Research output: Contribution to journal › Article › peer-review
Alternative PCR-Based Approaches for Generation of Komagataella phaffii Strains. / Макеева, Анастасия Станиславовна; Музаев, Дмитрий Михайлович; Шуберт, Мария Андреевна; Яньшина, Татьяна Михайловна; Сидорин, Антон Витальевич; Самбук, Елена Викторовна; Румянцев, Андрей Михайлович; Падкина, Марина Владимировна.
In: Microorganisms, Vol. 11, No. 9, 2297, 12.09.2023.Research output: Contribution to journal › Article › peer-review
}
TY - JOUR
T1 - Alternative PCR-Based Approaches for Generation of Komagataella phaffii Strains.
AU - Макеева, Анастасия Станиславовна
AU - Музаев, Дмитрий Михайлович
AU - Шуберт, Мария Андреевна
AU - Яньшина, Татьяна Михайловна
AU - Сидорин, Антон Витальевич
AU - Самбук, Елена Викторовна
AU - Румянцев, Андрей Михайлович
AU - Падкина, Марина Владимировна
PY - 2023/9/12
Y1 - 2023/9/12
N2 - Komagataella phaffii (Pichia pastoris) is a widely known microbial host for recombinant protein production and an emerging model organism in fundamental research. The development of new materials and techniques on this yeast improves heterologous protein synthesis. One of the most prominent ways to enhance protein production efficiency is to select K. phaffii strains with multiple expression cassettes and generate MutS strains using various vectors. In this study, we demonstrate approaches to expand the applications of pPICZ series vectors. Procedures based on PCR amplification and in vivo cloning allow rapid exchange of selectable markers. The combination of PCR amplification with split-marker-mediated transformation allows the development of K. phaffii MutS strains with two expression cassettes using pPICZ vectors. Both PCR-based approaches were applied to efficiently produce interleukin-2 mimetic Neo-2/15 in K. phaffii. The described techniques provide alternative ways to generate and improve K. phaffii strains without the need for obtaining new specific vectors or additional cloning of expression cassettes.
AB - Komagataella phaffii (Pichia pastoris) is a widely known microbial host for recombinant protein production and an emerging model organism in fundamental research. The development of new materials and techniques on this yeast improves heterologous protein synthesis. One of the most prominent ways to enhance protein production efficiency is to select K. phaffii strains with multiple expression cassettes and generate MutS strains using various vectors. In this study, we demonstrate approaches to expand the applications of pPICZ series vectors. Procedures based on PCR amplification and in vivo cloning allow rapid exchange of selectable markers. The combination of PCR amplification with split-marker-mediated transformation allows the development of K. phaffii MutS strains with two expression cassettes using pPICZ vectors. Both PCR-based approaches were applied to efficiently produce interleukin-2 mimetic Neo-2/15 in K. phaffii. The described techniques provide alternative ways to generate and improve K. phaffii strains without the need for obtaining new specific vectors or additional cloning of expression cassettes.
KW - Komagataella phaffii
KW - Neo-2/15
KW - Pichia pastoris
KW - heterologous protein production
KW - multicopy strains
KW - split markers
UR - https://www.mendeley.com/catalogue/d2f51c0f-6586-3a2d-8bd7-c68e9c31778d/
U2 - 10.3390/microorganisms11092297
DO - 10.3390/microorganisms11092297
M3 - Article
VL - 11
JO - Microorganisms
JF - Microorganisms
SN - 2076-2607
IS - 9
M1 - 2297
ER -
ID: 114209686