Improving cell-free expression of membrane proteins by tuning ribosome co-translational membrane association and nascent chain aggregation

Steinkühler, Jan; Peruzzi, Justin A.; Krüger, Antje; Jacobs, Miranda L.; Jewett, Michael C.; Kamat, Neha P.

doi:10.1101/2023.02.10.527944

Cited by 4 publications

(5 citation statements)

References 49 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…These results correspond to the previous time series ( Figure 2 b) and additionally suggest the requirement of further protein processing time for higher order oligomer assembly. It should be noted that the absence of microsomes reduced the protein yield, consistent with other studies [ 23 ] and thus causes overall weaker protein bands in the autoradiogram.…”

Section: Resultssupporting

confidence: 90%

Evaluation of the Ion Channel Assembly in a Eukaryotic Cell-Free System Focusing on Two-Pore Domain Potassium Channels K2P

Ullrich

Ohlhoff

Dondapati

et al. 2023

IJMS

View full text Add to dashboard Cite

Oligomeric ion channels are abundant in nature. However, the recombinant expression in cell culture-based systems remains tedious and challenging due to negative side effects, limiting the understanding of their role in health and disease. Accordingly, in this work, we demonstrate the cell-free synthesis (CFS) as an alternative platform to study the assembly of two-pore domain potassium channels (K2P) within endogenous endoplasmic reticulum-derived microsomes. Exploiting the open nature of CFS, we investigate the cotranslational translocation of TREK-2 into the microsomes and suggest a cotranslational assembly with typical single-channel behavior in planar lipid-bilayer electrophysiology. The heteromeric assembly of K2P channels is a contentious matter, accordingly we prove the successful assembly of TREK-2 with TWIK-1 using a biomolecular fluorescence complementation assay, Western blot analysis and autoradiography. The results demonstrate that TREK-2 homodimer assembly is the initial step, followed by heterodimer formation with the nascent TWIK-1, providing evidence of the intergroup heterodimerization of TREK-2 and TWIK-1 in eukaryotic CFS. Since K2P channels are involved in various pathophysiological conditions, including pain and nociception, CFS paves the way for in-depth functional studies and related pharmacological interventions. This study highlights the versatility of the eukaryotic CFS platform for investigating ion channel assembly in a native-like environment.

show abstract

Section: Resultssupporting

confidence: 90%

Evaluation of the Ion Channel Assembly in a Eukaryotic Cell-Free System Focusing on Two-Pore Domain Potassium Channels K2P

Ullrich

Ohlhoff

Dondapati

et al. 2023

IJMS

View full text Add to dashboard Cite

show abstract

“…3 C ). This nitrate-independent increase in luminescence upon addition of POPE may suggest that negative lipid curvature stabilizes the “on” conformation of NarX ( 44 ). The high induction of luciferase expression in POPE and POPG membranes is unsurprising as PE and PG make up the majority of lipid headgroups in E. coli membranes ( 46 ).…”

Section: Resultsmentioning

confidence: 98%

“…S5 ). Further, improper membrane protein folding has been found to increase aggregation and truncation products ( 41 , 44 ), and likely inhibits efficient expression of all protein components in the system. As a result of this relationship, we only considered NarX expression in our future analysis of the effect of membrane composition on NarX-L performance.…”

Section: Resultsmentioning

confidence: 99%

“…However, luminescence for the vancomycin sensor was highest across all conditions ( Fig. 4 E ), suggesting that the chimera may be locked into an on conformation, perhaps due to destabilizing the HAMP domain ( 44 ). These results demonstrate how protein and membrane engineering can be used to readily generate cell-free receptors by tapping into the large repertoire of known sensing domains of transmembrane proteins, and underscores the important relationship between membrane physical properties, protein sequence, and function.…”

Section: Resultsmentioning

confidence: 99%

See 1 more Smart Citation

Engineering transmembrane signal transduction in synthetic membranes using two-component systems

Peruzzi

Galvez

Kamat

2023

Proc. Natl. Acad. Sci. U.S.A.

Self Cite

View full text Add to dashboard Cite

Cells use signal transduction across their membranes to sense and respond to a wide array of chemical and physical signals. Creating synthetic systems which can harness cellular signaling modalities promises to provide a powerful platform for biosensing and therapeutic applications. As a first step toward this goal, we investigated how bacterial two-component systems (TCSs) can be leveraged to enable transmembrane-signaling with synthetic membranes. Specifically, we demonstrate that a bacterial two-component nitrate-sensing system (NarX-NarL) can be reproduced outside of a cell using synthetic membranes and cell-free protein expression systems. We find that performance and sensitivity of the TCS can be tuned by altering the biophysical properties of the membrane in which the histidine kinase (NarX) is integrated. Through protein engineering efforts, we modify the sensing domain of NarX to generate sensors capable of detecting an array of ligands. Finally, we demonstrate that these systems can sense ligands in relevant sample environments. By leveraging membrane and protein design, this work helps reveal how transmembrane sensing can be recapitulated outside of the cell, adding to the arsenal of deployable cell-free systems primed for real world biosensing.

show abstract

“…However, this peptide is unnecessary in our cell-free system that lacks a signal recognition particle and we hypothesized that the presence of the hydrophobic peptide in the nascent peptide chain might hinder the cotranslational integration of the membrane protein into liposome membranes. Further, we have previously found that sequence alterations in the nascent chain of a cell-free expressed membrane protein can have a profound impact on cell-free membrane protein expression (56). Specifically, we identified that alterations in protein sequence that inhibit protein-lipid interactions lead to membrane proteins that cannot successfully move off the ribosome and insert into membranes.…”

Section: Alterations In the Nascent Peptide Sequence Of Nipah Transme...mentioning

confidence: 99%

Cell-free expression of Nipah virus transmembrane proteins for proteoliposome vaccine design

Hu,

Ezzatpour,

Selivanovitch

et al. 2024

Preprint

Self Cite

View full text Add to dashboard Cite

Membrane proteins expressed on the surface of enveloped viruses are potent antigens in a vaccine, yet are difficult to produce and present due to their instability without a lipid scaffold. Current vaccination strategies that incorporate viral membrane proteins, such as live attenuated viruses, inactivated viruses, or extracellular vesicles, have limitations including lengthy production time, poor immunogenicity, extensive processing steps, and/or poor stability. Cell-free protein synthesis of viral membrane proteins offers a rapid, one-step method to assemble vaccine nanoparticles via cotranslational folding of membrane proteins into nanoscale liposomes. Here, we develop a vaccine candidate for the deadly Nipah virus (NiV), a highly lethal virus listed by the World Health Organization as a priority pathogen, by cell-free expressing two full-length Nipah virus membrane proteins. We demonstrate that both NiV fusion protein (NiV F) and NiV glycoprotein (NiV G) can be expressed and cotranslationally integrated into liposomes and that they fold into their native conformation. We find the removal of a signal peptide sequence and alteration of liposome lipid composition improves viral membrane protein incorporation. Furthermore, a lipid adjuvant, monophosphoryl lipid A (MPLA), can be readily added to liposomes without disrupting protein-vesicle loading or protein folding conformations. Finally, we demonstrate that our generated liposomal formulations lead to enhanced humoral responses in mice compared to empty and single-protein controls. This work establishes a platform to quickly assemble and present membrane antigens as multivalent vaccines that will enable a rapid response to the broad range of emerging pathogenic threats.

show abstract

Improving cell-free expression of membrane proteins by tuning ribosome co-translational membrane association and nascent chain aggregation

Cited by 4 publications

References 49 publications

Evaluation of the Ion Channel Assembly in a Eukaryotic Cell-Free System Focusing on Two-Pore Domain Potassium Channels K2P

Evaluation of the Ion Channel Assembly in a Eukaryotic Cell-Free System Focusing on Two-Pore Domain Potassium Channels K2P

Engineering transmembrane signal transduction in synthetic membranes using two-component systems

Cell-free expression of Nipah virus transmembrane proteins for proteoliposome vaccine design

Contact Info

Product

Resources

About