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首页> 外文期刊>Ultrasonics, Ferroelectrics and Frequency Control, IEEE Transactions on >Observations on the viability of C6-glioma cells after sonoporation with low-intensity ultrasound and microbubbles
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Observations on the viability of C6-glioma cells after sonoporation with low-intensity ultrasound and microbubbles

机译:低强度超声和微泡声处理C6-神经胶质瘤细胞活力的观察

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摘要

Ultrasound (US) and microbubbles can be used to facilitate cellular uptake of drugs through a cavitationinduced enhancement of cell membrane permeability. The mechanism is, however, still incompletely understood. A direct contact between microbubbles and cell membrane is thought to be essential to create membrane perturbations lasting from seconds to minutes after US exposure of the cells. A recent study showed that the effect may even last up to 8 h after cavitation (with residual permeability up to 24 h after cavitation). In view of possible membrane damage, the purpose of this study was to further investigate the evolution of cell viability in the range of the 24-h temporal window. Furthermore, a description of the functional changes in tumor cells after US exposure was initiated to obtain a better understanding of the mechanism of membrane perturbation after sonication with microbubbles. Our results suggest that US does not reduce cell viability up to 24 h post-exposure. However, a perturbation of the entire cell population exposed to US was observed in terms of enzymatic activity and characteristics of the mitochondrial membrane. Furthermore, we demonstrated that US cavitation induces a transient loss of cell membrane asymmetry, resulting in phosphatidylserine exposure in the outer leaflet of the cell membrane.
机译:超声(US)和微气泡可通过空化诱导的细胞膜通透性增强来促进药物的细胞摄取。但是,该机制仍未完全理解。人们认为,微泡与细胞膜之间的直接接触对于在细胞暴露于美国后数秒至数分钟内产生持续的膜扰动至关重要。最近的一项研究表明,这种作用甚至在空化后可持续长达8小时(在空化后残留渗透率长达24小时)。考虑到可能的膜损伤,该研究的目的是进一步研究24小时时间窗范围内细胞活力的演变。此外,开始了对US暴露后肿瘤细胞功能变化的描述,以更好地理解微泡超声处理后膜微扰的机制。我们的结果表明,在暴露后24小时内,US不会降低细胞活力。然而,就酶活性和线粒体膜特征而言,观察到暴露于US的整个细胞群均受到干扰。此外,我们证明了美国空化会引起细胞膜不对称性的短暂丧失,从而导致磷脂酰丝氨酸在细胞膜的外部小叶中暴露。

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