Terpene cyclizations are one of the most complex reactions that occur in nature. Scientists have found that replicating this reaction in a lab setting has proved to be immensely challenging as result of the numerous intermediates that must be controlled through the cyclization process in the absence of an enzyme. This study uses commercially available lipases to conduct reactions with geraniol-derived starting materials to identify conditions for performing a terpene cyclization effectively and efficiently. Through hypothesized screening of enzymes and reaction conditions, we have identified a protocol for the successful cyclization of limonene and other geranyl-derived products.

A form of nanoscale steganography exists described as DNA origami cryptography which is a technique of secure information encryption through scaffold, staple, and varying docking strand self- assembling mixtures. The all-DNA steganography based origami was imaged through high-speed DNA-PAINT super-resolution imaging which uses periodic docking sequences to eliminate the need for protein binding. The purpose of this research was to improve upon the DNA origami cryptography protocol by encrypting information in 2D Rothemund Rectangular DNA Origami (RRO) and 3D cuboctahedron DNA origami as a platform of self-assembling DNA nanostructures to increase the routing possibilities of the scaffold. The initial focus of the work was increasing the incorporation efficiency of all individual docking spots for full 20nm grid RRO pattern readout. Due to this procedural optimization was pursued by altering annealing cycle length, centrifugal spin rates for purification, and lengthening docking strands vs. imager poly T linkers. A 14nm grid was explored as an intermediate prior to the 10nm grid for comparison of optimized experimental procedure for a higher density encryption pattern option. Imager concentration was discovered to be a vital determining factor in effectively resolving the 10nm grids due to high concentrations of imager strands inducing simultaneous blinking of adjacent docking strands to be more likely causing the 10nm grids to not be resolved. A 2 redundancy and 3 redundancy encryption scheme was developed for the 10nm grid RRO to be encrypted with. Further experimentation was completed to resolve full 10nm DNA-origami grids and encrypt with the message ”ASU”. The message was successfully encrypted and resolved through the high density 10nm grid with 2 and 3 redundancy patterns. A cuboctahedron 3D origami was explored with DNA-PAINT techniques as well resulting in successful resolution of the z-axis through variation of biotin linker length and calibration file. Positive results for short message ”0407” encryption of the cuboctahedron were achieved. Data encryption in DNA origami is further being explored and could be an optimal solution for higher density data storage with greater longevity of media.

With climate change threatening to increase the frequency of global pandemics, the need for quick and adaptable responses to novel viruses will become paramount. DNA nanotechnology offers a highly customizable, biocompatible approach to combating novel outbreaks. For any DNA nanotechnology-based therapeutic to have future success in vivo, the structure must be able to withstand serological conditions for an extended time period. In this study, the stability of a wireframe DNA snub cube with attached nbGFP used to bind a nonessential viral epitope on Pseudorabies virus is evaluated in vitro both with and without one of two modifications designed to enhance stability: 1) the use of trivalent spermidine cations during thermal annealing of the nanostructure, and 2) the introduction of a polylysine-polyethylene glycol coating to the conjugated nanostructure. The design, synthesis, and purification of the multivalent inhibitor were also evaluated and optimized. Without modification, the snub cube nanostructure was stable for up to 8 hours in culture media supplemented with 10% FBS. The spermidine-annealed nanostructures demonstrated lesser degrees of stability and greater degradation than the unmodified structures, whereas the polylysine-coated structures demonstrated equivalent stability at lower valencies and enhanced stability at the highest valency of the snub cube inhibitor. These results support the potential for the polylysine-polyethylene glycol coating as a potential method for enhancing the stability of the snub cube for future in vivo applications.

This qualitative study sought to investigate the potential reaction between the 3,3',5,5'-tetramethylbenzidine (TMB) radical and LAF-1 RGG, the N-terminus domain of an RNA helicase which functions as a coacervating intrinsically disordered protein. The study was performed by adding horseradish peroxidase to a solution containing TMB and either LAF-1 or tyrosine in various concentrations, and monitoring the output through UV-Vis spectroscopy. The reacted species was also analyzed via MALDI-TOF mass spectrometry. UV-Vis spectroscopic monitoring showed that in the presence of LAF-1 or tyrosine, the reaction between HRP and TMB occurred more quickly than the control, as well as in the highest concentration of LAF-1, the evolution of a peak at 482 nm. The analysis through MALDI-TOF spectrometry showed the development of a second peak likely due to the reaction between LAF-1 and TMB, as the Δ between the peaks is 229 Da and the size of the TMB species is 240 Da.