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Construction of Out-of-Equilibrium Metabolic Networks in Nano- and Micrometer-Sized Vesicles
In This Article
Summary
We present a protocol for reconstituting membrane proteins and encapsulating enzymes and other water-soluble components in lipid vesicles of sub-micrometer and micrometer size.
Abstract
We present a method to incorporate into vesicles complex protein networks, involving integral membrane proteins, enzymes, and fluorescence-based sensors, using purified components. This method is relevant for the design and construction of bioreactors and the study of complex out-of-equilibrium metabolic reaction networks. We start by reconstituting (multiple) membrane proteins into large unilamellar vesicles (LUVs) according to a previously developed protocol. We then encapsulate a mixture of purified enzymes, metabolites, and fluorescence-based sensors (fluorescent proteins or dyes) via freeze-thaw-extrusion and remove non-incorporated components by centrifugation and/or size-exclusion chromatography. The performance of the metabolic networks is measured in real time by monitoring the ATP/ADP ratio, metabolite concentration, internal pH, or other parameters by fluorescence readout. Our membrane protein-containing vesicles of 100-400 nm diameter can be converted into giant-unilamellar vesicles (GUVs), using existing but optimized procedures. The approach enables the inclusion of soluble components (enzymes, metabolites, sensors) into micrometer-size vesicles, thus upscaling the volume of the bioreactors by orders of magnitude. The metabolic network containing GUVs areĀ trapped in microfluidic devices for analysis by optical microscopy.
Introduction
The field of bottom-up synthetic biology focuses on constructing (minimal) cells1,2 and metabolic bioreactors for biotechnological3,4 or biomedical purposes5,6,7,8. The construction of synthetic cells provides a unique platform that allows researchers to study (membrane) proteins in well-defined conditions mimicking those of native environments, enabling the discovery of emergent properties and concealed biochemical ....
Protocol
1. General preparation
- Chemicals
- Dissolve lipids (in powder form) to 25 mg/mL in CHCl3 for making preformed liposomes.
NOTE: It is preferable to prepare fresh lipid stocks, but the stock solutions can also be stored at -20 Ā°C for a few weeks. Working with lipids in powder form is more accurate than using lipids already solubilized in CHCl3. CHCl3 should be handled using glass pipettes and/or syringes and stored in glass containers as C.......
- Dissolve lipids (in powder form) to 25 mg/mL in CHCl3 for making preformed liposomes.
Representative Results
The reconstitution of solubilized membrane proteins in liposomes requires the destabilization of preformed vesicles. The addition of low amounts of Triton X-100 initially results in an increase of absorbance at 540 nm (A540) due to an increase in light scattering by the swelling of the vesicles (Figure 4). The maximum A540 value is the point where the liposomes are saturated with detergent (Rsat), after which any further addition of Triton X-100 will.......
Discussion
We present a protocol for the synthesis of (membrane) protein containing sub-micrometer size lipid vesicles (proteoLUVs), and the conversion of proteoLUVs into giant-unilamellar vesicles (proteoGUVs). The protocol should be applicable for the reconstitution of other membrane proteins13,19,30,40 and the encapsulation of metabolic networks other than the L-arginine breakdown and glycerol 3-phosph.......
Acknowledgements
The authors thank Aditya Iyer for the cloning of the pBAD-PercevalHR gene and Gea Schuurman-Wolters for aiding with protein production and purification. The research was funded by the NWO Gravitation program "Building a Synthetic Cell" (BaSyC).
....Materials
| Name | Company | Catalog Number | Comments |
| Agarose | Sigma Aldrich | A9414-25g | |
| Amicon cut-off filter | Sigma Aldrich | Milipore centrifugal filter units Amicon UltraĀ | |
| BioBeads | BioRad | 152-3920 | |
| CHCl3 | Macron Fine Chemicals | MFCD00000826 | |
| D(+)-Glucose | Formedium | - | |
| D(+)-Sucrose | Formedium | - | |
| DDM | Glycon | D97002 -C | |
| Diethyl Ether | Biosolve | 52805 | |
| DMSO | Sigma-Aldrich | 276855-100ml | |
| DOPC | Avanti | 850375P-1g | |
| DOPE | Avanti | 850725P-1g | |
| DOPG | Avanti | 840475P-1g | |
| DTT | FormediumĀ | DTT005 | |
| EtOH | J.T.Baker Avantor | MFCD00003568 | |
| Extruder | Avestin Inc | LF-1 | |
| Fluorimeter | Jasco | Spectrofluorometer FP-8300 | |
| Glycerol | BOOM | 51171608 | |
| Gravity flow column | Bio-Rad | 732-1010 | |
| Hamilton syringe 100 ĀµL | Hamilton | 7656-01 | |
| Hamilton syringe 1000 ĀµL | Hamilton | 81320 | |
| Handheld LCP dispenser | Art Robbins Instruments | 620-411-00 | |
| Handheld Sonicator | Hielscher Ultrasound Technology | UP50H | |
| HCl | BOOM | x76021889.1000 | |
| Imidazole | Roth | X998.4-250g | |
| K2HPO4 | Supelco | 1.05099.1000 | |
| KCl | BOOM | 76028270.1 | |
| KH2PO4 | Supelco | 1.04873.1000 | |
| Kimwipe | Kimtech Science | 7552 | |
| Large Falcon tube centrifuge | Eppendorf | Centrifuge 5810 R | |
| L-Arginine | Sigma-Aldrich | A5006-100G | |
| Light microscope | Leica | DM LS2 | |
| L-Ornithine | Roth | T204.1 | |
| LSM Laser Scanning Confocal Microscope | Zeiss | LSM 710 ConfoCor 3 | |
| MgCl2 | Sigma-Aldrich | M2670-1KG | |
| Microfluidic chip | HomemadeĀ | PDMS based | DOI: https://doi.org/10.1039/C8LC01275J |
| Na-ADP | Sigma-Aldrich | A2754-1G | |
| NaCl | Supelco | 1.06404.1000 | |
| Nanodrop Spectrometer | Isogen Life Science | ND-1000 spectrophotometer NanoDrop | |
| NaOH | Supelco | 1.06498.1000 | |
| Needles for GUVs | Henke-Ject | 14-14575 | 27 G x 3/4'' 0.4 x 20 mm |
| Needles for microfluidics | Henke-Ject | 14-15538 | 18 G x 1 1/2'' 1.2 x 40 mm |
| Ni2+ Sepharose | Cytiva | 17526802 | |
| Nigericin | Sigma-Aldrich | N7143-5MG | |
| Nutator | VWR | 83007-210 | |
| Osmolality meter | Gonotec Salmenkipp | Osmomat 3000 basic freezing point osmometer | |
| Plasmacleaner | Plasma Etch | PE-Avenger | |
| Polycarbonate filter | Cytiva Whatman | Nuclepor Track-Etch Membrane Product: 10417104 | 0.4 Āµm |
| Polycarbonate ultracentrifuge tube | Beckman Coulter | 355647 | |
| Pyranine | Acros Organics | H1529-1G | |
| Quartz cuvette (black) | Hellma Analytics | 108B-10-40 | |
| Sephadex G-75 resinĀ | GE Healthcare | 17-0050-01 | |
| Sonicator | Sonics Sonics & Materials INC | Sonics vibra cell | |
| Syringe filter | Sarstedt | Filtropur S plus 0.2 | 0.2 Āµm |
| Syringe pump | Harvard Apparatus | A-42467 | |
| Tabletop centrifuge | Eppendorf | centrifuge 5418 | |
| Teflon spacer | HomemadeĀ | Teflon based | 45 x 26 x 1.5 or 45 x 26 x 3 or 20 x 20 x 3 mm |
| Tris | PanReac AppliChem | A1086.1000 | |
| Triton X-100 | Sigma Aldrich | T8787-100 ml | |
| Ultracentrifuge | Beckman Coulter | Optima Max-E | |
| UV lamp | Spectroline | ENB-280C/FE | |
| UV/VIS Spectrometer | Jasco | V730 spectrophotometer | |
| Valinomycin | Sigma-Aldrich | V0627-10MG | |
| Widefield fluorescence microscope | Zeiss | AxioObserver | |
| Ī²-Casein | Sigma Aldrich | C5890-500g |
References
- Hirschi, S., Ward, T. R., Meier, W. P., MĆ¼ller, D. J., Fotiadis, D. Synthetic biology: bottom-up assembly of molecular systems. Chem Rev. 122 (21), 16294-16328 (2022).
- Ivanov, I., et al. Bottom-up synthesis o....
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