首页> 外文期刊>Journal of Pharmaceutical and Biomedical Analysis: An International Journal on All Drug-Related Topics in Pharmaceutical, Biomedical and Clinical Analysis >Rapid quantification of tryptophan and tyrosine in chemically defined cell culture media using fluorescence spectroscopy
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Rapid quantification of tryptophan and tyrosine in chemically defined cell culture media using fluorescence spectroscopy

机译:使用荧光光谱法对化学定义的细胞培养基中的色氨酸和酪氨酸进行快速定量

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摘要

The rapid and inexpensive analysis of the complex cell culture media used in industrial mammalian cell culture is required for quality and variance monitoring. Excitation-emission matrix (EEM) spectroscopy combined with multi-way chemometrics is a robust methodology applicable for the analysis of raw materials, media, and bioprocess broths. We have shown that the methodology can identify compositional changes and predict the efficacy of media in terms of downstream titer [1]. Here we describe how to extend the measurement methodology for the quantification of tryptophan (Trp), tyrosine (Tyr) in complex chemically defined media. The sample type is an enriched basal RDF medium in which five significant fluorophores were identified: Trp, Tyr, pyridoxine, folic acid, and riboflavin. The relatively high chromophore concentrations and compositional complexity lead to very significant matrix effects which were assessed using PARAllel FACtor analysis2 (PARAFAC2). Taking these effects into account, N-way partial least squares (NPLS) combined with a modified standard addition method was used to build calibration models capable of quantifying Trp and Tyr with errors of ~4.5 and 5.5% respectively. This demonstrates the feasibility of using the EEM method for the rapid, quantitative analysis of Trp and Tyr in complex cell culture media with minimal sample handling as an alternative to chromatographic based methods.
机译:需要对工业哺乳动物细胞培养中使用的复杂细胞培养基进行快速而廉价的分析,以进行质量和方差监测。激发-发射矩阵(EEM)光谱与多路化学计量学相结合是一种可靠的方法,适用于分析原材料,培养基和生物工艺肉汤。我们已经表明,该方法学可以识别组成变化并根据下游滴度[1]预测培养基的功效。在这里,我们描述了如何扩展在复杂的化学定义介质中定量色氨酸(Trp),酪氨酸(Tyr)的测量方法。样品类型是一种富集的基础RDF培养基,其中鉴定了五个重要的荧光团:Trp,Tyr,吡ido醇,叶酸和核黄素。较高的生色团浓度和组成复杂性会导致非常显着的基质效应,可使用PARAllel FACtor分析2(PARAFAC2)对其进行评估。考虑到这些影响,使用N向偏最小二乘(NPLS)结合改进的标准加法建立了能够量化Trp和Tyr的校正模型,其误差分别约为4.5%和5.5%。这证明了使用EEM方法对复杂细胞培养基中的Trp和Tyr进行快速,定量分析的可行性,并且只需最少的样品处理即可替代基于色谱的方法。

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