Structural basis for the mechanisms of human presequence protease conformational switch and substrate recognition

Author:

Liang Wenguang G.,Wijaya Juwina,Wei HuiORCID,Noble Alex J.ORCID,Mancl Jordan M.,Mo Swansea,Lee DavidORCID,Lin King John V.,Pan ManORCID,Liu Chang,Koehler Carla M.,Zhao MingleiORCID,Potter Clinton S.,Carragher BridgetORCID,Li ShengORCID,Tang Wei-JenORCID

Abstract

AbstractPresequence protease (PreP), a 117 kDa mitochondrial M16C metalloprotease vital for mitochondrial proteostasis, degrades presequence peptides cleaved off from nuclear-encoded proteins and other aggregation-prone peptides, such as amyloid β (Aβ). PreP structures have only been determined in a closed conformation; thus, the mechanisms of substrate binding and selectivity remain elusive. Here, we leverage advanced vitrification techniques to overcome the preferential denaturation of one of two ~55 kDa homologous domains of PreP caused by air-water interface adsorption. Thereby, we elucidate cryoEM structures of three apo-PreP open states along with Aβ- and citrate synthase presequence-bound PreP at 3.3–4.6 Å resolution. Together with integrative biophysical and pharmacological approaches, these structures reveal the key stages of the PreP catalytic cycle and how the binding of substrates or PreP inhibitor drives a rigid body motion of the protein for substrate binding and catalysis. Together, our studies provide key mechanistic insights into M16C metalloproteases for future therapeutic innovations.

Funder

Simons Foundation

U.S. Department of Health & Human Services | National Institutes of Health

Publisher

Springer Science and Business Media LLC

Subject

General Physics and Astronomy,General Biochemistry, Genetics and Molecular Biology,General Chemistry,Multidisciplinary

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