nm) NPs. Light aggregometry was used to study platelet aggregation in macroscale. Optical, immunofluorescence, and scanning electron microscopy were also used to visualize platelet aggregates.
RESULTS
Platelet microaggregation was enhanced by thrombin receptor-activating peptide, whereas prostacyclin, nitric oxide donors, acetylsalicylic acid, and phenanthroline, but not adenosine diphosphate (ADP) blockers, were able to inhibit platelet microaggregation. NPs caused platelet microaggregation, an effect not detectable by light aggregometry. NP-induced microaggregation was attenuated by platelet inhibitors.
CONCLUSION
NP-induced platelet microaggregation appears to involve classical proaggregatory pathways (thromboxane A2-mediated and matrix metalloproteinase-2-mediated) and can be regulated by endogenous (prostacyclin) and pharmacological (acetylsalicylic acid, phenanthroline, and nitric oxide donors) inhibitors of platelet function. Quartz crystal microbalance with dissipation, but not light aggregometry, is an appropriate method for studying NP-induced microaggregation.
背景
工程纳米颗粒(NPs)可诱导血小板活化和聚集,但其相互作用的潜在机制尚未完全明确。部分原因可能是所使用的设备在准静态条件下研究血小板功能,对测量血小板微聚集的灵敏度较低。因此,在本研究中,我们使用具有耗散功能的石英晶体微天平(QCM-D)在纳米尺度的流动条件下研究了NPs诱导血小板微聚集的药理途径和调节因子,并将所得数据与光聚集法产生的数据进行了比较。
方法
采集健康志愿者的血液,获得富含血小板的血浆。在存在/不存在二氧化硅(10 nm和50 nm)和聚苯乙烯(23 nm)NPs的情况下,使用凝血酶受体激活肽(一种有效的血小板功能刺激剂)和药理抑制剂来调节血小板微聚集。光聚集法用于研究宏观尺度下的血小板聚集。光学、免疫荧光和扫描电子显微镜也用于观察血小板聚集体。
结果
凝血酶受体激活肽增强了血小板微聚集,而前列环素、一氧化氮供体、乙酰水杨酸和菲咯啉能够抑制血小板微聚集,而二磷酸腺苷(ADP)阻滞剂则不能。NPs导致血小板微聚集,这一效应无法通过光聚集法检测到。血小板抑制剂可减弱NPs诱导的微聚集。
结论
NPs诱导的血小板微聚集似乎涉及经典的促聚集途径(血栓素A2介导和基质金属蛋白酶-2介导),并且可以被血小板功能的内源性(前列环素)和药理(乙酰水杨酸、菲咯啉和一氧化氮供体)抑制剂所调节。具有耗散功能的石英晶体微天平是研究NPs诱导微聚集的合适方法,而光聚集法并非如此。
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