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Piezotolerance of the cytoskeletal structure in cultured deep-sea fish cells using DNA transfection and protein introduction techniques

机译:DNA转染和蛋白质导入技术对深海鱼类细胞骨架的压电耐受性

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We used DNA transfection and protein introduction techniques to investigate the pressure tolerance of cytoskeletal structures in pectoral fin cells derived from the deep-sea fish Simenchelys parasiticus (habitat depth, 366–2,630 m). The deep-sea fish cells have G418 resistance. The cell number increased until day 6 of cultivation and all cells had died by day 35 when cultured in 35-mm Petri dishes in medium containing G418. Enhanced yellow fluorescent protein-tagged human β-actin (EYFP-actin) was stably expressed by 1 in 100,000 deep-sea fish cells. Because almost none of the EYFP-actin was incorporated into actin filaments of the cells, we replaced the relatively large EYFP tag with a chemical fluorescent compound and succeeded in incorporating fluorescently labeled rabbit actins into the deep-sea fish actin filaments. Most of the filament structure in the cells with rabbit actin inserted underwent depolymerization when subjected to pressure of 100 MPa for 20 min, in contrast to control cells. There were no differences in the tubulin filament structure between control cells and deep-sea fish cells with fluorescein-labeled bovine tubulin inserted after the application of pressure ranging from 40 to 100 MPa for 20 min.
机译:我们使用DNA转染和蛋白质导入技术研究了深海鱼类Simenchelys parasiticus(栖息地深度366-2,630 m)的胸鳍细胞中细胞骨架结构的耐压性。深海鱼细胞具有G418抗性。在培养的第6天之前,细胞数量增加,并且当在含G418的35mm培养皿中培养时,所有细胞在第35天都死亡。标记有黄色荧光蛋白的增强型人β-肌动蛋白(EYFP-actin)在100,000个深海鱼类细胞中稳定表达了1个。因为几乎没有EYFP-actin掺入细胞的肌动蛋白丝中,所以我们用化学荧光化合物代替了较大​​的EYFP标签,并成功地将荧光标记的兔肌动蛋白掺入了深海鱼类肌动蛋白丝中。与对照细胞相比,插入兔肌动蛋白的细胞中的大多数细丝结构在100 MPa的压力下持续20分钟时都会发生解聚。在施加40至100 MPa的压力20分钟后,插入荧光素标记的牛微管蛋白的对照细胞和深海鱼细胞之间的微管蛋白丝结构没有差异。

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