白细胞介素-2对大肠杆菌外周质的靶向作用。

G Halfmann, H Brailly, A Bernadac, F A Montero-Julian, C Lazdunski, D Baty
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引用次数: 17

摘要

利用合成的白介素-2 (IL-2)编码基因在大肠杆菌中产生大量重组IL-2 (met-IL-2)。发现Met-IL-2以不溶性聚集形式积聚在细胞质中。利用免疫金标记法检测位于细胞极帽的包涵体。构建的目的是将IL-2基因融合到大肠杆菌外膜蛋白(OmpA)或外质蛋白(PhoA)的编码信号肽的DNA片段上。这些融合蛋白在细胞质中以不溶性形式存在,未观察到明显的成熟。通过用谷氨酸取代带正电的氨基酸,研究了蛋白质成熟部分n端电荷配置的影响。引入的替代都没有任何效果。检测可能影响表达、分泌和折叠的各种因素,试图获得分泌。通过将IL-2与前体麦芽糖结合蛋白(preMBP)融合,大部分preMBP-IL-2蛋白被正确加工并运输到质周空间。FXa切割后由MBP-IL-2衍生的IL-2与中国仓鼠卵巢细胞中产生的重组IL-2具有相似的特异性活性。
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Targeting of interleukin-2 to the periplasm of Escherichia coli.

A synthetic gene coding for interleukin-2 (IL-2) was used to produce large amounts of recombinant IL-2 (met-IL-2) in Escherichia coli. Met-IL-2 was found to accumulate in the cytoplasm in an insoluble, aggregated form. Inclusion bodies located at the pole caps of cells were detected using immunogold labelling. Constructs were designed to fuse the IL-2 gene to DNA fragments encoding signal peptides for an outer-membrane protein (OmpA) or for a periplasmic protein (PhoA) of E. coli. No significant maturation was observed with these fusion proteins which were found in an insoluble form in the cytoplasm. The influence of charge disposition at the N-terminus of the mature portion of the protein was investigated by replacing positively charged amino acids with glutamic acid. None of the introduced substitutions had any effect. Various factors that might affect expression, secretion and folding were examined in an attempt to obtain secretion. By fusing IL-2 to the precursor maltose-binding protein (preMBP) a large fraction of the preMBP-IL-2 protein was correctly processed and transported to the periplasmic space. IL-2 derived from MBP-IL-2 after FXa cleavage possessed similar specific activity to recombinant IL-2 produced in Chinese Hamster ovary cells.

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