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Fast method for the estimation of heart valve leaflet viability

机译:评估心脏瓣膜小叶生存力的快速方法

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Background: The assessing of heart valve viability is critical for the preparing of viable and implantable biological value. Non-viable valves should be cross-linked with various agents whereas viable tissues are suitable for cryoprotection. Cell viability assessment should be rapid, simple, easy and low cost.Material/Methods: A simple method, simultaneous fluorescent staining of both viable and damaged valve cells was described. The material was consisted of 2 groups: a) with ischemic time below 3 hours (5 swine valves), and b) with ischemic time over 3 hours (5 swine valves). The supravital staining of leaflet fragments was conducted with single solution of fluorescein diacetate (living cells staining) and propodium iodide (damaged cells staining).Results: The simultaneous staining predominantly showed green fluorescence typical for living cells and few red damaged cells in the short ischemic time group, whereas the second group showed the predominance of the red stained damaged cells.Conclusions: The presented one-step supravital staining method is rapid and simple it allows differentiation of the viability of the valve cells, so it may be of value for the routine evaluation of cadaveric valve homografts
机译:背景:心脏瓣膜生存力的评估对于准备可行的和可植入的生物学价值至关重要。无效的瓣膜应与各种试剂交联,而有效的组织则适合进行冷冻保护。细胞生存力评估应快速,简单,容易且成本低廉。材料/方法:描述了一种简单的方法,同时对生存和受损的瓣膜细胞进行了荧光染色。该材料由2组组成:a)缺血时间低于3小时(5个猪瓣膜),b)缺血时间超过3小时(5个猪瓣膜)。小叶片段的上膜染色用荧光素双乙酸盐(活细胞染色)和碘化丙啶(损伤的细胞染色)的单一溶液进行。结论:所提出的一步式胃上染色方法快速,简单,可以区分瓣膜细胞的活力,因此可能具有一定的价值。尸体瓣膜同种异体移植的常规评估

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