Creating a bifunctional protein by insertion of β-lactamase into the maltodextrin-binding protein

Creating a bifunctional protein by insertion of β-lactamase into the maltodextrin-binding protein

Hybrid proteins were generated by inserting the penicillin-hydrolyzing enzyme, TEM β-lactamase (Bla), into the maltodextrin-binding protein (MalE). The inserted Bla was functionally accommodated by MalE when it was placed within permissive sites. The maltose binding and penicillinase activities of p...

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Veröffentlicht in:Nature biotechnology 1997-11, Vol.15 (12), p.1276-1279
Hauptverfasser: Betton, Jean-Michel, Jacob, Jansen P, Hofnung, Maurice, Broome-Smith, Jenny K
Format: Artikel
Sprache:eng
Schlagworte:
Agriculture
Bacterial Proteins - chemistry
beta-Lactamases - chemistry
beta-Lactamases - metabolism
Binding Sites
Bioinformatics
Biological and medical sciences
Biomedical and Life Sciences
Biomedical Engineering/Biotechnology
Biomedicine
Biotechnology
Carrier Proteins - chemistry
Escherichia coli - chemistry
Escherichia coli - genetics
Escherichia coli Proteins
Fundamental and applied biological sciences. Psychology
Life Sciences
Methods. Procedures. Technologies
Periplasmic Binding Proteins
Plasmids
Protein engineering
Protein Folding
research-article
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Zusammenfassung:Hybrid proteins were generated by inserting the penicillin-hydrolyzing enzyme, TEM β-lactamase (Bla), into the maltodextrin-binding protein (MalE). The inserted Bla was functionally accommodated by MalE when it was placed within permissive sites. The maltose binding and penicillinase activities of purified hybrids were indistinguishable from those of the wild-type MalE and Bla proteins. Moreover, these hybrids displayed an additional unexpected property: maltose stabilized the active site of inserted Bla.
ISSN:1087-0156
1546-1696
DOI:10.1038/nbt1197-1276