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适用于高通量应用的全细胞细胞色素P450定量测定。

Quantitative whole-cell cytochrome P450 measurement suitable for high-throughput application.

作者信息

Johnston Wayne A, Huang Weiliang, De Voss James J, Hayes Martin A, Gillam Elizabeth M J

机构信息

Physiology and Pharmacology, School of Biomedical Sciences, University of Queensland, St Lucia, Brisbane, Australia.

出版信息

J Biomol Screen. 2008 Feb;13(2):135-41. doi: 10.1177/1087057107312780. Epub 2008 Jan 23.

Abstract

The recombinant expression of cytochrome P450 enzymes involved in drug metabolism is of interest to the pharmaceutical and biotechnological industries due to the versatile catalytic properties of these enzymes. Accurate quantification of cytochrome P450 enzymes expressed in bacterial culture generally depends on disruption and fractionation of cells to prepare membranes for spectral analysis. Although whole-cell methods for spectral determination have been reported, problems with poor reproducibility and low signal-to-noise ratio confound the use of such techniques where P450 hemoprotein expression levels are relatively low, such as in cultures of certain mammalian forms. In particular, interference from bacterial hemoproteins often obscures the P450 peak. In the current study, the combination of culture concentration, incubation under microaerobic conditions, and a modified method of baseline correction enabled reproducible quantification of cytochrome P450s in whole cells. This whole-cell method is well suited to high-throughput application, as large sets or libraries of enzymes can be expressed in parallel and relative expression levels measured without downstream cell processing.

摘要

由于细胞色素P450酶具有多种催化特性,参与药物代谢的细胞色素P450酶的重组表达受到制药和生物技术行业的关注。准确量化细菌培养物中表达的细胞色素P450酶通常依赖于细胞的破碎和分级分离,以制备用于光谱分析的膜。尽管已经报道了用于光谱测定的全细胞方法,但在细胞色素P450血红蛋白表达水平相对较低的情况下,如某些哺乳动物细胞培养物中,重现性差和信噪比低的问题使得这些技术的应用受到困扰。特别是,细菌血红蛋白的干扰常常会掩盖细胞色素P450的峰。在本研究中,培养物浓缩、微需氧条件下孵育以及改进的基线校正方法相结合,实现了全细胞中细胞色素P450的可重现定量。这种全细胞方法非常适合高通量应用,因为大量的酶集或文库可以并行表达,并且无需下游细胞处理即可测量相对表达水平。

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