Phospholipid bilayer nanodiscs: a powerful tool to study the structural organization and biochemical reactivity of proteins in membrane-like environments.

Nanodiscs are disc-like structures formed by two copies of a membrane scaffold protein, engineered from apolipoprotein A-I, surrounding a phospholipid mixture that can incorporate membrane proteins preserving their natural properties. They behave as soluble entities allowing the use of high-resolution structural techniques to determine the structural organization of the embedded membrane protein, and the use of solution biochemical-biophysical tools to measure its activity, assembly and interactions with other proteins in membranelike environments. In addition, nanodiscs are biocompatible which makes them an attractive technology to be used in therapy, drug discovery, and other biotechnological applications.

MinC protein shortens FtsZ protofilaments by preferentially interacting with GDP-bound subunits.

The interaction of MinC with FtsZ and its effects on FtsZ polymerization were studied under close to physiological conditions by a combination of biophysical methods. The Min system is a widely conserved mechanism in bacteria that ensures the correct placement of the division machinery at midcell. MinC is the component of this system that effectively interacts with FtsZ and inhibits the formation of the Z-ring. Here we report that MinC produces a concentration-dependent reduction in the size of GTP-induced FtsZ protofilaments (FtsZ-GTP) as demonstrated by analytical ultracentrifugation, dynamic light scattering, fluorescence correlation spectroscopy, and electron microscopy. Our experiments show that, despite being shorter, FtsZ protofilaments maintain their narrow distribution in size in the presence of MinC. The protein had the same effect regardless of its addition prior to or after FtsZ polymerization. Fluorescence anisotropy measurements indicated that MinC bound to FtsZ-GDP with a moderate affinity (apparent KD ∼10 µM at 100 mm KCl and pH 7.5) very close to the MinC concentration corresponding to the midpoint of the inhibition of FtsZ assembly. Only marginal binding of MinC to FtsZ-GTP protofilaments was observed by analytical ultracentrifugation and fluorescence correlation spectroscopy. Remarkably, MinC effects on FtsZ-GTP protofilaments and binding affinity to FtsZ-GDP were strongly dependent on ionic strength, being severely reduced at 500 mM KCl compared with 100 mM KCl. Our results support a mechanism in which MinC interacts with FtsZ-GDP, resulting in smaller protofilaments of defined size and having the same effect on both preassembled and growing FtsZ protofilaments.

Reconstitution of the Escherichia coli cell division ZipA-FtsZ complexes in nanodiscs as revealed by electron microscopy.

ZipA is an element of the bacterial division ring complex that provides an anchor to the membrane to FtsZ, a GTPase ancestor of tubulin. In vitro reconstitution and characterization of these interactions is challenged by the difficulty to integrate a physiological membrane environment. Here a single copy of the full-length ZipA protein from Escherichia coli incorporated into phospholipid bilayer nanodiscs (Nd-ZipA) has been visualized using negative-staining electron microscopy (EM). The EM images reveal the presence of discs, mostly organized in two distinct populations of 11 and 13nm in diameter. The globular FtsZ-binding C-terminal domain of ZipA (ZBD) was not visible in 3D reconstructions of Nd-ZipA or 2D averages, suggesting that this domain is separated from the membrane by the large flexible domain connecting the N-terminal trans-membrane region to the ZBD. We tested if Nd-ZipA were appropriate models for the in vitro reconstitution of ZipA-FtsZ interactions. First we observed that the ZBD region of ZipA was accessible for the interaction with other proteins in the context of the nanodisc, as revealed by its recognition by specific antibodies. In addition, Nd-ZipA attached to carbon coated EM grids, but not empty nanodiscs, were able to capture FtsZ filaments without inducing significant filament bundling, consistent with a model in which FtsZ filaments are loosely attached to the cell-membrane. These observations are compatible with the plastic nature of the ZipA-FtsZ complexes formed at the membrane, evidenced in the moderate binding affinity of Nd-ZipA to FtsZ oligomers and polymers recently measured.