Cell-free methods to produce structurally intact mammalian membrane proteins

Shinoda, Takehiro; Shinya, Naoko; Ito, Kaori; Ishizuka-Katsura, Yoshiko; Ohsawa, Noboru; Terada, Takaho; Hirata, Kunio; Kawano, Yoshiaki; Yamamoto, Masaki; Tomita, Taisuke; Ishibashi, Yoshihiro; Hirabayashi, Yoshio; Kimura‐Someya, Tomomi; Shirouzu, Mikako; Yokoyama, Shigeyuki

doi:10.1038/srep30442

Cited by 58 publications

(51 citation statements)

References 53 publications

(76 reference statements)

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“…Membrane protein synthesis in insect cell‐free systems has already started over 10 years ago. Although yields for soluble proteins are frequently lower compared to E.coli and wheat germ based cell‐free systems, membrane protein synthesis in insect based cell‐free systems has meanwhile reached a comparable level (Shinoda et al, ). The insect cell‐free synthesis system initially achieved membrane protein yields in the range of 5–20 μg/mL.…”

Section: Discussionmentioning

confidence: 99%

Production of G protein‐coupled receptors in an insect‐based cell‐free system

Sonnabend

Spahn

Stech

et al. 2017

Biotech & Bioengineering

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The biochemical analysis of human cell membrane proteins remains a challenging task due to the difficulties in producing sufficient quantities of functional protein. G protein‐coupled receptors (GPCRs) represent a main class of membrane proteins and drug targets, which are responsible for a huge number of signaling processes regulating various physiological functions in living cells. To circumvent the current bottlenecks in GPCR studies, we propose the synthesis of GPCRs in eukaryotic cell‐free systems based on extracts generated from insect (Sf21) cells. Insect cell lysates harbor the fully active translational and translocational machinery allowing posttranslational modifications, such as glycosylation and phosphorylation of de novo synthesized proteins. Here, we demonstrate the production of several GPCRs in a eukaryotic cell‐free system, performed within a short time and in a cost‐effective manner. We were able to synthesize a variety of GPCRs ranging from 40 to 133 kDa in an insect‐based cell‐free system. Moreover, we have chosen the μ opioid receptor (MOR) as a model protein to analyze the ligand binding affinities of cell‐free synthesized MOR in comparison to MOR expressed in a human cell line by “one‐point” radioligand binding experiments. Biotechnol. Bioeng. 2017;114: 2328–2338. © 2017 The Authors. Biotechnology and Bioengineering Published by Wiley Periodicals, Inc.

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Section: Discussionmentioning

confidence: 99%

Production of G protein‐coupled receptors in an insect‐based cell‐free system

Sonnabend

Spahn

Stech

et al. 2017

Biotech & Bioengineering

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“…Composition of the cell-free protein synthesis reactions were basically the same as previously reported (31). Dialysis method (53) was performed by using a 24-well plate filled with 1 ml feeding solution per well.…”

Section: Measurement Of the Protein Synthesis Activity Of The Extractmentioning

confidence: 99%

“…6). The addition of 'N11-tag', whose sequence is similar to that of the poly-histidine affinity tag (HAT) (31,62), to the N-terminus exhibited 20-fold increase in the yield of GST-GFPS2 fusion protein (N11GST-GFPS2 in Fig. 6), suggesting that this problem could be overcome by altering the N-terminal sequence of GST.…”

Section: Determination Of Protein Synthesis Activity Of S30 Extractmentioning

confidence: 99%

A reproducible and scalable procedure for preparing bacterial extracts for cell-free protein synthesis

Katsura

Matsuda

Tomabechi

et al. 2017

The Journal of Biochemistry

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Cell-free protein synthesis is a useful method for preparing proteins for functional or structural analyses. However, batch-to-batch variability with regard to protein synthesis activity remains a problem for large-scale production of cell extract in the laboratory. To address this issue, we have developed a novel procedure for large-scale preparation of bacterial cell extract with high protein synthesis activity. The developed procedure comprises cell cultivation using a fermentor, harvesting and washing of cells by tangential flow filtration, cell disruption with high-pressure homogenizer and continuous diafiltration. By optimizing and combining these methods, ∼100 ml of the cell extract was prepared from 150 g of Escherichia coli cells. The protein synthesis activities, defined as the yield of protein per unit of absorbance at 260 nm of the cell extract, were shown to be reproducible, and the average activity of several batches was twice that obtained using a previously reported method. In addition, combinatorial use of the high-pressure homogenizer and diafiltration increased the scalability, indicating that the cell concentration at disruption varies from 0.04 to 1 g/ml. Furthermore, addition of Gam protein and examinations of the N-terminal sequence rendered the extract prepared here useful for rapid screening with linear DNA templates.

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“…For crystallization, the C‐terminal fragments of claudins are truncated in all of the expression constructs . The flexible C‐terminus is dispensable for forming TJ‐like strand polymers in vitro , although the majority of claudins have a PDZ‐binding motif (–YV) at the C‐terminus that is critical for binding to many kinds of scaffolding proteins in vivo as well as for proper recruitment of claudins at TJ regions .…”

Section: Overall Structure Of the Claudin Foldmentioning

confidence: 99%

“…For crystallization, the C-terminal fragments of claudins are truncated in all of the expression constructs. [6][7][8]18 The flexible C-terminus is dispensable for forming TJ-like strand polymers in vitro, 6 although the majority of claudins have a PDZ-binding motif (-YV) at the C-terminus that is critical for binding to many kinds of scaffolding proteins in vivo 3,19 as well as for proper recruitment of claudins at TJ regions. 4 In addition, none of the three claudins contained any posttranslational lipid modifications owing to the deficient mutations in the expression constructs or properties of the cell-free protein synthesis method.…”

Section: Overall Structure Of the Claudin Foldmentioning

confidence: 99%

Crystal structures of claudins: insights into their intermolecular interactions

Suzuki

Tani

Fujiyoshi

2017

Annals of the New York Academy of Sciences

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Claudins are four-transmembrane proteins that constitute the backbone of tight junction strands via selfpolymerization in the apicolateral membranes of epithelial cells. Together with their cell-cell adhesion function, claudin proteins form the paracellular barrier and/or channels through epithelial cell sheets whose permeability is primarily dependent on the claudin subtype. Recently determined crystal structures of several claudins revealed the unique claudin fold of four transmembrane helices in a left-handed helical bundle with an extracellular ␤-sheet domain. Here, we focus on the structural basis of the intermolecular interactions between claudin molecules and between the Clostridium perfringens enterotoxin and its receptor claudins.

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Cell-free methods to produce structurally intact mammalian membrane proteins

Cited by 58 publications

References 53 publications

Production of G protein‐coupled receptors in an insect‐based cell‐free system

Production of G protein‐coupled receptors in an insect‐based cell‐free system

A reproducible and scalable procedure for preparing bacterial extracts for cell-free protein synthesis

Crystal structures of claudins: insights into their intermolecular interactions

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