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Expression of the Bacterial Enzyme IdeS Using a GFP Fusion in the Yeast Saccharomyces cerevisiae

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Sammanfattning

Bacterial proteases are important enzymes used in several technical applications where controlled cleavage of proteins is needed. They are challenging enzymes to express recombinantly as parts of the proteome can be hydrolyzed by their activity. The eukaryotic model organism Saccharomyces cerevisiae is potentially a good expression host as it tolerates several stress conditions and is known to better express insoluble proteins compared to bacterial systems. In this chapter we describe how the protease IdeS from Streptococcus pyogenes can be expressed in S. cerevisiae. The expression of IdeS was followed by constructing a fused protein with GFP and measuring the fluorescence with flow cytometry. The protease presence was confirmed with a Western blot assay and activity was measured with an in vitro assay. To reduce potentially toxic effect on the host cell, the growth and production phases were separated by using the inducible promoter GAL1p to control recombinant gene expression. The protocol provided may be adopted for other bacterial proteases through minor modifications of the fused protein.

Originalspråkengelska
Titel på värdpublikationBacterial pathogenesis
Undertitel på värdpublikationMethods and protocols
Redaktörer/författarePontus Nordenfelt, Mattias Collin
FörlagHumana Press
Kapitel9
Sidor131-146
Utgåva2nd
ISBN (elektroniskt)978-1-0716-3243-7
DOI
StatusPublished - 2023

Publikationsserier

NamnMethods in molecular biology (Clifton, N.J.)
FörlagSpringer
ISSN (tryckt)1940-6029

Ämnesklassifikation (UKÄ)

  • Mikrobiologi inom det medicinska området

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