Structure
The structure of IDE is a monomer with two N-terminal domains, which forms the catalytic site and two C-terminal domains that facilitates the substrate binding. The N-terminal domains are connected to the C-terminal domains via a 28-residue loop that forms a chamber that is shaped like a triangular prism.
Domain 1 houses the active site with two histidine's (his 108 and his 112), one glutamate (Glu 189) and the Zn2+ ion cofactor. Several residues of domains 1 & 4 create a polar area of the triangular cavity, while residues of domains 2 & 3 create a nonpolar region of the cavity.
In the open conformation, the insulin protein enters the enzyme opening causing a conformational change that allows the enzyme to fully recognize the protein and catalyzes protein degradation.
Function
Once the insulin molecule enters the active site and is recognized, the enzyme changes conformation from the open state to the closed state and begins to unfold the insulin and makes initial cleavages in the middle of both the A and B chains. The enzyme then makes six more cleavages. One cleavage site right next to the first one on the A chain and 5 more on the B chain [5]. Three near the middle and two near the C-terminus. There are no cleavage sites that are near the N-terminus of either chain.
Disease
• Mutation of Glu-111 causes the enzyme to become inactive
• Mutation of Pro-286 reduces the activity of the enzyme
• Three mutations, when combined with mutations from another site causes an increase of enzyme activity for the breakdown of insulin and amyloids
1. Ser-132 & Glu-817
2. Asn-184 & Gln-828
3. Asp-426 & Lys-899
Hyperproinsulinemia – Asp 34 mutation and/or His-89
Insulin-dependent diabetes – Cys-55
Permanent neonatal diabetes - ASP-24; ARG-32; SER-32; GLY-43; VAL-47; CYS-48; CYS-89; CYS- 90; TYR-96 AND CYS-108.
Alzheimer’s - Ile-714
Relevance
Structural highlights
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