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Recombinant production of cyanovirin-N, a potent human immunodeficiency virus inactivating protein derived from a cultured Cyanobacterium

机译:重组生产cyanovirin-N,一种有效的人免疫缺陷病毒灭活蛋白,来源于培养的蓝细菌

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摘要

Here we describe the recombinant production and purification of a novel anti-human immunodeficiency virus (HIV) protein, cyanovirin-N (CV-N), in Escherichia coli, Initial attempts to express CV-N using a vector containing an ompA signal peptide sequence resulted in production of an intractable mixture of the full-length (101 amino acid residue) protein and a truncated form lacking the first two N-terminal amino acids, The truncated protein was observed regardless of the host cell line, culture conditions, or induction time. These observations suggested that an as yet unidentified protease or peptidase was responsible for proteolytic cleavage between the second and third N-terminal amino acids of CV-N when presented as an ompA-CV-N fusion protein, When the ompA signal peptide sequence was replaced by a pelB signal peptide sequence, CV-N was produced in high yield as a single, homogeneous protein. This was confirmed by electrospray ionization mass spectrometry and N-terminal sequencing, This expression system provides a basis for large-scale production of clinical grade CV-N for further research and development as an anti-HIV microbicide. (C) 1998 Academic Press. [References: 8]
机译:在这里,我们描述了在大肠杆菌中重组生产和纯化的新型抗人免疫缺陷病毒(HIV)蛋白cyanovirin-N(CV-N),使用包含ompA信号肽序列的载体表达CV-N的初步尝试导致产生全长(101个氨基酸残基)蛋白质和缺少前两个N末端氨基酸的截短形式的顽固混合物,无论宿主细胞系,培养条件或诱导如何,均观察到截短的蛋白质时间。这些观察结果表明,当被替换为ompA-CV-N融合蛋白时,尚未鉴定的蛋白酶或肽酶负责CV-N的第二个和第三个N末端氨基酸之间的蛋白水解切割。通过pelB信号肽序列,CV-N以单一,均质的蛋白高产。这已通过电喷雾电离质谱和N端测序得到了证实。该表达系统为大规模生产临床级CV-N提供了基础,以作为抗HIV杀菌剂进行进一步的研究和开发。 (C)1998年学术出版社。 [参考:8]

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