Over the past decade, researchers have been working to create nanoscale materials and devices using DNA as construction materials through a process called DNA origami. A single long “sca old” strand of DNA can be folded into specific shapes by hundreds of shorter strands, for example. The order of bases in each short strand acts as a blueprint that dictates the sca old DNA’s final 3-D shape.

A collection of 120 3-D images of Bennett linkages. The images were created using individualparticle electron tomography (IPET), a technique developed at Berkeley Lab. (Image courtesy of Lawrence Berkeley National Laboratory)

Scientists hope to use this method to develop molecular devices that function as nanoscale machines, drug-delivery devices, markers for medical imaging or biological research, and components for electronic devices.

Long DNA sca olds – composed of more than 10,000 DNA structural units called nucleotides – have remained difficult to manufacture and manipulate, which has so far limited the size of the origami structures. It has also proven difficult to study the 3-D structure of these nanoparticles in their natural, flexible state.

Now, for the first time, a team of researchers from Lawrence Berkeley National Laboratory and Ohio State University have generated 3-D images from 129 individual molecules of flexible DNA origami particles. Their work provides the first experimental verification of the theoretical model of DNA origami.

The methods used here could easily be applied to other types of fabricated DNA origami structures, and help inform the design and optimization of future structures. The research team focused on DNA structures modeled after a basic mechanism called a “Bennett linkage,” which is a 3-D structure consisting of a chain of four rods connected by hinges. This creates a skewed quadrilateral shape in which the hinges are not parallel nor in-line. Using Bennett linkages as building blocks, it’s possible to create expandable, useful structures, like supports for tents that can be rapidly assembled.

DNA origami structures are challenging to study because they are very flexible and delicate, and each molecule has a unique 3-D shape. This variability makes conventional imaging methods, like single-particle cryoelectron microscopy (cryo-EM), less suitable. Cryo-EM involves extensive computer averaging from thousands to hundreds of thousands of similar molecules. As a result, information about the flexible portions of DNA origami structures can be easily averaged away, yielding an incomplete picture of the structure.

The researchers relied on a technique developed at Berkeley Lab’s Molecular Foundry, a research facility for nanoscale science, to image the individual molecules that make up these structures. The method, called individual-particle electron tomography (IPET), takes pictures of a target molecule from multiple viewing angles, and then combines these pictures to create one 3-D, whole-molecule rendering, similar to how a medical computed tomography (CT) scan works.

Researchers captured the 129 3-D images, with a resolution of 6 to 14 nanometers, which enabled them to tease out information about the dynamics and flexibility of the DNA origami structures. The reconstructions confirmed that Bennett linkages have a high degree of structural diversity.

A geometric analysis of these reconstructions showed that the conformations of Bennett linkage mechanisms are in good agreement with the theoretical models. When the linkages are near their “open” state, the “hinge” is almost fully extended. When the structures are nearer to their “closed” conformation, the structures take on different shapes and are extremely flexible and distorted.

Based on these results and the model visualizations of the Bennett linkages, the researchers will propose a new strategy for improving control of Bennett linkages in large DNA scaffolds. The approach includes redesigning the DNA sequences near the joints to stiffen the structure and prevent it from distorting.

For more information, Contact Glenn Roberts Jr. at 510-486-5582.