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可溶性哺乳动物细胞色素b5在大肠杆菌中的基因剂量依赖性表达。

Gene-dose-dependent expression of soluble mammalian cytochrome b5 in Escherichia coli.

作者信息

Gallagher J, Kaderbhai N, Kaderbhai M A

机构信息

Department of Biochemistry, School of Life Sciences, University College of Wales, Penglais, Aberystwyth, UK.

出版信息

Appl Microbiol Biotechnol. 1992 Oct;38(1):77-83. doi: 10.1007/BF00169423.

DOI:10.1007/BF00169423
PMID:1369012
Abstract

A synthetic structural gene encoding a mammalian cytochrome b5, carrying an optimised ribosomal binding sequence, was tandemly polymerised ranging from one (n = 1) to six (n = 6) gene copies. The gene, placed in p lambda-ncyt under the control of the lambda PL promoter, transcribed mono- to hexahomocistronic mRNA, expressing one to six copies of cytochrome b5. The expressed levels of cytochrome b5 in Escherichia coli p lambda-ncyt corresponded linearly with the gene dose when up to five copies were present; saturating build-up of the recombinant protein was reached at six gene copies. Cells bearing p lambda-6cyt produced 75 micrograms cytochrome b5/ml of unit optical density at 600 nm culture, constituting 55% of the soluble bacterial protein. The recombinant protein accumulated predominantly in a haem-deficient, apoform, together with lesser amounts of the holocytochrome b5. Whereas the overall expressed protein (apo and holo forms) was gene dose dependent, there was an inverse relationship between holocytochrome b5 production and gene dose. Incubation of the thermally induced bacterial lysates with exogenous haem a converted all of the soluble apocytochrome b5 into holocytochrome b5 that was spectrally indistinguishable with its native counterpart. Culture supplementation with the likely metabolic precursors of haem synthesis, 5-aminolevulinic acid, glycine/succinate or glutamate, significantly alleviated the protoporphyrin deficiency during hyperproduction of cytochrome b5 in E. coli.

摘要

一个编码哺乳动物细胞色素b5的合成结构基因,携带优化的核糖体结合序列,以串联方式聚合,基因拷贝数从1个(n = 1)到6个(n = 6)。该基因置于λPL启动子控制下的pλ-ncyt载体中,转录产生单顺反子至六顺反子的mRNA,表达1至6个拷贝的细胞色素b5。当存在多达5个拷贝时,大肠杆菌pλ-ncyt中细胞色素b5的表达水平与基因剂量呈线性关系;在6个基因拷贝时达到重组蛋白的饱和积累。携带pλ-6cyt的细胞在600 nm培养物的单位光密度下每毫升产生75微克细胞色素b5,占可溶性细菌蛋白的55%。重组蛋白主要以血红素缺陷的脱辅基形式积累,同时伴有少量的全细胞色素b5。虽然总的表达蛋白(脱辅基和全辅基形式)依赖于基因剂量,但全细胞色素b5的产生与基因剂量呈反比关系。将热诱导的细菌裂解物与外源性血红素a一起孵育,可将所有可溶性脱辅基细胞色素b5转化为全细胞色素b5,其光谱与天然对应物无法区分。用血红素合成的可能代谢前体5-氨基乙酰丙酸、甘氨酸/琥珀酸或谷氨酸补充培养,可显著缓解大肠杆菌中细胞色素b5过量产生期间的原卟啉缺乏。

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