Browsing by Author "Chuchana, P."
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- Cloning and expression in Escherichia coli of full-length complementary DNA coding for human α1-antitrypsinPublication . Bollen, A.; Herzog, A.; Cravador, A.; Hérion, P.; Chuchana, P.; Vander Straten, A.; Loriau, R.; Jacobs, P.; Van Elsen, A.A cDNA library prepared from human liver was screened for α₁-antitrypsin, a major constituent of plasma which functions as inhibitor of proteolytic enzyms. The library was screened using a 12-base-long synthetic oligodeoxyribonucleotide corresponding to a known DNA fragment of human α₁-antitrypsin and by hybrid-selection of α₁-antitrypsin mRNA.
- Molecular cloning, sequencing, and expression in Escherichia coli of human preprourokinase cDNAPublication . Jacobs, P.; Cravador, A.; Loriau, R.; Brockly, F.; Colau, B.; Chuchana, P.; Van Elsen, A.; Herzog, A.; Bollen, A.A cDNA library derived from human carcinoma cells was used to isolate a clone, pULB1000, coding for the preproenzyme form of human urokinase. This clone carries the full-length sequence coding for the signal peptide and for the A chain (157 amino acids) and B chain (253 amino acids) of urokinase in tandem. The sequence of the cDNA predicts the presence of a single lysine residue between the last amino acid of the mature A polypeptide (Phe-157) and the first amino acid of the mature B polypeptide (Ile-1). The amino acid sequence deduced from the cDNA sequence fits the published amino acid sequence data with three exceptions, the reported cysteine residue at position 131 in the A chain is a tryptophan, and glycine 366 and alanine 410 in the B chain are, respectively, a cysteine and a valine in our clone. A large Bgl I fragment (1482 bp), derived from the clone pULB1000 coding for most of the signal peptide and for the A and B chains, has been subcloned into the expression vector pCQV2. Heat induction of E. coli cells carrying the recombinant plasmid leads to the production of urokinase-like polypeptides having the expected molecular weights and being specifically recognized by antibodies raised against natural human urokinase.