The N‐terminal peptide of the transglutaminase‐activating metalloprotease inhibitor from Streptomyces mobaraensis accommodates both inhibition and glutamine cross‐linking sites

Juettner, Norbert E. ; Schmelz, Stefan ; Anderl, Anita ; Colin, Felix ; Classen, Moritz ; Pfeifer, Felicitas ; Scrima, Andrea ; Fuchsbauer, Hans‐Lothar (2024)
The N‐terminal peptide of the transglutaminase‐activating metalloprotease inhibitor from Streptomyces mobaraensis accommodates both inhibition and glutamine cross‐linking sites.
In: The FEBS Journal, 2020, 287 (4)
doi: 10.26083/tuprints-00016178
Artikel, Zweitveröffentlichung, Verlagsversion

Es ist eine neuere Version dieses Eintrags verfügbar.

URL / URN: https://tuprints.ulb.tu-darmstadt.de/16178

Kurzbeschreibung (Abstract)

Streptomyces mobaraensis is a key player for the industrial production of the protein cross‐linking enzyme microbial transglutaminase (MTG). Extra‐cellular activation of MTG by the transglutaminase‐activating metalloprotease (TAMP) is regulated by the TAMP inhibitory protein SSTI that belongs to the large Streptomyces subtilisin inhibitor (SSI) family. Despite decades of SSI research, the binding site for metalloproteases such as TAMP remained elusive in most of the SSI proteins. Moreover, SSTI is a MTG substrate, and the preferred glutamine residues for SSTI cross‐linking are not determined. To address both issues, that is, determination of the TAMP and the MTG glutamine binding sites, SSTI was modified by distinct point mutations as well as elongation or truncation of the N‐terminal peptide by six and three residues respectively. Structural integrity of the mutants was verified by the determination of protein melting points and supported by unimpaired subtilisin inhibitory activity. While exchange of single amino acids could not disrupt decisively the SSTI TAMP interaction, the N‐terminally shortened variants clearly indicated the highly conserved Leu40‐Tyr41 as binding motif for TAMP. Moreover, enzymatic biotinylation revealed that an adjacent glutamine pair, upstream from Leu40‐Tyr41 in the SSTI precursor protein, is the preferred binding site of MTG. This extension peptide disturbs the interaction with TAMP. The structure of SSTI was furthermore determined by X‐ray crystallography. While no structural data could be obtained for the N‐terminal peptide due to flexibility, the core structure starting from Tyr41 could be determined and analysed, which superposes well with SSI‐family proteins.

Typ des Eintrags:	Artikel
Erschienen:	2024
Autor(en):	Juettner, Norbert E. ; Schmelz, Stefan ; Anderl, Anita ; Colin, Felix ; Classen, Moritz ; Pfeifer, Felicitas ; Scrima, Andrea ; Fuchsbauer, Hans‐Lothar
Art des Eintrags:	Zweitveröffentlichung
Titel:	The N‐terminal peptide of the transglutaminase‐activating metalloprotease inhibitor from Streptomyces mobaraensis accommodates both inhibition and glutamine cross‐linking sites
Sprache:	Englisch
Publikationsjahr:	9 Januar 2024
Ort:	Darmstadt
Publikationsdatum der Erstveröffentlichung:	2020
Ort der Erstveröffentlichung:	Oxford
Verlag:	John Wiley & Sons
Titel der Zeitschrift, Zeitung oder Schriftenreihe:	The FEBS Journal
Jahrgang/Volume einer Zeitschrift:	287
(Heft-)Nummer:	4
DOI:	10.26083/tuprints-00016178
URL / URN:	https://tuprints.ulb.tu-darmstadt.de/16178
Zugehörige Links:	Verlags-DOI
Herkunft:	Zweitveröffentlichung DeepGreen
Kurzbeschreibung (Abstract):	Streptomyces mobaraensis is a key player for the industrial production of the protein cross‐linking enzyme microbial transglutaminase (MTG). Extra‐cellular activation of MTG by the transglutaminase‐activating metalloprotease (TAMP) is regulated by the TAMP inhibitory protein SSTI that belongs to the large Streptomyces subtilisin inhibitor (SSI) family. Despite decades of SSI research, the binding site for metalloproteases such as TAMP remained elusive in most of the SSI proteins. Moreover, SSTI is a MTG substrate, and the preferred glutamine residues for SSTI cross‐linking are not determined. To address both issues, that is, determination of the TAMP and the MTG glutamine binding sites, SSTI was modified by distinct point mutations as well as elongation or truncation of the N‐terminal peptide by six and three residues respectively. Structural integrity of the mutants was verified by the determination of protein melting points and supported by unimpaired subtilisin inhibitory activity. While exchange of single amino acids could not disrupt decisively the SSTI TAMP interaction, the N‐terminally shortened variants clearly indicated the highly conserved Leu40‐Tyr41 as binding motif for TAMP. Moreover, enzymatic biotinylation revealed that an adjacent glutamine pair, upstream from Leu40‐Tyr41 in the SSTI precursor protein, is the preferred binding site of MTG. This extension peptide disturbs the interaction with TAMP. The structure of SSTI was furthermore determined by X‐ray crystallography. While no structural data could be obtained for the N‐terminal peptide due to flexibility, the core structure starting from Tyr41 could be determined and analysed, which superposes well with SSI‐family proteins.
Freie Schlagworte:	crystal structure, metalloprotease inhibitor, serine protease inhibitor, Streptomyces mobaraensis, transglutaminase
Status:	Verlagsversion
URN:	urn:nbn:de:tuda-tuprints-161787
Zusätzliche Informationen:	Enzymes: Chymotrypsin, EC3.4.21.1; griselysin (SGMPII, SgmA), EC3.4.24.27; snapalysin (ScNP), EC3.4.24.77; streptogrisin‐A (SGPA), EC3.4.21.80; streptogrisin‐B (SGPB), EC3.4.21.81; subtilisin BPN’, EC3.4.21.62; transglutaminase, EC2.3.2.13; transglutaminase‐activating metalloprotease (TAMP), EC3.4.‐.‐; tri‐/tetrapeptidyl aminopeptidase, EC3.4.11.‐; trypsin, EC3.4.21.4. Databases: The atomic coordinates and structure factors (PDB 6I0I) have been deposited in the Protein Data Bank (http://www.rcsb.org).
Sachgruppe der Dewey Dezimalklassifikatin (DDC):	500 Naturwissenschaften und Mathematik > 570 Biowissenschaften, Biologie
Fachbereich(e)/-gebiet(e):	10 Fachbereich Biologie 10 Fachbereich Biologie > Microbiology and Archaea
Hinterlegungsdatum:	09 Jan 2024 12:14
Letzte Änderung:	10 Jan 2024 09:51
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The N‐terminal peptide of the transglutaminase‐activating metalloprotease inhibitor from Streptomyces mobaraensis accommodates both inhibition and glutamine cross‐linking sites. (deposited 09 Jan 2024 12:14) [Gegenwärtig angezeigt]
- The N-terminal peptide of the transglutaminase-activating metalloprotease inhibitor from Streptomyces mobaraensis accommodates both inhibition and glutamine cross-linking sites. (deposited 26 Aug 2019 11:07)

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