Structure, interdomain dynamics, and pH-dependent autoactivation of pro-rhodesain, the main lysosomal cysteine protease from African trypanosomes

6533b871fe1ef96bd12d26ed

RESEARCH PRODUCT

Structure, interdomain dynamics, and pH-dependent autoactivation of pro-rhodesain, the main lysosomal cysteine protease from African trypanosomes

Tanja Schirmeister Patrick Johe Christian Kersten Hannes Neuweiler Elmar Jaenicke Ute A. Hellmich Ute A. Hellmich

subject

Models Molecular Trypanosoma brucei rhodesiense 0301 basic medicine medicine.medical_treatment Biochemistry cysteine protease proenzyme fluorescence correlation spectroscopy (FCS)Trypanosoma brucei BBB blood–brain barrier CD circular dichroism chemistry.chemical_classification Enzyme Precursors biology Chemistry hsCathL human cathepsin L Hydrogen-Ion Concentration Cysteine protease FCS fluorescence correlation spectroscopy Cysteine Endopeptidases Biochemistry HAT Human African Trypanosomiasis NTD neglected tropical disease Research Article crystal structure Proteases SEC size-exclusion chromatography PET-FCS photoinduced electron transfer–fluorescence correlation spectroscopy African Sleeping Sickness Trypanosoma brucei Cleavage (embryo)03 medical and health sciences TbCathB T. brucei cathepsin B Protein Domains Zymogen medicine Molecular Biology zymogen rhodesain Cathepsin Protease 030102 biochemistry & molecular biology Active site Trypanosoma brucei rhodesiense Cell Biology biology.organism_classification molecular dynamics Enzyme Activation Enzyme 030104 developmental biology biology.protein autoinhibition Heterologous expression

description

AbstractRhodesain is the lysosomal cathepsin L-like cysteine protease ofT. brucei rhodesiense, the causative agent of Human African Trypanosomiasis. The enzyme is essential for the proliferation and pathogenicity of the parasite as well as its ability to overcome the blood-brain barrier of the host. Lysosomal cathepsins are expressed as zymogens with an inactivating pro-domain that is cleaved under acidic conditions. A structure of the uncleaved maturation intermediate from a trypanosomal cathepsin L-like protease is currently not available. We thus established the heterologous expression ofT. brucei rhodesiensepro-rhodesain inE. coliand determined its crystal structure. The trypanosomal pro-domain differs from non-parasitic pro-cathepsins by a unique, extended α-helix that blocks the active site and whose interactions resemble that of the antiprotozoal inhibitor K11777. Interdomain dynamics between pro- and core protease domain as observed by photoinduced electron transfer fluorescence correlation spectroscopy increase at low pH, where pro-rhodesain also undergoes autocleavage. Using the crystal structure, molecular dynamics simulations and mutagenesis, we identify a conserved interdomain salt bridge that prevents premature intramolecular cleavage at higher pH values and may thus present a control switch for the observed pH-sensitivity of pro-enzyme cleavage in (trypanosomal) CathL-like proteases.

year	journal	country	edition	language
2021-03-01	Journal of Biological Chemistry

https://doi.org/10.1016/j.jbc.2021.100565