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基于氧传质的摇瓶规模缩小,可应用于平行、非侵入性和时间分辨的 48 孔微量滴定板中氧传递速率的监测。

Scale-down of CHO cell cultivation from shake flasks based on oxygen mass transfer allows application of parallelized, non-invasive, and time-resolved monitoring of the oxygen transfer rate in 48-well microtiter plates.

机构信息

AVT - Biochemical Engineering, RWTH Aachen University, Aachen, Germany.

KTH Royal Institute of Technology, Department of Industrial Biotechnology, School of Engineering Sciences in Chemistry, Biotechnology and Health, Stockholm, Sweden.

出版信息

Biotechnol J. 2023 Nov;18(11):e2300053. doi: 10.1002/biot.202300053. Epub 2023 Jul 21.

Abstract

Cultivating Chinese hamster ovary (CHO) cells in microtiter plates (MTPs) with time-resolved monitoring of the oxygen transfer rate (OTR) is highly desirable to provide process insights at increased throughput. However, monitoring of the OTR in MTPs has not been demonstrated for CHO cells, yet. Hence, a CHO cultivation process was transferred from shake flasks to MTPs to enable monitoring of the OTR in each individual well of a 48-well MTP. For this, the cultivation of an industrially relevant, antibody-producing cell line was transferred from shake flask to MTP based on the volumetric oxygen mass transfer coefficient (k a). Culture behavior was well comparable (deviation of the final IgG titer less than 10%). Monitoring of the OTR in 48-well MTPs was then used to derive the cytotoxicity of dimethyl sulfoxide (DMSO) based on a dose-response curve in a single experiment using a second CHO cell line. Logistic fitting of the dose-response curve determined after 100 h was used to determine the DMSO concentration that resulted in a cytotoxicity of 50% (IC50). A DMSO concentration of 2.70% ± 0.25% was determined, which agrees with the IC50 previously determined in shake flasks (2.39% ± 0.1%). Non-invasive, parallelized, and time-resolved monitoring of the OTR of CHO cells in MTPs was demonstrated and offers excellent potential to speed up process development and assess cytotoxicity.

摘要

在微滴板(MTP)中培养中国仓鼠卵巢(CHO)细胞,并对氧传递率(OTR)进行时变监测,以提高通量,从而深入了解工艺,这是非常可取的。然而,目前尚未在 MTP 中监测 CHO 细胞的 OTR。因此,将 CHO 培养工艺从摇瓶转移到 MTP,以实现对 48 孔 MTP 中每个孔的 OTR 进行监测。为此,根据体积氧传质系数(k a),将一种具有工业相关性的、生产抗体的细胞系从摇瓶转移到 MTP 中进行培养。培养行为具有很好的可比性(最终 IgG 滴度的偏差小于 10%)。然后,使用第二种 CHO 细胞系,在单次实验中基于剂量-反应曲线,通过在 48 孔 MTP 中监测 OTR,来确定二甲基亚砜(DMSO)的细胞毒性。对 100 小时后得到的剂量-反应曲线进行逻辑拟合,以确定导致细胞毒性为 50%(IC50)的 DMSO 浓度。确定 DMSO 浓度为 2.70%±0.25%,与摇瓶中先前确定的 IC50(2.39%±0.1%)一致。证明了可以在 MTP 中对 CHO 细胞的 OTR 进行非侵入式、平行和时变监测,这为加快工艺开发和评估细胞毒性提供了巨大的潜力。

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