Bioconjugate chemistry, 1993-11, Vol.4 (6), p.537-544
1993
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- Autor(en) / Beteiligte
- Titel
- Site-directed double fluorescent tagging of human renin and collagenase (MMP-1) substrate peptides using the periodate oxidation of N-terminal serine. An apparently general strategy for provision of energy-transfer substrates for proteases
- Ist Teil von
- Bioconjugate chemistry, 1993-11, Vol.4 (6), p.537-544
- Ort / Verlag
- Washington, DC: American Chemical Society
- Erscheinungsjahr
- 1993
- Quelle
- MEDLINE
- Beschreibungen/Notizen
- Periodate in neutral aqueous solution rapidly converts N-terminal Ser or Thr to an alpha-N-glyoxylyl moiety that can serve as the locus for incorporation of a modifying group [Geoghegan, K. F., and Stroh, J. G. (1992) Bioconjugate Chem. 3, 138-146. Gaertner, H. F. et al. (1992) Bioconjugate Chem. 3, 262-268]. The usefulness of this procedure has been further illuminated in a route to "energy-transfer" substrates for endoproteases. Each such substrate is an oligopeptide cleavable by a proteinase, but modified (usually at its termini) with two chromophores that form an energy donor-acceptor pair. Production of these substrates is an exercise in double site-directed peptide modification. The new route is composed of three steps, beginning from an unprotected peptide in which a sequence recognized by the pertinent enzyme is placed between N-terminal Ser and C-terminal Lys. Lys may not occur elsewhere in the peptide. Periodate oxidation converts the N-terminal Ser to an alpha-N-glyoxylyl group, which is then allowed to form a hydrazone with the carbohydrazide derivative Lucifer Yellow CH, a hydrophilic fluor with a large Stokes shift (excitation maximum, 425 nm; emission maximum, 525 nm). Finally, the modified peptide is allowed to react with 5-carboxytetramethylrhodamine succinimidyl ester. This reaction selectively modifies the epsilon-amino group of C-terminal Lys, the only amino group remaining in the peptide. 5-Carboxytetramethylrhodamine strongly (> 90%) quenches Lucifer Yellow fluorescence by resonance energy transfer in the intact substrate, but enzyme-catalyzed cleavage eliminates the quenching. The resulting increase in fluorescence may be used to follow the hydrolytic reaction.
- Sprache
- Englisch
- Identifikatoren
- ISSN: 1043-1802eISSN: 1520-4812DOI: 10.1021/bc00024a017Titel-ID: cdi_proquest_miscellaneous_76209258
- Format
- –
- Schlagworte
- Amino Acid Sequence, Binding Sites, Biological and medical sciences, Collagenases - analysis, Collagenases - chemistry, Collagenases - metabolism, Endopeptidases - analysis, Endopeptidases - chemistry, Endopeptidases - metabolism, Energy Transfer, Fluorescent Dyes - chemistry, Fundamental and applied biological sciences. Psychology, Humans, Hydrolysis, Isoquinolines, Matrix Metalloproteinase 1, Mechanisms. Catalysis. Electron transfer. Models, Molecular biophysics, Molecular Sequence Data, Oxidation-Reduction, Peptides - metabolism, Periodic Acid - metabolism, Periodic Acid - pharmacology, Physical chemistry in biology, Renin - analysis, Renin - chemistry, Renin - metabolism, Serine - chemistry, Serine - metabolism, Substrate Specificity