Hydrolysis by Cathepsin B of Fluorescent Peptides Derived From Human Prorenin

Hydrolysis by Cathepsin B of Fluorescent Peptides Derived From Human Prorenin

Cathepsin B is a lysosomal thiolprotease that, because of its colocalization with renin and its ability to activate prorenin, has been proposed as a prorenin processing enzyme. To characterize the biochemical aspect of this potential cathepsin B activity in more detail, we synthesized and assayed wi...

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Bibliographic Details
Published in:Hypertension (Dallas, Tex. 1979) Vol. 35; no. 6; pp. 1278 - 1283
Main Authors: Almeida, Paulo Cezar, Oliveira, Vitor, Chagas, Jair Ribeiro, Meldal, Morten, Juliano, Maria Aparecida, Juliano, Luiz
Format: Journal Article
Language:English
Published: Philadelphia, PA American Heart Association, Inc 01-06-2000
Hagerstown, MD Lippincott
Subjects:
Animals
Biological and medical sciences
Cathepsin B - metabolism
Cells, Cultured
Endocrine kidney. Renin-angiotensin-aldosterone system
Enzyme Precursors - chemistry
Enzyme Precursors - metabolism
Fluorescence
Fundamental and applied biological sciences. Psychology
Glomerular Mesangium - cytology
Glomerular Mesangium - metabolism
Humans
Hydrolysis
Oligopeptides - metabolism
Peptide Fragments - metabolism
Protein Processing, Post-Translational
Rats
Rats, Wistar
Recombinant Proteins - metabolism
Renin - chemistry
Renin - metabolism
Vertebrates: endocrinology
Human
Rat
Enzyme
Mesangial cell
Cysteine endopeptidases
Rodentia
In vitro
Peptidases
Vertebrata
Specificity
Mammalia
Renin
Animal
Prorenin
Cathepsin B
Value
Hydrolases
Aspartic endopeptidases
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Summary:Cathepsin B is a lysosomal thiolprotease that, because of its colocalization with renin and its ability to activate prorenin, has been proposed as a prorenin processing enzyme. To characterize the biochemical aspect of this potential cathepsin B activity in more detail, we synthesized and assayed with human cathepsin B the internally quenched fluorescent peptide Abz-FSQPMKRLTLGNTTQ-EDDnp (Abz, ortho- aminobenzoic acid fluorescent group and EDDnp, N-[2,4-dinitrophenyl]-ethylenediamine quencher group) that contains 7 amino acids for each side of the R-L bond that is the processing site of human prorenin. Human cathepsin B hydrolyzed this peptide at the correct site (R-L bond), with kcat/Km=75 mmol/L s. Analogues of this peptide obtained by Ala scanning at positions P5 to P5’ were also synthesized and assayed as substrates for human cathepsin B. The obtained specificity constant (kcat/Km) values have a significant parallel with the previous data of prorenin activation by AtT-20 cells and in vitro by cathepsin B. In addition, we demonstrated the presence of cathepsin B–like activity in rat mesangial cells and the ability of its whole soluble fraction lysates, as well as that of purified cloned rat cathepsin B, to hydrolyze Abz-IKKSSF-EDDnp at the K-S bond, which contains 6 amino acids of rat prorenin processing site. The specificity data of cathepsin B toward peptides derived from prorenin processing site support the view that human or rodent cathepsin B could be involved in the intracellular processing of prorenin that is locally synthesized or taken up from the extracellular compartment.
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ISSN:0194-911X
1524-4563
DOI:10.1161/01.HYP.35.6.1278