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[编码胸腺素α1的人工基因的合成及其在大肠杆菌中与人肿瘤坏死因子杂交的表达]

[Synthesis of an artificial gene coding for thymosin alpha1 and its expression in Escherichia coli as a hybrid with human tumor necrosis factor].

作者信息

Korobko V G, Boldyreva E F, Filippov S A, Berkova N P, Dobrynin V N, Shmelev V A, Popov S G, Evsegneev S I, Nosova L Iu

出版信息

Bioorg Khim. 1992 May;18(5):646-59.

PMID:1417992
Abstract

Chemical-enzymatic synthesis and cloning in Escherichia coli of an artificial gene encoding the immunoactive peptide thymosin alpha 1 have been carried out. Recombinant plasmids were constructed which contain fusion genes coding for hybrids of human tumour necrosis factor (TNF) and thymosin alpha 1 as N- or C-terminal part of the hybrid protein. In the C-terminal hybrid protein, TNF and thymosin alpha 1 are linked through a methionine residue, thus allowing for thymosin alpha 1 to be cleaved off the rest of the hybrid protein with cyanogen bromide. In case of the N-terminal hybrid protein, the linker between the thymosin alpha 1 and TNF sequences is the acid-labile dipeptide Asp-Pro. Expression of the hybrid genes in E. coli and properties of the recombinant proteins were studied. The N-terminal hybrid protein was secreted into periplasmic space, in contrast with the C-terminal hybrid protein, which formed insoluble aggregates inside bacterial cells. Procedures for the isolation of both hybrid proteins were developed. The N-terminal hybrid protein displayed full biological activity in the cytotoxic assay on the mouse fibroblast L-929 whereas the C-terminal hybrid protein proved to be much less active. Treatment of the hybrid protein TNF-thymosin alpha 1 with cyanogen bromide lead to a mixture of two polypeptides, from which thymosin alpha 1 was purified to homogeneity by simple chromatographic procedures.

摘要

已进行了编码免疫活性肽胸腺素α1的人工基因在大肠杆菌中的化学酶促合成及克隆。构建了重组质粒,其包含编码人肿瘤坏死因子(TNF)与胸腺素α1的杂种的融合基因,作为杂种蛋白的N端或C端部分。在C端杂种蛋白中,TNF和胸腺素α1通过甲硫氨酸残基相连,从而使得胸腺素α1能用溴化氰从杂种蛋白的其余部分切割下来。对于N端杂种蛋白,胸腺素α1与TNF序列之间的连接子是酸不稳定二肽天冬氨酸-脯氨酸。研究了杂种基因在大肠杆菌中的表达及重组蛋白的性质。与形成不溶性聚集体的C端杂种蛋白相反,N端杂种蛋白分泌到周质空间中。开发了两种杂种蛋白的分离方法。N端杂种蛋白在对小鼠成纤维细胞L-929的细胞毒性测定中显示出完全的生物学活性,而C端杂种蛋白的活性则低得多。用溴化氰处理杂种蛋白TNF-胸腺素α1产生两种多肽的混合物,通过简单的色谱方法将胸腺素α1纯化至同质。

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