Mark Bathe

A primer to scaffolded DNA origami

Molecular self-assembly with scaffolded DNA origami enables building custom-shaped nanometer-scale objects with molecular weights in the megadalton regime. Here we provide a practical guide for design and assembly of scaffolded DNA origami objects. We also introduce a computational tool for predicting the structure of DNA origami objects and provide information on the conditions under which DNA origami objects can be expected to maintain their structure.

A fluid--structure interaction finite element analysis of pulsatile blood flow through a compliant stenotic artery

A new model is used to analyze the fully coupled problem of pulsatile blood flow through a compliant, axisymmetric stenotic artery using the finite element method. The model uses large displacement and large strain theory for the solid, and the full Navier-Stokes equations for the fluid. The effect of increasing area reduction on fluid dynamic and structural stresses is presented. Results show that pressure drop, peak wall shear stress, and maximum principal stress in the lesion all increase dramatically as the area reduction in the stenosis is increased from 51 to 89 percent. Further reductions in stenosis cross-sectional area, however, produce relatively little additional change in these parameters due to a concomitant reduction in flow rate caused by the losses in the constriction. Inner wall hoop stretch amplitude just distal to the stenosis also increases with increasing stenosis severity, as downstream pressures are reduced to a physiological minimum. The contraction of the artery distal to the stenosis generates a significant compressive stress on the downstream shoulder of the lesion. Dynamic narrowing of the stenosis is also seen, further augmenting area constriction at times of peak flow. Pressure drop results are found to compare well to an experimentally based theoretical curve, despite the assumption of laminar flow.

Quantitative prediction of 3D solution shape and flexibility of nucleic acid nanostructures

DNA nanotechnology enables the programmed synthesis of intricate nanometer-scale structures for diverse applications in materials and biological science. Precise control over the 3D solution shape and mechanical flexibility of target designs is important to achieve desired functionality. Because experimental validation of designed nanostructures is time-consuming and cost-intensive, predictive physical models of nanostructure shape and flexibility have the capacity to enhance dramatically the design process. Here, we significantly extend and experimentally validate a computational modeling framework for DNA origami previously presented as CanDo [Castro,C.E., Kilchherr,F., Kim,D.-N., Shiao,E.L., Wauer,T., Wortmann,P., Bathe,M., Dietz,H. (2011) A primer to scaffolded DNA origami. Nat. Meth., 8, 221–229.]. 3D solution shape and flexibility are predicted from basepair connectivity maps now accounting for nicks in the DNA double helix, entropic elasticity of single-stranded DNA, and distant crossovers required to model wireframe structures, in addition to previous modeling (Castro,C.E., et al.) that accounted only for the canonical twist, bend and stretch stiffness of double-helical DNA domains. Systematic experimental validation of nanostructure flexibility mediated by internal crossover density probed using a 32-helix DNA bundle demonstrates for the first time that our model not only predicts the 3D solution shape of complex DNA nanostructures but also their mechanical flexibility. Thus, our model represents an important advance in the quantitative understanding of DNA-based nanostructure shape and flexibility, and we anticipate that this model will increase significantly the number and variety of synthetic nanostructures designed using nucleic acids.

Casting inorganic structures with DNA molds.

Introduction The ability to manufacture inorganic nanoparticles (NPs) with arbitrarily prescribed three-dimensional (3D) shapes and positional surface modifications is essential to enabling diverse applications (e.g., in nano-optics and biosensing). However, it is challenging to achieve 3D arbitrary user-specified shapes with sub–5-nm resolution. Top-down lithography has limited resolution, particularly for 3D shapes; capping ligands can be used to tune the energy difference of selected crystallographic facets, but typically only for highly symmetric shapes with identical surface facets. Casting metal particles with prescribed 3D shapes using programmable DNA nanostructure molds. (Top) Schematic of computational shape-by-design framework to encode the user-specified 3D shape of an inorganic particle in the linear sequences of DNA. (Middle) Assembly of the mold and casting growth of the metal particle. (Bottom) Experimental characterization of cast products (transmission electron micrographs; scale bars, 20 nm). Rationale We developed a framework to program arbitrary 3D inorganic NPs using DNA, which serves both as an informational “genome” to encode the 3D shape of a NP and as a physical “fabricator” to retrieve the information and execute the instruction to manufacture the NP. Specifically, our method uses a computationally designed, mechanically stiff synthetic DNA nanostructure with a user-specified cavity as a “mold” to cast the target inorganic NP. The mold encloses a small gold (Au) “seed.” Under mild conditions, the Au seed grows into a larger metal NP that fills the entire cavity, thereby replicating its prescribed 3D shape. The remaining DNA mold additionally acts as a spatially programmable functionalization surface. Results Using this DNA nanocasting method, we constructed three distinct sub–25-nm 3D cuboid silver (Ag) NPs with three independently tunable dimensions. The shape versatility of DNA-based nanocasting was further demonstrated via the synthesis of Ag NPs with equilateral triangular, right triangular, and circular cross sections. The material versatility was demonstrated via synthesis of a Au cuboid in addition to the Ag NPs. The DNA mold served as an addressable coating for the casted NP and thus enabled the construction of higher-order composite structures, including a Y-shaped Ag NP composite and a quantum dot (QD)–Ag-QD sandwiched structure through one-step casting growth. We investigated the key design parameters for stiff DNA molds through mechanical simulations. Multilayered DNA molds provided higher mechanical stiffness for confining NP growth within the mold than single-layer DNA molds, as confirmed by experimental observation. We additionally characterized plasmonic properties of the designer equilateral Ag triangle and Ag sphere through electron energy loss spectroscopy. Tuning of particle symmetry produced a shape-specific spectrum, which is consistent with the predictions of electromagnetism-based simulations. Conclusion DNA nanocasting represents a new framework for the programmable digital fabrication of 3D inorganic nanostructures with prescribed shapes, dimensions, and surface modifications at sub– 5-nm resolution. The key design strategy is to encode linear sequences of DNA with the sophisticated user-specified 3D spatial and surface information of an inorganic NP, as well as to retrieve and execute the information to physically produce this structure via geometric confinement. Such a method may lead to computationally designed functional materials for the digital manufacture of optical nanocircuits, electronic nanocomputers, and perhaps even sophisticated inorganic nanorobots, each with their blueprints (or “genomes’’) encoded in the DNA molecules that constitute their “nanofabricators.” Casting gold and silver with DNA origami Controlling the size and shape of nanoparticles synthesized in solution can be challenging, especially if the goal is to create less symmetric shapes for use in electronic and plasmonic applications. Sun et al. show that DNA “origami”—nanostructures in which the contacts between DNA strands are designed to assemble a particular shape—are sufficiently stiff to act as a mold for the growth of gold and silver nanostructures. The authors created shapes, including a gold particle with a rectangular cross section and a silver triangle with designed plasmonic properties. Science, this issue 10.1126/science.1258361 Shape-tunable metal nanoparticles form by replicating the hollow space inside designed DNA nanostructures. We report a general strategy for designing and synthesizing inorganic nanostructures with arbitrarily prescribed three-dimensional shapes. Computationally designed DNA strands self-assemble into a stiff “nanomold” that contains a user-specified three-dimensional cavity and encloses a nucleating gold “seed.” Under mild conditions, this seed grows into a larger cast structure that fills and thus replicates the cavity. We synthesized a variety of nanoparticles with 3-nanometer resolution: three distinct silver cuboids with three independently tunable dimensions, silver and gold nanoparticles with diverse cross sections, and composite structures with homo- and heterogeneous components. The designer equilateral silver triangular and spherical nanoparticles exhibited plasmonic properties consistent with electromagnetism-based simulations. Our framework is generalizable to more complex geometries and diverse inorganic materials, offering a range of applications in biosensing, photonics, and nanoelectronics.

Neutrophil Transit Times Through Pulmonary Capillaries : The Effects of Capillary Geometry and fMLP-stimulation

The deformations of neutrophils as they pass through the pulmonary microcirculation affect their transit time, their tendency to contact and interact with the endothelial surface, and potentially their degree of activation. Here we model the cell as a viscoelastic Maxwell material bounded by constant surface tension and simulate indentation experiments to quantify the effects of (N-formyl-L-methionyl-L-leucyl-L-phenylalanine (fMLP)-stimulation on its mechanical properties (elastic shear modulus and viscosity). We then simulate neutrophil transit through individual pulmonary capillary segments to determine the relative effects of capillary geometry and fMLP-stimulation on transit time. Indentation results indicate that neutrophil viscosity and shear modulus increase by factors of 3.4, for 10(-9) M fMLP, and 7.3, for 10(-6) M fMLP, over nonstimulated cell values, determined to be 30.8 Pa.s and 185 Pa, respectively. Capillary flow results indicate that capillary entrance radius of curvature has a significant effect on cell transit time, in addition to minimum capillary radius and neutrophil stimulation level. The relative effects of capillary geometry and fMLP on neutrophil transit time are presented as a simple dimensionless expression and their physiological significance is discussed.

Statistical mechanics of semiflexible bundles of wormlike polymer chains

We demonstrate that a semiflexible bundle of wormlike chains exhibits a state-dependent bending stiffness that alters fundamentally its scaling behavior with respect to the standard wormlike chain. We explore the equilibrium conformational and mechanical behavior of wormlike bundles in isolation, in cross-linked networks, and in solution.

A finite element framework for computation of protein normal modes and mechanical response.

A computational framework based on the Finite Element Method is presented to calculate the normal modes and mechanical response of proteins and their supramolecular assemblies. Motivated by elastic network models, proteins are treated as continuum elastic solids with molecular volume defined by their solvent‐excluded surface. The discretized Finite Element representation is obtained using a surface simplification algorithm that facilitates the generation of models of arbitrary prescribed spatial resolution. The procedure is applied to a mutant of T4 phage lysozyme, G‐actin, syntenin, cytochrome‐c′, beta‐tubulin, and the supramolecular assembly filamentous actin (F‐actin). Equilibrium thermal fluctuations of alpha‐carbon atoms and their inter‐residue correlations compare favorably with all‐atom‐based results, the Rotational‐Translational Block procedure, and experiment. Additionally, the free vibration and compressive buckling responses of F‐actin are in quantitative agreement with experiment. The proposed methodology is applicable to any protein or protein assembly and facilitates the incorporation of specific atomic‐level interactions, including aqueous‐electrolyte‐mediated electrostatic effects and solvent damping. The procedure is equally applicable to proteins with known atomic coordinates as it is to electron density maps of proteins, protein complexes, and supramolecular assemblies of unknown atomic structure. Proteins 2008.

Cytokinesis and the contractile ring in fission yeast: towards a systems-level understanding

Cytokinesis, the final stage of the cell division cycle, requires the proper placement, assembly and contraction of an actomyosin-based contractile ring. Conserved sets of cytokinesis proteins and pathways have now been identified and characterized functionally. Additionally, fluorescent protein fusion technology enables quantitative high-resolution imaging of protein dynamics in living cells. For these reasons, the study of cytokinesis is now ripe for quantitative, systems-level approaches. Here, we review our current understanding of the molecular mechanisms of contractile ring dynamics in the model organism Schizosaccharomyces pombe (fission yeast), focusing on recent examples that illustrate a synergistic integration of quantitative experimental data with computational modeling. A picture of a highly dynamic and integrated system consisting of overlapping networks is beginning to emerge, the detailed nature of which remains to be elucidated.

Structure, evolutionary conservation, and conformational dynamics of Homo sapiens fascin-1, an F-actin crosslinking protein.

Eukaryotes have several highly conserved actin-binding proteins that crosslink filamentous actin into compact ordered bundles present in distinct cytoskeletal processes, including microvilli, stereocilia and filopodia. Fascin is an actin-binding protein that is present predominantly in filopodia, which are believed to play a central role in normal and aberrant cell migration. An important outstanding question regards the molecular basis for the unique localization and functional properties of fascin compared with other actin crosslinking proteins. Here, we present the crystal structure of full-length Homo sapiens fascin-1, and examine its packing, conformational flexibility, and evolutionary sequence conservation. The structure reveals a novel arrangement of four tandem beta-trefoil domains that form a bi-lobed structure with approximate pseudo 2-fold symmetry. Each lobe has internal approximate pseudo 2-fold and pseudo 3-fold symmetry axes that are approximately perpendicular, with beta-hairpin triplets located symmetrically on opposite sides of each lobe that mutational data suggest are actin-binding domains. Sequence conservation analysis confirms the importance of hydrophobic core residues that stabilize the beta-trefoil fold, as well as interfacial residues that are likely to stabilize the overall fascin molecule. Sequence conservation also indicates highly conserved surface patches near the putative actin-binding domains of fascin, which conformational dynamics analysis suggests to be coupled via an allosteric mechanism that might have important functional implications for F-actin crosslinking by fascin.

Mapping translation 'hot-spots' in live cells by tracking single molecules of mRNA and ribosomes

Messenger RNA localization is important for cell motility by local protein translation. However, while single mRNAs can be imaged and their movements tracked in single cells, it has not yet been possible to determine whether these mRNAs are actively translating. Therefore, we imaged single β-actin mRNAs tagged with MS2 stem loops colocalizing with labeled ribosomes to determine when polysomes formed. A dataset of tracking information consisting of thousands of trajectories per cell demonstrated that mRNAs co-moving with ribosomes have significantly different diffusion properties from non-translating mRNAs that were exposed to translation inhibitors. These data indicate that ribosome load changes mRNA movement and therefore highly translating mRNAs move slower. Importantly, β-actin mRNA near focal adhesions exhibited sub-diffusive corralled movement characteristic of increased translation. This method can identify where ribosomes become engaged for local protein production and how spatial regulation of mRNA-protein interactions mediates cell directionality. DOI: http://dx.doi.org/10.7554/eLife.10415.001