EMD-7062
Cryo-EM structure of human insulin degrading enzyme in complex with insulin
EMD-7062
Single-particle3.7 Å
Deposition: 03/10/2017Map released: 27/12/2017
Last modified: 13/11/2024
Sample Organism:
Homo sapiens
Sample: Insulin degrading enzyme/Insulin
Fitted models: 6b70 (Avg. Q-score: 0.374)
Deposition Authors: Zhang Z, Liang WG, Bailey LJ, Tan YZ
,
Wei H,
Kossiakoff AA,
Carragher B ,
Potter SC,
Tang WJ
Sample: Insulin degrading enzyme/Insulin
Fitted models: 6b70 (Avg. Q-score: 0.374)
Deposition Authors: Zhang Z, Liang WG, Bailey LJ, Tan YZ
,
Wei H,
Kossiakoff AA,
Carragher B ,
Potter SC,
Tang WJ
Ensemble cryoEM elucidates the mechanism of insulin capture and degradation by human insulin degrading enzyme.
Zhang Z,
Liang WG,
Bailey LJ,
Tan YZ ,
Wei H,
Wang A,
Farcasanu M,
Woods VA,
McCord LA,
Lee D ,
Shang W,
Deprez-Poulain R ,
Deprez B,
Liu DR,
Koide A,
Koide S,
Kossiakoff AA,
Li S,
Carragher B ,
Potter CS ,
Tang WJ
(2018) eLife , 7
,
Wei H,
Wang A,
Farcasanu M,
Woods VA,
McCord LA,
Lee D ,
Shang W,
Deprez-Poulain R ,
Deprez B,
Liu DR,
Koide A,
Koide S,
Kossiakoff AA,
Li S,
Carragher B ,
Potter CS ,
Tang WJ
(2018) eLife , 7
Abstract:
Insulin degrading enzyme (IDE) plays key roles in degrading peptides vital in type two diabetes, Alzheimer's, inflammation, and other human diseases. However, the process through which IDE recognizes peptides that tend to form amyloid fibrils remained unsolved. We used cryoEM to understand both the apo- and insulin-bound dimeric IDE states, revealing that IDE displays a large opening between the homologous ~55 kDa N- and C-terminal halves to allow selective substrate capture based on size and charge complementarity. We also used cryoEM, X-ray crystallography, SAXS, and HDX-MS to elucidate the molecular basis of how amyloidogenic peptides stabilize the disordered IDE catalytic cleft, thereby inducing selective degradation by substrate-assisted catalysis. Furthermore, our insulin-bound IDE structures explain how IDE processively degrades insulin by stochastically cutting either chain without breaking disulfide bonds. Together, our studies provide a mechanism for how IDE selectively degrades amyloidogenic peptides and offers structural insights for developing IDE-based therapies.
Insulin degrading enzyme (IDE) plays key roles in degrading peptides vital in type two diabetes, Alzheimer's, inflammation, and other human diseases. However, the process through which IDE recognizes peptides that tend to form amyloid fibrils remained unsolved. We used cryoEM to understand both the apo- and insulin-bound dimeric IDE states, revealing that IDE displays a large opening between the homologous ~55 kDa N- and C-terminal halves to allow selective substrate capture based on size and charge complementarity. We also used cryoEM, X-ray crystallography, SAXS, and HDX-MS to elucidate the molecular basis of how amyloidogenic peptides stabilize the disordered IDE catalytic cleft, thereby inducing selective degradation by substrate-assisted catalysis. Furthermore, our insulin-bound IDE structures explain how IDE processively degrades insulin by stochastically cutting either chain without breaking disulfide bonds. Together, our studies provide a mechanism for how IDE selectively degrades amyloidogenic peptides and offers structural insights for developing IDE-based therapies.