Human Furin is a Calcium-dependent Serine Endoprotease That Recognizes the Sequence Arg-X-X-Arg and Efficiently Cleaves Anthrax Toxin Protective Antigen

Overview

Journal J Biol Chem

Specialty Biochemistry

Date 1992 Aug 15

PMID 1644824

Citations 241

Authors

S S Molloy

P A Bresnahan

S H Leppla

K R Klimpel

G Thomas

Affiliations

Soon will be listed here.

Abstract

Previous work demonstrated that human furin is a predominantly Golgi membrane-localized endoprotease that can efficiently process precursor proteins at paired basic residues (-Lys-Arg- or -Arg-Arg-) in transfected cells. Anion-exchange chromatography of culture supernatant from cells expressing a soluble truncated form of human furin resulted in a greatly enriched preparation of the endoprotease (approximately 70% pure as determined by protein staining). Enzymatic studies show that furin is a calcium-dependent (K0.5 = 200 microM) serine endoprotease which has greater than 50% of maximal activity between pH 6.0 and 8.5. The inhibitor sensitivity of furin suggests that it is similar to, yet distinct from, other calcium-dependent proteases. Evidence that furin may require a P4 Arg in fluorogenic peptide substrates suggested that this enzyme might cleave the protective antigen (PA) component of anthrax toxin at the sequence -Arg-Lys-Lys-Arg-. Indeed, PA was cleaved by purified furin at the proposed consensus site (-Arg-X-Lys/Arg-Arg decreases-) at a rate (8 mumol/min/mg total protein) 400-fold higher than that observed with synthetic peptides. In addition, the processing of mutant PA molecules with altered cleavage sites suggests that furin-catalyzed endoproteolysis minimally requires an -Arg-X-X-Arg- recognition sequence for efficient cleavage. Together, these results support the hypothesis that furin processes protein precursors containing this cleavage site motif in the exocytic pathway and in addition, raises the possibility that the enzyme also cleaves extracellular substrates, including PA.

Citing Articles

Tumor-specific cytosol-penetrating antibodies for antigen- and TME-dependent intracellular cargo delivery.

Dombrowsky C, Geyer F, Zakharchuk D, Kolmar H Mol Ther Oncol. 2025; 33(1):200931.

PMID: 39895690 PMC: 11786873. DOI: 10.1016/j.omton.2024.200931.

Impaired SERCA2a phosphorylation causes diabetic cardiomyopathy through impinging on cardiac contractility and precursor protein processing.

Quan C, Zhu S, Wang R, Chen J, Chen Q, Li M Life Metab. 2025; 1(1):54-66.

PMID: 39872684 PMC: 11749685. DOI: 10.1093/lifemeta/loac013.

Chemigenetic Ca2+ indicators report elevated Ca2+ levels in endothelial Weibel-Palade bodies.

Terglane J, Mertes N, Weischer S, Zobel T, Johnsson K, Gerke V PLoS One. 2025; 20(1):e0316854.

PMID: 39869616 PMC: 11771901. DOI: 10.1371/journal.pone.0316854.

A PSA SNP associates with cellular function and clinical outcome in men with prostate cancer.

Srinivasan S, Kryza T, Bock N, Tse B, Sokolowski K, Janaththani P Nat Commun. 2024; 15(1):9587.

PMID: 39505858 PMC: 11541583. DOI: 10.1038/s41467-024-52472-6.

Human parainfluenza virus 3 field strains undergo extracellular fusion protein cleavage to activate entry.

Stearns K, Lampe G, Hanan R, Marcink T, Niewiesk S, Sternberg S mBio. 2024; 15(11):e0232724.

PMID: 39382296 PMC: 11559058. DOI: 10.1128/mbio.02327-24.