Enzymatic Regulation of Protein–Protein Interactions in Artificial Cells

Veldhuisen, Thijs W van; Altenburg, Wiggert J.; Verwiel, Madelief A M; Lemmens, Lenne J M; Mason, Alexander F.; Merkx, Maarten; Brunsveld, Luc; Hest, Jan C. M. van

doi:10.1002/adma.202300947

Cited by 6 publications

(4 citation statements)

References 52 publications

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“…1 ). This local concentration represents a 350-fold enhancement of concentration compared to the bulk concentration of 100 nM and is comparable to the 14-3-3 loading that was determined in our previous work 26 . The fluorescein isothiocyanate (FITC)-labeled bivalent c-Raf pS233/pS259 (c-Raf pS) client peptide was added to the separate populations of coacervates at a concentration of 25 nM yielding a 14-3-3/c-Raf pS binding site ratio of 2:1 (Fig.…”

Section: Resultssupporting

confidence: 86%

“…Although we have previously used a bioluminescence assay for PPIs in coacervates 26 , confocal microscopy is more suited for determining the localization of a client in a multi-population coacervate sample over time since it additionally provides spatial information and is not enzyme substrate-dependent. Confocal micrographs of the single population coacervates with the different 14-3-3 isoforms showed that, indeed, similar recruitment levels of c-Raf pS were observed after overnight incubation (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…Exchange or recruitment of client proteins in synthetic cells can also be governed by protein-protein interactions (PPIs) 23 – 27 . For us, in particular interactions of client proteins with the hub protein 14-3-3, a native protein which is important for the regulation of many signaling pathways 28 , 29 , yielded specific uptake based on affinity for 14-3-3 26 . 14-3-3 generally binds to serine/threonine phosphorylated client proteins, although there are also examples of nonphosphorylated binding motifs in client proteins, such as the 14-3-3-binding motif of the bacterial toxin Exoenzyme S 30 , 31 .…”

Section: Introductionmentioning

confidence: 99%

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Competitive protein recruitment in artificial cells

van Veldhuisen,

Verwiel,

Novosedlik

et al. 2024

Commun Chem

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Living cells can modulate their response to environmental cues by changing their sensitivities for molecular signals. Artificial cells are promising model platforms to study intercellular communication, but populations with such differentiated behavior remain underexplored. Here, we show the affinity-regulated exchange of proteins in distinct populations of coacervate-based artificial cells via protein-protein interactions (PPI) of the hub protein 14-3-3. By loading different coacervates with different isoforms of 14-3-3, featuring varying PPI affinities, a client peptide is directed to the more strongly recruiting coacervates. By switching affinity of client proteins through phosphorylation, weaker binding partners can be outcompeted for their 14-3-3 binding, inducing their release from artificial cells. Combined, a communication system between coacervates is constructed, which leads to the transport of client proteins from strongly recruiting coacervates to weakly recruiting ones. The results demonstrate that affinity engineering and competitive binding can provide directed protein uptake and exchange between artificial cells.

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Section: Resultssupporting

confidence: 86%

Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Competitive protein recruitment in artificial cells

van Veldhuisen,

Verwiel,

Novosedlik

et al. 2024

Commun Chem

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“…Consequently, the incorporation of proteins into synthetic vesicles has attracted massive attention for advanced biological applications, including drug delivery vehicles 21 and artificial cell platforms. 22,23…”

Section: Introductionmentioning

confidence: 99%

Rational design and engineering of polypeptide/protein vesicles for advanced biological applications

Shin

Jang

2023

J. Mater. Chem. B

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Spatiotemporal Control Over Protein Release from Artificial Cells via a Light‐Activatable Protease

Hazegh Nikroo,

Altenburg,

van Veldhuisen

et al. 2024

Advanced Biology

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The regulation of protein uptake and secretion by cells is paramount for intercellular signaling and complex multicellular behavior. Mimicking protein‐mediated communication in artificial cells holds great promise to elucidate the underlying working principles, but remains challenging without the stimulus‐responsive regulatory machinery of living cells. Therefore, systems to precisely control when and where protein release occurs should be incorporated in artificial cells. Here, a light‐activatable TEV protease (LaTEV) is presented that enables spatiotemporal control over protein release from a coacervate‐based artificial cell platform. Due to the presence of Ni2+‐nitrilotriacetic acid moieties within the coacervates, His‐tagged proteins are effectively sequestered into the coacervates. LaTEV is first photocaged, effectively blocking its activity. Upon activation by irradiation with 365 nm light, LaTEV cleaves the His‐tags from sequestered cargo proteins, resulting in their release. The successful blocking and activation of LaTEV provides control over protein release rate and triggerable protein release from specific coacervates via selective irradiation. Furthermore, light‐activated directional transfer of proteins between two artificial cell populations is demonstrated. Overall, this system opens up avenues to engineer light‐responsive protein‐mediated communication in artificial cell context, which can advance the probing of intercellular signaling and the development of protein delivery platforms.

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Enzymatic Regulation of Protein–Protein Interactions in Artificial Cells

Cited by 6 publications

References 52 publications

Competitive protein recruitment in artificial cells

Competitive protein recruitment in artificial cells

Rational design and engineering of polypeptide/protein vesicles for advanced biological applications

Spatiotemporal Control Over Protein Release from Artificial Cells via a Light‐Activatable Protease

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