Studying Nucleoid-Associated Protein-DNA Interactions Using Polymer Microgels as Synthetic Mimics

Microfluidically fabricated polymer microgels are used as an experimental platform to analyze protein-DNA interactions regulating bacterial cell division. In particular, we focused on the nucleoid-associated protein SlmA, which forms a nucleoprotein complex with short DNA binding sequences (SBS) that acts as a negative regulator of the division ring stability in Escherichia coli. To mimic the bacterial nucleoid as a dense DNA region of a bacterial cell and investigate the influence of charge and permeability on protein binding and diffusion in there, we have chosen nonionic polyethylene glycol and anionic hyaluronic acid as precursor materials for hydrogel formation, previously functionalized with SBS. SlmA binds specifically to the coupled SBS for both types of microgels while preferentially accumulating at the microgels' surface. We could control the binding specificity by adjusting the buffer composition of the DNA-functionalized microgels. The microgel charge did not impact protein binding; however, hyaluronic acid-based microgels exhibit a higher permeability, promoting protein diffusion; thus, they were the preferred choice for preparing nucleoid mimics. The approaches described here provide attractive tools for bottom-up reconstitution of essential cellular processes in media that more faithfully reproduce intracellular environments.

Automated summary

In this study, microfluidically fabricated polymer microgels were used as an experimental platform to analyze protein-DNA interactions that regulate bacterial cell division. By controlling the charge and permeability of the microgels, the researchers successfully mimicked the bacterial nucleoid and studied the binding and diffusion of proteins. These approaches provide attractive tools for reconstructing essential cellular processes in a more realistic intracellular environment.