Monitoring mRNA and protein levels in bulk and in model vesicle-based artificial cells.

With rising interest in utilizing cell-free gene expression systems in bottom-up synthetic biology projects, novel labeling tools need to be developed to accurately report the dynamics and performance of the biosynthesis machinery operating in various reaction conditions. Monitoring the transcription activity has been simplified by the Spinach technology, an RNA aptamer that emits fluorescence upon binding to a small organic dye. Recently, we tracked the fluorescence of Spinach-tagged messenger RNA (mRNA) and its translation product the yellow fluorescent protein (YFP), both synthesized in the protein synthesis using recombinant elements system from a DNA template.

Toward the assembly of a minimal divisome.

The construction of an irreducible minimal cell having all essential attributes of a living system is one of the biggest challenges facing synthetic biology. One ubiquitous task accomplished by any living systems is the division of the cell envelope. Hence, the assembly of an elementary, albeit sufficient, molecular machinery that supports compartment division, is a crucial step towards the realization of self-reproducing artificial cells.

Unbiased tracking of the progression of mRNA and protein synthesis in bulk and in liposome-confined reactions.

The compartmentalization of a cell-free gene expression system inside a self-assembled lipid vesicle is envisioned as the simplest chassis for the construction of a minimal cell. Although crucial for its realization, quantitative understanding of the dynamics of gene expression in bulk and liposome-confined reactions is scarce. Here, we used two orthogonal fluorescence labeling tools to report the amounts of mRNA and protein produced in a reconstituted biosynthesis system, simultaneously and in real-time.

Linking genotype and phenotype in protein synthesizing liposomes with external supply of resources.

Reconstituting an elementary gene expression system inside self-assembled lipid vesicles to mimic the cellular synthesis machinery is at the core of the development of a minimal cell following a bottom-up synthetic biology approach. The ability to operate the expression of multiple genes in a controlled manner and to generate the output proteins with predictable dynamics in liposomes relies on the link between genotype and phenotype. Here, we established this link in surface-tethered liposomes producing proteins from a linear DNA template using a reconstituted transcription/translation/aminoacylation apparatus fuelled by external supply of feedstock.