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Complete Cell Killing by Applying High Hydrostatic Pressure for Acellular Vascular Graft Preparation

机译:通过施加高的静水压力来制备无细胞血管移植物从而完全杀死细胞。

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摘要

Pressure treatment has been developed in tissue engineering application. Although the tissue scaffold prepared by a ultrahydrostatic pressure treatment has been reported, an excessive pressure has a potential to disrupt a structure of extracellular matrix through protein denaturation. It is important to understand the suitable low-pressure condition and mechanisms for cell killing. In this study, cellular morphology, mitochondria activity, and membrane permeability of mammalian cells with various pressure treatments were investigated with in vitro models. When the cells were treated with a pressure of 100 MPa for 10 min, cell morphology and adherence were the same as an untreated cells. Dehydrogenase activity in mitochondria was almost the same as untreated cells. On the other hand, when the cells were treated with the pressure of more than 200 MPa, the cells did not adhere, and the dehydrogenase activity was completely suppressed. However, green fluorescence was observed in the live/dead staining images, and the cells were completely stained as red after above 500 MPa. That is, membrane permeability was disturbed with the pressure treatment of above 500 MPa. These results indicated that the pressure of 200 MPa for 10 min was enough to induce cell killing through inactivation of mitochondria activity.
机译:在组织工程应用中已经开发了压力治疗。尽管已经报道了通过超静水压处理制备的组织支架,但是过大的压力可能通过蛋白质变性破坏细胞外基质的结构。重要的是要了解合适的低压条件和杀死细胞的机制。在这项研究中,通过体外模型研究了各种压力处理下的哺乳动物细胞的细胞形态,线粒体活性和膜通透性。将细胞在100 MPa的压力下处理10分钟,其细胞形态和粘附性与未处理的细胞相同。线粒体中的脱氢酶活性与未处理的细胞几乎相同。另一方面,当用大于200 MPa的压力处理细胞时,细胞不粘附,并且脱氢酶活性被完全抑制。然而,在活/死染色图像中观察到绿色荧光,并且在高于500 MPa后细胞被完全染成红色。即,超过500 MPa的压力处理会破坏膜的渗透性。这些结果表明200 MPa的压力持续10分钟,足以通过灭活线粒体活性来诱导细胞杀伤。

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