Saccharomyces cerevisiae as a superior host for overproduction of prokaryotic integral membrane proteins

Preisler, Sarah Spruce; Wiuf, Anders; Friis, M.D.Steffen U.; Kjaergaard, L L; Hurd, Molly; Becares, Eva Ramos; Nurup, Casper Normann; Bjoerkskov, Frederik Bühring; Szathmáry, Zsófia; Gourdon, Pontus; Calloe, Kirstine; Klærke, Dan A.; Gotfryd, Kamil; Pedersen, Per Amstrup

doi:10.1016/j.crstbi.2021.02.001

Cited by 7 publications

(2 citation statements)

References 67 publications

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“…6a and Table 2 ). These current values are consistent with the previously reported single channel recording experimental data of NavAb or BacNavs 31 , 32 . Therefore, the simulation applying the ECC well represented the actual situation.…”

Section: Resultssupporting

confidence: 93%

The structural basis of divalent cation block in a tetrameric prokaryotic sodium channel

et al. 2023

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Divalent cation block is observed in various tetrameric ion channels. For blocking, a divalent cation is thought to bind in the ion pathway of the channel, but such block has not yet been directly observed. So, the behaviour of these blocking divalent cations remains still uncertain. Here, we elucidated the mechanism of the divalent cation block by reproducing the blocking effect into NavAb, a well-studied tetrameric sodium channel. Our crystal structures of NavAb mutants show that the mutations increasing the hydrophilicity of the inner vestibule of the pore domain enable a divalent cation to stack on the ion pathway. Furthermore, non-equilibrium molecular dynamics simulation showed that the stacking calcium ion repel sodium ion at the bottom of the selectivity filter. These results suggest the primary process of the divalent cation block mechanism in tetrameric cation channels.

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Section: Resultssupporting

confidence: 93%

The structural basis of divalent cation block in a tetrameric prokaryotic sodium channel

et al. 2023

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“…Obtaining sufficient quantities of pure membrane protein can be both challenging and time consuming due to low expression levels, solubility issues and challenges in obtaining and maintaining uniformly folded protein. To overcome some of these challenges, we employed the previously developed PAP1500 S. cerevisiae -based membrane protein expression platform [ 31 , 32 , 33 , 34 , 35 , 36 ], and coupled this with GFP tagging to produce full-length human FICD ( Figure 2 ). This platform has been successfully used to produce multi-spanning membrane proteins such as aquaporins, transmembrane ATPases and ion channels [ 32 , 33 , 34 , 35 , 37 , 38 , 39 , 40 ].…”

Section: Introductionmentioning

confidence: 99%

Production of an Active, Human Membrane Protein in Saccharomyces cerevisiae: Full-Length FICD

Virolainen

Søltoft

Pedersen

et al. 2022

IJMS

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The human Fic domain-containing protein (FICD) is a type II endoplasmic reticulum (ER) membrane protein that is important for the maintenance of ER proteostasis. Structural and in vitro biochemical characterisation of FICD AMPylase and deAMPylase activity have been restricted to the soluble ER-luminal domain produced in Escherichia coli. Information about potentially important features, such as structural motifs, modulator binding sites or other regulatory elements, is therefore missing for the approximately 100 N-terminal residues including the transmembrane region of FICD. Expressing and purifying the required quantity and quality of membrane proteins is demanding because of the low yields and poor stability often observed. Here, we produce full-length FICD by combining a Saccharomyces cerevisiae-based platform with green fluorescent protein (GFP) tagging to optimise the conditions for expression, solubilisation and purification. We subsequently employ these conditions to purify milligram quantities of His-tagged FICD per litre of culture, and show that the purified, detergent-solubilised membrane protein is an active deAMPylating enzyme. Our work provides a straightforward methodology for producing not only full-length FICD, but also other membrane proteins in S. cerevisiae for structural and biochemical characterisation.

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Overproduction of Membrane-Associated, and Integrated, Proteins Using Saccharomyces cerevisiae

Haslem

Brown

Zhang

et al. 2022

Methods in Molecular Biology

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Saccharomyces cerevisiae as a superior host for overproduction of prokaryotic integral membrane proteins

Cited by 7 publications

References 67 publications

The structural basis of divalent cation block in a tetrameric prokaryotic sodium channel

The structural basis of divalent cation block in a tetrameric prokaryotic sodium channel

Production of an Active, Human Membrane Protein in Saccharomyces cerevisiae: Full-Length FICD

Overproduction of Membrane-Associated, and Integrated, Proteins Using Saccharomyces cerevisiae

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