Dns-Gly-(p-NO2)Phe-βAla, a Specific Fluorogenic Substrate for Neutral Endopeptidase 24.11

A novel fluorogenic peptide, dansyl-Gly- (\left(p-\mathrm{NO}{2}\right)) Phe- (\boldsymbol{\beta A l a}) (DGNPA), was synthesized as a selective substrate for neutral endopeptidase 24.11 , an enzyme involved in enkephalin and atrial natriuretic peptide degradation and a marker of differentiation (CD10) on the surface of lymphohematopoietic cells. Cleavage of the substrate (\mathrm{Gly}-\left(\mathrm{p}-\mathrm{NO}{2}\right)) Phe amide bond leads to an increase in fluorescence related to the disappearance of the intramolecular quenching of the dansyl fluorescence by the nitrophenyl residue. This new fluorogenic substrate is an improvement over the commercially available dansyl-p-Ala-Gly- (\left(p-\mathrm{NO}{2}\right)) Phe-Gly, as the Gly ({ }^{4}) residue of the latter has been replaced by a (\beta)-alanine, therefore eliminating a residual sensitivity of the peptide toward angiotensin converting enzyme. Moreover, deletion of the (\mathrm{D}-\mathrm{Ala}^{2}) residue was shown to increase the quenching efficiency, thus raising the sensitivity of the assay, which was further improved by stopping the reaction with dioxane. The present substrate has improved affinity (\left(K{\mathrm{m}}=37 \mu \mathrm{M}, \mathrm{V}=0.72 \mu \mathrm{mol}\right.) (\min ^{-1} \mathrm{mg}^{2}) protein (\left.{ }^{-1}\right)), selectivity, and sensitivity over its precursor and was used in automated assays using 96 -well microplates and a fluorescence plate reader. (c) 1894 Academic Press, Inc.