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Improvement of the culture stability of non-anchorage-dependent animal cells grown in serum-free media through immobilization

机译:通过固定提高在无血清培养基中生长的非锚定依赖性动物细胞的培养稳定性

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A murine hybridoma cell line producing a monoclonal antibody against penicillin-G-amidase and a murine transfectoma cell line secreting a monovalent chimeric human/mouse Fab-antibody fragment were cultivated in three different media (serum-containing, low protein serum-free, and iron-rich protein-free) in flask cultures, stirred reactors and a fixed bed reactor. In static batch cultures in flasks both cell lines showed similar good growth in all three media.In suspension in a stirred reactor, the hybridoma cell line could be cultivated satisfactory only in serum-containing medium. In low protein serum-free medium, Pluronic F68 had to be added to protect the hybridoma cells against shear stress. But even with this supplement only batch, not chemostat mode was possible. In iron-rich protein-free medium the hybridoma cells grew also in continuous chemostat mode, but the stability of the culture was low. The transfectoma cell line did not grow in stirred reactors in any of the three media.Good results with both cell lines were obtained in fixed bed experiments, where the cells were immobilized in macroporous Siran?-carriers. The media, which were optimized in flask cultures, could be used without any further adaptation in the fixed bed reactor. Immobilization improved the stability and reliability of cultures of non-adherent animal cells in serum-free media tremendously compared to suspension cultures in stirred reactors. The volume-specific glucose uptake rate, an, indicator of the activity of the immobilized cells, was similar in all three media. Deviations in the metabolism of immobilized and suspended cells seem to be mainly due to low oxygen concentrations within the macroporous carriers, where the cells are supplied with oxygen only by diffusion.
机译:在三种不同的培养基(含血清,低蛋白,无血清和无血清)中培养产生抗青霉素-G-酰胺酶单克隆抗体的鼠杂交瘤细胞系和分泌单价嵌合人/小鼠Fab-抗体片段的鼠转染瘤细胞系。烧瓶培养,搅拌反应器和固定床反应器中)。在烧瓶中进行静态分批培养时,两种细胞在所有三种培养基中均表现出相似的良好生长。在搅拌反应器中的悬浮液中,杂交瘤细胞仅在含血清的培养基中才能令人满意地培养。在低蛋白无血清培养基中,必须添加Pluronic F68以保护杂交瘤细胞免受剪切应力。但是即使仅使用此补充剂,也无法实现恒化器模式。在富含铁的无蛋白培养基中,杂交瘤细胞也以连续的化学恒温模式生长,但是培养物的稳定性很低。在三种培养基中的任何一种中,转染瘤细胞系均未在搅拌反应器中生长。在固定床实验中,将两种细胞系固定在大孔Siran?载体中,均获得了良好的结果。在烧瓶培养中优化的培养基可以在固定床反应器中使用而无需任何进一步的调整。与搅拌反应器中的悬浮培养相比,固定化极大地提高了无血清培养基中非贴壁动物细胞培养的稳定性和可靠性。在所有三种培养基中,体积特异性葡萄糖摄取率(固定化细胞活性的指标)相似。固定和悬浮细胞代谢的偏差似乎主要是由于大孔载体内的氧气浓度低,在这种情况下,仅通过扩散为细胞提供氧气。

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