| Literature DB >> 31075444 |
Bryan Ferlez1, Markus Sutter2, Cheryl A Kerfeld3.
Abstract
Microbes often augment their metabolism by conditionally constructing proteinaceous organelles, known as bacterial microcompartments (BMCs), that encapsulate enzymes to degrade organic compounds or assimilate CO2. BMCs self-assemble and are spatially delimited by a semi-permeable shell made up of hexameric, trimeric, and pentameric shell proteins. Bioengineers aim to recapitulate the organization and efficiency of these complex biological architectures by redesigning the shell to incorporate non-native enzymes from biotechnologically relevant pathways. To meet this challenge, a diverse set of synthetic biology tools are required, including methods to manipulate the properties of the shell as well as target and organize cargo encapsulation. We designed and determined the crystal structure of a synthetic shell protein building block with an inverted sidedness of its N- and C-terminal residues relative to its natural counterpart; the inversion targets genetically fused protein cargo to the lumen of the shell. Moreover, the titer of fluorescent protein cargo encapsulated using this strategy is controllable using an inducible tetracycline promoter. These results expand the available set of building blocks for precision engineering of BMC-based nanoreactors and are compatible with orthogonal methods which will facilitate the installation and organization of multi-enzyme pathways.Entities:
Keywords: Bacterial microcompartments; Metabolic engineering; Protein design; Synthetic biology
Mesh:
Substances:
Year: 2019 PMID: 31075444 PMCID: PMC6884132 DOI: 10.1016/j.ymben.2019.04.011
Source DB: PubMed Journal: Metab Eng ISSN: 1096-7176 Impact factor: 9.783