Using S. cerevisiae cell wall proteins as a anchor for expression of heterologous proteins at the cell surface

Teparić, Renata; Mrša, Vladimir

Pregled bibliografske jedinice broj: 464755

Using S. cerevisiae cell wall proteins as a anchor for expression of heterologous proteins at the cell surface

Teparić, Renata; Mrša, Vladimir

Using S. cerevisiae cell wall proteins as a anchor for expression of heterologous proteins at the cell surface // Acta Microbiologica at Immunologica Hungarica / Marialigeti, K. (ur.).
Budimpešta: Akadémiai Kiadó, 2009. (poster, međunarodna recenzija, sažetak, znanstveni)

CROSBI ID: 464755 Za ispravke kontaktirajte CROSBI podršku putem web obrasca

Naslov
Using S. cerevisiae cell wall proteins as a anchor for expression of heterologous proteins at the cell surface

Autori
Teparić, Renata ; Mrša, Vladimir

Vrsta, podvrsta i kategorija rada
Sažeci sa skupova, sažetak, znanstveni

Izvornik
Acta Microbiologica at Immunologica Hungarica / Marialigeti, K. - Budimpešta : Akadémiai Kiadó, 2009

Skup
Second Central European Forum for Microbiology

Mjesto i datum
Keszthely, Mađarska, 07.10.2009. - 09.10.2009

Vrsta sudjelovanja
Poster

Vrsta recenzije
Međunarodna recenzija

Ključne riječi
cell wall; Pir4p; Ccw12p; heterologous expression

Sažetak
In the past several years much efforts have been devoted to the study of expression systems for the display of heterologous proteins at the surface of microorganisms, opening new perspectives in biotechnology. Yeast cell surface systems have the advantages of simplicity of genetic manipulation and ability for proper post-translational modifications and folding of mammalian proteins. Yeast whole-cell biocatalysts displaying enzymes on their cell surface can be produced at a low cost and show a high enzymatic activity. Recently a number of surface – engineered yeasts, displaying different heterologous proteins interesting for biotechnological or medical applications, have been constructed. S. cerevisiae cell wall proteins that are covalently bound to the carbohydrate components of the wall can be divided in two main groups. Majority of proteins of this class are bound at their C-termini through a remnant of the GPI-anchor. A smaller group of proteins are directly covalently bound at their N-termini to beta-1, 3-glucan by the alkali labile ester linkage between the glutamic acid gamma-carboxyl group and hydroxyl groups of glucoses (Pir – proteins). Almost all heterologous proteins constructed so far for yeast surface display are GPI-anchored to the cell wall using C-terminal part of alpha-agglutinin as anchor. Some enzymes, whose active sites are located near their C-terminiare not suitable for display through GPI anchor that must be fused at their C-terminal region. Possible approach for such enzymes is to use Pir –proteins as a cell wall anchor. In this work Pir4p was used as anchor for N-terminal immobilization and Ccw12p for C-terminal immobilization of heterologous proteins to the yeast cell surface.

Izvorni jezik
Engleski

Znanstvena područja
Biotehnologija

POVEZANOST RADA

Projekti:
058-0580477-2240 - Molekularni mehanizmi ugradnje proteina u staničnu stijenku kvasca (Mrša, Vladimir, MZOS ) ( CroRIS)

Ustanove:
Prehrambeno-biotehnološki fakultet, Zagreb

Profili:

Vladimir Mrša (autor)