Nucleotide sequence of the neutral protease gene (nprL) from Lactobacillus sp. and characterization of the enzyme

Autor: Masahiro Takagi, Tadayuki Imanaka, Takuya Maeda, Shigeru Kawano
Rok vydání: 1994
Předmět:
Zdroj: Journal of Fermentation and Bioengineering. 77:339-346
ISSN: 0922-338X
Popis: The neutral protease gene (nprL) from Lactobacillus sp. no. 1 was cloned and sequenced. Cloning was performed with Bacillus subtilis DB104 [his nprR2 nprE18 ΔaprA3] as a host and pISA ts412 as a vector plasmid. The protease-productive clone harbored a plasmid with a 4.5 kb fragment insert. Nucleotide sequencing revealed that the nprL gene was composed of 1,698 bases (566 amino acids, M.W. 60,961 Da). However, the molecular weight of the purified extracellular NprL was 37,000 by SDS-PAGE. The amino acid sequence of the first 9 residues of the purified protease completely matched that deduced from the DNA sequence starting from GTA (Val), 747 bases (249 amino acids) downstream from the initiation codon, ATG. These results indicated that NprL was initially translated as a pre-pro structure. NprL could not degrade gramicidin S, unlike the previously reported protease from the same strain. The optimal temperature and pH for NprL activity were 60°C and 8.0, respectively. About 70% of the activity was retained after treatment at 60°C for 30 min. The protease activity was inhibited by EDTA, but not by phenylmethylsulfonyl fluoride (PMSF). The amino acid sequence of the secreted form of the neutral protease (317 amino acids) was homologous to the neutral protease from Bacillus cereus (95%) and thermolysin (72%). Accordingly, NprL was suggested to be a kind of metal-chelator-sensitive neutral protease. Analyses of hydrolysates of oxidized insulin A and B chains and of synthetic dipeptides by NprL revealed that the protease preferentially cleaves the peptide bonds at the amino side of bulky and/or hydrophobic residues such as Leu and Phe, in a similar but more limited fashion to that of thermolysin.
Databáze: OpenAIRE
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