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[生长抑素细菌合成中的基因工程]

[Genetic engineering in the bacterial synthesis of somatostatin].

作者信息

Karpova S K, Sazina E T, Bader L B, Sergienko O V, Khodun M L, Krivtsov V F, Lunin V G, Tikhonenko T I, Pankov Iu A

出版信息

Vestn Ross Akad Med Nauk. 1994(12):24-9.

PMID:7742653
Abstract

Series of recombinant plasmids for expression of the synthetic gene somatostatin-14 (SST) as a fusion protein were obtained. The somatostatin gene was fused to chloramphenicol acetyltransferase (cat) or its deleted variant genes. Both parts of the resultant fusion protein were joined through a Met residue. The hybrid gene was expressed under the control of the cat gene promoter (Pcat), the tryptophan operon promoter (Ptrp) or the promoter of bacteriophage T5 (PT5). These fusions gave insoluble polypeptide products amounting from 5-10% of the total cellular protein under constitutive biosynthetic conditions (Pcat) to 5-30% upon induction (Ptrp, PT5). A correlation between the efficiency of expression and the length of cat, the power of the promoter used and the absence or presence of transcription terminators, was studied. The scheme for SST isolation from bacterial cells was developed. SST was liberated from the fused polypeptide by treatment with cyanogen bromide and purified to homogenity by a combination of chromatographic steps: gel filtration, ion-exchange and rpHPLC. The renaturated recombinant SST showed specific biological and immunological activities and had 98% purity. The yield was 1 mg of the purified cyclic SST/1 culture of E.coli.

摘要

获得了一系列用于表达作为融合蛋白的合成生长抑素 - 14(SST)基因的重组质粒。生长抑素基因与氯霉素乙酰转移酶(cat)或其缺失变体基因融合。所得融合蛋白的两部分通过一个甲硫氨酸残基连接。杂合基因在cat基因启动子(Pcat)、色氨酸操纵子启动子(Ptrp)或噬菌体T5启动子(PT5)的控制下表达。在组成型生物合成条件下(Pcat),这些融合产生的不溶性多肽产物占总细胞蛋白的5 - 10%,诱导后(Ptrp,PT5)占5 - 30%。研究了表达效率与cat长度、所用启动子的强度以及转录终止子的有无之间的相关性。制定了从细菌细胞中分离SST的方案。通过用溴化氰处理从融合多肽中释放出SST,并通过凝胶过滤、离子交换和反相高效液相色谱等色谱步骤组合纯化至同质。复性后的重组SST显示出特定的生物学和免疫学活性,纯度为98%。产量为每1升大肠杆菌培养物产生1毫克纯化的环状SST。

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