Onderwater R C, Goeptar A R, Levering P R, Vos R M, Konings P N, Doehmer J, Commandeur J N, Vermeulen N P
Division of Molecular Toxicology, Leiden/Amsterdam Center for Drug Research (LACDR), Vrije Universiteit, The Netherlands.
Protein Expr Purif. 1996 Dec;8(4):439-46. doi: 10.1006/prep.1996.0122.
In this study, macroporous microcarriers were used for the large-scale growth of parental V79 cells and V79 cells genetically engineered to express a single human cytochrome P4501A1 isoenzyme (V79h1A1). Starting from 2 x 10(5) cells/ml, approximately 1 x 10(7) cells/ml could easily be harvested after 6 days in the case of the V79h1A1 cells, resulting in a total of 3.6 x 10(10) cells. For the first time, the presence of cytochrome P450 (CYP) in the expressed V79 cells could be demonstrated by CO difference spectra with a Soret maximum around 450 nm. CYP levels in microsomes derived from the V79h1A1 cells of 14 pmol/mg protein were achieved. Importantly, no CYP was detected in microsomal fractions of the parental V79 cells. Cytochrome b5 levels could also be measured by difference spectrophotometry. No significant differences were found between cytochrome b5 levels in microsomes derived from the large-scale growth of V79h1A1 cells and parental V79 cells, i.e., 16.7 +/- 7.9 vs 14.5 +/- 7.6 pmol/mg protein. The presence of human cytochrome P4501A1 (CYPh1A1) in microsomal fractions derived from the large-scale growth of V79h1A1 cells was further substantiated by measuring 7-ethoxyresorufin-O-deethylase (EROD), 7-ethoxycoumarin-O-dealkylase (ECOD), and testosterone-6 beta-hydroxylation activities. EROD, ECOD, and testosterone-6 beta-hydroxylation activities of the V79h1A1 microsomes were 40 pmol resorufin/min/pmol CYPh1A1, 13 pmol hydroxy-coumarin/min/pmol CYPh1A1, and 0.16 pmol 6 beta-hydroxytestosterone/min/pmol CYPh1A1, respectively, indicating the presence of a highly active human CYP1A1 enzyme system. Further confirmation that the CYP protein was correctly expressed was obtained by Western blotting. In conclusion, the use of macroporous microcarriers is suitable for large-scale growth of V79 cells expressing human CYP isoenzymes. The present method may provide an easy and rather inexpensive tool in obtaining large quantities of microsomes containing human CYP isoenzymes, which are involved in the bioactivation and bioinactivation of xenobiotics. High yields of microsomes containing human CYP isoenzymes may substantially facilitate the production of sufficient quantities of human metabolites to allow isolation and identification in an early stage of development of pharmacologically interesting drugs.
在本研究中,大孔微载体用于亲代V79细胞以及经基因工程改造以表达单一人类细胞色素P4501A1同工酶的V79细胞(V79h1A1)的大规模培养。对于V79h1A1细胞,从2×10⁵个细胞/毫升开始培养,6天后可轻松收获约1×10⁷个细胞/毫升,总共得到3.6×10¹⁰个细胞。首次通过一氧化碳差光谱法在表达的V79细胞中证实了细胞色素P450(CYP)的存在,其Soret峰最大值约在450纳米处。源自V79h1A1细胞的微粒体中CYP水平达到14皮摩尔/毫克蛋白质。重要的是,在亲代V79细胞的微粒体组分中未检测到CYP。细胞色素b5水平也可通过差示分光光度法测量。源自V79h1A1细胞大规模培养的微粒体与亲代V79细胞的微粒体中细胞色素b5水平之间未发现显著差异,即分别为16.7±7.9和14.5±7.6皮摩尔/毫克蛋白质。通过测量7 - 乙氧基试卤灵 - O - 脱乙基酶(EROD)、7 - 乙氧基香豆素 - O - 脱烷基酶(ECOD)和睾酮 - 6β - 羟基化活性,进一步证实了源自V79h1A1细胞大规模培养的微粒体组分中存在人类细胞色素P4501A1(CYPh1A1)。V79h1A1微粒体的EROD、ECOD和睾酮 - 6β - 羟基化活性分别为40皮摩尔试卤灵/分钟/皮摩尔CYPh1A1、13皮摩尔羟基香豆素/分钟/皮摩尔CYPh1A1和0.16皮摩尔6β - 羟基睾酮/分钟/皮摩尔CYPh1A1,表明存在高度活跃的人类CYP1A1酶系统。通过蛋白质免疫印迹法进一步证实了CYP蛋白的正确表达。总之,大孔微载体的使用适用于表达人类CYP同工酶的V79细胞的大规模培养。本方法可能为获得大量含有参与异生物素生物活化和生物失活的人类CYP同工酶的微粒体提供一种简便且相对廉价的工具。含有人类CYP同工酶的微粒体的高产率可能极大地促进足够量人类代谢物的产生,以便在具有药理活性的药物开发早期进行分离和鉴定。
