Cleavage site analysis of a serralysin‐like protease, PrtA, from an insect pathogen Photorhabdus luminescens and development of a highly sensitive and specific substrate

The aim of this study was the development of a sensitive and specific substrate for protease A (PrtA), a serralysin‐like metzincin from the entomopathogenic microorganism, Photorhabdus. First, cleavage of three biological peptides, the A and B chains of insulin and β‐lipotropin, and of 15 synthetic...

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Published in:The FEBS journal 2007-04, Vol.274 (8), p.1946-1956
Main Authors: Marokházi, Judit, Mihala, Nikolett, Hudecz, Ferenc, Fodor, András, Gráf, László, Venekei, István
Format: Article
Language:English
Subjects:
Amino Acid Sequence
Amino acids
Animals
Biochemistry
cleavage site
Insects
Metalloendopeptidases - chemistry
Metalloendopeptidases - metabolism
metalloprotease
Moths - microbiology
Peptides
Photorhabdus
Photorhabdus - enzymology
Photorhabdus luminescens
Proteases
PrtA of Photorhabdus
serralysin
specific substrate
Substrate Specificity
Substrates
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Summary:The aim of this study was the development of a sensitive and specific substrate for protease A (PrtA), a serralysin‐like metzincin from the entomopathogenic microorganism, Photorhabdus. First, cleavage of three biological peptides, the A and B chains of insulin and β‐lipotropin, and of 15 synthetic peptides, was investigated. In the biological peptides, a preference for the hydrophobic residues Ala, Leu and Val was observed at three substrate positions, P2, P1′ and P2′. At these positions in the synthetic peptides the preferred residues were Val, Ala and Val, respectively. They contributed to the efficiency of hydrolysis in the order P1′ > P2 > P2′. Six amino acids of the synthetic peptides were sufficient to reach the maximum rate of hydrolysis, in accordance with the ability of PrtA to cleave three amino acids from both the N‐ and the C‐terminus of some fragments of biological peptides. Using the best synthetic peptide, a fluorescence‐quenched substrate, N‐(4‐[4′(dimethylamino)phenylazo]benzoyl–EVYAVES−5‐[(2‐aminoethyl)amino]naphthalene‐1‐sulfonic acid, was prepared. The ∼ 4 × 106 m−1·s−1 specificity constant of PrtA (at Km ∼ 5 × 10−5 m and kcat ∼ 2 × 102 s−1) on this substrate was the highest activity for a serralysin‐type enzyme, allowing precise measurement of the effects of several inhibitors and pH on PrtA activity. These showed the characteristics of a metalloenzyme and a wide range of optimum pH, similar to other serralysins. PrtA activity could be measured in biological samples (Photorhabdus‐infected insect larvae) without interference from other enzymes, which indicates that substrate selectivity is high towards PrtA. The substrate sensitivity allowed early (14 h post infection) detection of PrtA, which might indicate PrtA's participation in the establishment of infection and not only, as it has been supposed, in bioconversion.
ISSN:1742-464X
1742-4658
DOI:10.1111/j.1742-4658.2007.05739.x