AI Article Synopsis

  • Dipeptidyl peptidase III (DPP III) contains a unique helix in its metal-binding region, which is crucial for enzyme activity.
  • Cu(II)-rat DPP III demonstrates reduced activity compared to its wild-type form, while a modified version with a deletion (del-DPP III) drastically loses its enzyme function.
  • The deletion of Leu453 disrupts the enzyme's flexibility around copper ions, affecting the formation of the enzyme-metal-substrate complex and altering the accessibility of a key residue (Glu451) to water.

Article Abstract

Dipeptidyl peptidase III (DPP III), the zinc peptidase, has a unique helix portion in the metal-binding motif (HELLGH). The enzyme activity of the cupric derivative of rat DPP III (Cu(II)-rat DPP III) for Lys-Ala-β-NA is about 30% of that of the wild-type enzyme. On the other hand, the enzyme activity of Cu(II)-rat del-DPP III, in which Leu453 is deleted from the metal-binding motif, possesses only 1-2% of the enzyme activity of rat del-DPP III. The EPR spectra of Cu(II)-rat DPP III in the presence of various concentrations of the substrate, Lys-Ala-β-NA, changed dramatically, showing formation of the enzyme-metal-substrate complex. The EPR spectra of Cu(II)-rat del-DPP III did not change in the presence of excess Lys-Ala-β-NA. The deletion of Leu453 from the HELLGH motif of rat DPP III leads to a complete loss of flexibility in the ligand geometry around the cupric ions. Under the formation of the enzyme-metal-substrate complex, Glu451 of Cu(II)-rat DPP III is sufficiently able to approach the water molecule via a very different orientation from that of the resting state; however, Glu451 of Cu(II)-rat del-DPP III is not able to access the water molecule.

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http://dx.doi.org/10.1016/j.abb.2012.05.018DOI Listing

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