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通过对二氢叶酸还原酶阳性转化体进行单次筛选来生成重组中国仓鼠卵巢(二氢叶酸还原酶缺陷型)细胞系。

Generation of recombinant CHO(dhfr-) cell lines by single selection for dhfr+ transformants.

作者信息

Wernicke D, Will H

机构信息

Central Institute of Molecular Biology, Berlin-Buch, Germany.

出版信息

Anal Biochem. 1992 May 15;203(1):146-50. doi: 10.1016/0003-2697(92)90055-c.

Abstract

In order to establish a mammalian cell expression system with a minimum of selection steps and a stable expression of microgram amounts of recombinant protein (human tissue-type plasminogen activator mutants and chimeric proteins) per 10(6) cells per day, we investigated Chinese hamster ovary cells and the dihydrofolate reductase-deficient Chinese hamster ovary cell line CHO(dhfr-). The 1tPA expression vector pCMVtPA was cotransfected either with the SV40 enhancer sequence containing dhfr expression vector pMT2 or with the enhancerless dhfr expression vector pAdD26SV(A) into CHO(dhfr-) cells. With both dhfr expression plasmids, selection for dhfr+ transformants followed by single dilution cloning was sufficient to generate cell lines with a production level of up to 4.6 micrograms tPA/10(6) cells.day. This approach is useful if gene amplification procedures are time-consuming and impracticable because of a large number of recombinant proteins. In order to establish CHO cell lines with a tPA expression level as high as that in the case of CHO(dhfr-) cells, repeated dilution cloning is necessary.

摘要

为了建立一个只需最少筛选步骤且能稳定表达重组蛋白(人组织型纤溶酶原激活剂突变体和嵌合蛋白)的哺乳动物细胞表达系统,每天每10⁶个细胞能表达微克量的重组蛋白,我们研究了中国仓鼠卵巢细胞及二氢叶酸还原酶缺陷型中国仓鼠卵巢细胞系CHO(dhfr⁻)。将1tPA表达载体pCMVtPA与含有dhfr表达载体pMT2的SV40增强子序列或与无增强子的dhfr表达载体pAdD26SV(A)共转染到CHO(dhfr⁻)细胞中。使用这两种dhfr表达质粒,对dhfr⁺转化体进行筛选,随后进行单倍稀释克隆,足以产生产量高达4.6微克tPA/10⁶细胞·天的细胞系。如果由于大量重组蛋白导致基因扩增程序耗时且不可行,这种方法是有用的。为了建立tPA表达水平与CHO(dhfr⁻)细胞情况一样高的CHO细胞系,重复稀释克隆是必要的。

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