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Abstract The composition of fluorescent polymer nanoparticles, commonly referred to as carbon dots, synthesized by microwave‐assisted reaction of citric acid and ethylenediamine was investigated by¹³C,¹³C{¹H},¹H─¹³C,¹³C{¹⁴N}, and¹⁵N solid‐state nuclear magnetic resonance (NMR) experiments.¹³C NMR with spectral editing provided no evidence for significant condensed aromatic or diamondoid carbon phases.¹⁵N NMR showed that the nanoparticle matrix has been polymerized by amide and some imide formation. Five small, resolved¹³C NMR peaks, including an unusual ═CH signal at 84 ppm (¹H chemical shift of 5.8 ppm) and ═CN₂at 155 ppm, and two distinctive¹⁵N NMR resonances near 80 and 160 ppm proved the presence of 5‐oxo‐1,2,3,5‐tetrahydroimidazo[1,2‐a]pyridine‐7‐carboxylic acid (IPCA) or its derivatives. This molecular fluorophore with conjugated double bonds, formed by a double cyclization reaction of citric acid and ethylenediamine as first shown by Y. Song, B. Yang, and coworkers in 2015, accounts for the fluorescence of the carbon dots. Cross‐peaks in a¹H─¹³C HETCOR spectrum with brief¹H spin diffusion proved that IPCA is finely dispersed in the polyamide matrix. From quantitative¹³C and¹⁵N NMR spectra, a high concentration (18 ± 2 wt%) of IPCA in the carbon dots was determined. A pronounced gradient in¹³C chemical‐shift perturbations and peak widths, with the broadest lines near the COO group of IPCA, indicated at least partial transformation of the carboxylic acid of IPCA by amide or ester formation. 

Abstract Metal film over nanosphere (FON) substrates are a mainstay of surface‐enhanced Raman scattering (SERS) measurements because they are inexpensive to fabricate, have predictable enhancement factors, and are relatively robust. This work includes a systematic investigation of how the three major FON fabrication parameters—nanosphere size, deposited metal thickness, and metal choice—impact the resulting localized surface plasmon resonance (LSPR). With these three parameters, it is quite simple to fabricate FONs with an optimal LSPR for SERS experiments with various excitation wavelengths. Some SERS experiments require that the substrates be incubated in organic solvents that have the potential to damage the substrate; as such, this work also explores how solvent incubation impacts the physical and optical properties of the FON substrate. Although no significant increase in physical damage is obvious, the LSPR does shift significantly. Finally, these optimized FONs were employed for the sensing of an important allergen, soybean agglutinin. The FONs were modified with a glycopolymer that has affinity for soybean agglutinin and clear Raman bands demonstrate detection of 10 μg/ml soybean agglutinin. Overall, this work serves the dual purpose of both sharing critical details about FON design and demonstrating detection of an important lectin analyte. 

Abstract Cryopreservation technology allows long‐term banking of biological systems. However, a major challenge to cryopreserving organs remains in the rewarming of large volumes (>3 mL), where mechanical stress and ice formation during convective warming cause severe damage. Nanowarming technology presents a promising solution to rewarm organs rapidly and uniformly via inductive heating of magnetic nanoparticles (IONPs) preloaded by perfusion into the organ vasculature. This use requires the IONPs to be produced at scale, heat quickly, be nontoxic, remain stable in cryoprotective agents (CPAs), and be washed out easily after nanowarming. Nanowarming of cells and blood vessels using a mesoporous silica‐coated iron oxide nanoparticle (msIONP) in VS55, a common CPA, has been previously demonstrated. However, production of msIONPs is a lengthy, multistep process and provides only mg Fe per batch. Here, a new microporous silica‐coated iron oxide nanoparticle (sIONP) that can be produced in as little as 1 d while scaling up to 1.4 g Fe per batch is presented. sIONP high heating, biocompatibility, and stability in VS55 is also verified, and the ability to perfusion load and washout sIONPs from a rat kidney as evidenced by advanced imaging and ICP‐OES is demonstrated.