Hydrogen Bonding Study of Quinoline and Coal-Derived Asphaltene Components with o-Phenylphenol by Proton Magnetic Resonance

Abstract

Proton magnetic resonance (PMR) studies are reported of hydrogen bonding between the OH proton of o-phenylphenol (OPP) and the nitrogen electron donor of quinoline (Qu). Data are also reported on the hydrogen bonding of a coal-derived asphaltene and its acid and base components with OPP. Determination was made of the equilibrium constants of the 1:1 complex between OPP and Qu at 39, 32, 1, and ?18°C from the PMR studies. Qualitative results are reported for the interaction between the base fraction of asphaltene and OPP at 32, 1, and ?26°C.     

Theoretical and spectroscopic study of 2-substituted indan-1,3-diones: a coherent picture of the tautomeric equilibrium

The structures of some 2-substituted indan-1,3-diones are investigated in the gas phase and solution using quantum chemical calculations and spectral (NMR, IR, and UV) measurements. The influence of the substituent at the 2-position on the tautomeric equilibrium of 2-substituted indan-1,3-diones in solvents with different polarity is evaluated. It is shown that the equilibrium in 2-formyl-indan-1,3-dione and 2-acetyl-indan-1,3-dione is shifted to the 2-hydroxyalkylidene-indan-1,3-dione tautomer, while 2-carboxyamide-indan-1,3-dione exists as a mixture of two tautomers, 2-(hydroxyaminomethylidene)-indan-1,3-dione and 2-carboamide-1-hydroxy-3-oxo-indan, with extremely fast proton transfer between them. The situation for 2-carboxy-indan-1,3-dione is quite different - on the basis of the analysis of the obtained results, the possible existence of an anionic form of 2-carboxy-indan-1,3-dione in solution can be inferred.     

Spectrophotometric Determination of Molybdenum(VI) as a Ternary Complex with 4-Nitrocatechol and Benzalkonium Chloride

A new liquid—liquid extraction system for molybdenum(VI) was studied. It contains 4-nitrocatechol (4NC) as a complexing chromogenic reagent and benzalkonium chloride (BZC) as a source of heavy cations (BZ⁺), which are prone to form chloroform-extractable ion-association complexes. The optimum conditions for the determination of trace molybdenum(VI) were found: concentrations of 4NC and BZC (7.5 × 10⁻⁴ mol dm⁻³ and 1.9 × 10⁻⁴ mol dm⁻³, respectively), acidity (3.75 × 10⁻² mol dm⁻³ H₂SO₄), extraction time (3 min), and wavelength (439 nm). The molar absorptivity, limit of detection, and linear working range were 5.5 × 10⁴ dm³ mol⁻¹ cm⁻¹, 5.6 ng cm⁻³, and 18.6–3100 μg cm⁻³, respectively. The effect of foreign ions was examined, and the developed procedure was applied to the analysis of synthetic mixtures and real samples (potable waters and steels). The composition of the extracted complex was 1:1:2 (Mo:4NC:BZ). Three possible structures of its anionic part [Mo^VI(4NC)O₂(OH)₂]²⁻ were discussed based on optimizations at the B3LYP/3-21G level of theory, and simulated UV/Vis absorption spectra were obtained with the TD Hamiltonian.     

From Lobry de Bruyn to enzyme-catalyzed ammonia channelling: molecular studies of D-glucosamine-6P synthase

This review summarizes the state of knowledge on D-glucosamine-6P synthesis catalyzed by glucosamine-6P synthase. The mechanisms of L-glutamine hydrolysis, ammonia transfer and fructose-6P conversion into D-glucosamine-6P are analyzed with the E. coli enzyme in light of recent X-ray structures. With 92 references this paper covers the literature up to June 2001 and emphasizes the potential implication of the mammalian glucosamine-6P synthase in type 2 diabetes.     

<Superscript>13</Superscript>C NMR and mass spectrometry of soil organic matter

Liquid state, high resolution ¹³C NMR spectroscopy and mass spectrometry were used to study the composition and structure of soil organic matter (SOM) using soil extracts from two long-term experiments at the Rothamsted Experimental Station. Both one- and two-dimensional NMR techniques were applied. ¹³C NMR sub-spectra of the CH _n (n=0...3) groups, obtained by the Distortionless Enhancement by Polarisation Transfer (DEPT) technique, were used for the elucidation of the qualitative and quantitative composition of humic and fulvic acids in the soils. The chemical structure of SOM was further analysed at the molecular level through Fast Atom Bombardment Mass Spectrometry (FABMS) and Gas Chromatography-Mass Spectrometry (GC/MS). Humic and fulvic extract results were not only compared to each other, but also to the solid state ¹³C NMR results for the complete soil sample.     

Multicolor polymeric carbon dots: synthesis,separation and polyamide-supported molecular fluorescence

Multicolor carbon dots (CDs) have been developed recently and demonstrate great potential in bio-imaging, sensing, and LEDs. However, the fluorescence mechanism of their tunable colors is still under debate, and efficient separation methods are still challenging. Herein, we synthesized multicolor polymeric CDs through solvothermal treatment of citric acid and urea in formamide. Automated reversed-phase column separation was used to achieve fractions with distinct colors, including blue, cyan, green, yellow, orange and red. This work explores the physicochemical properties and fluorescence origins of the red, green, and blue fractions in depth with combined experimental and computational methods. Three dominant fluorescence mechanism hypotheses were evaluated by comparing time-dependent density functional theory and molecular dynamics calculation results to measured characteristics. We find that blue fluorescence likely comes from embedded small molecules trapped in carbonaceous cages, while pyrene analogs are the most likely origin for emission at other wavelengths, especially in the red. Also important, upon interaction with live cells, different CD color fractions are trafficked to different sub-cellular locations. Super-resolution imaging shows that the blue CDs were found in a variety of organelles, such as mitochondria and lysosomes, while the red CDs were primarily localized in lysosomes. These findings significantly advance our understanding of the photoluminescence mechanism of multicolor CDs and help to guide future design and applications of these promising nanomaterials.

Understanding the origin and sensitivity of carbon dot emission will improve their utility in various applications.

Since the accidental discovery of luminescent carbon fragments in 2004,¹ carbon dots (CDs) have attracted great research interest due to the diverse synthetic methods, tunable luminescence, and applicability in a broad range of fields, including bio-imaging,^2–4 sensing,^5,6 and light emitting diodes (LEDs).^7,8 Typically, CDs are fluorescent carbon nanostructures of sizes less than 10 nm, composed of carbon, oxygen, and nitrogen.^9–12 CDs can be produced through bottom-up methods, which involve small molecular precursors like citric acid, malic acid, urea, ethylenediamine, and so on.^13–15 In a high temperature reaction, polymerization and dehydration occur among various functional groups, and the resulting products are usually a mixture of small molecule residues, oligomers, and long chain polymers.¹⁶ The unclear fluorescence mechanisms and poorly understood internal structure of CDs limit the ability to understand, tune, and fully exploit their fluorescence properties.Fortunately, in recent years, breakthrough syntheses of multicolor CDs have been achieved.^17–19 Several different multicolor CDs have been synthesized with aromatic compounds such as phenylenediamine.^4,20–22 However, it should be noted that precursors such as aniline and phenol may have toxic effects on human health and the environment,^23,24 and thus should be avoided where possible. Syntheses of colorful CDs from non-aromatic compounds such as citric acid and urea often employ solvothermal methods. Utilizing different solvents such as formamide and dimethylformamide have been shown to play a significant role in tuning CD emission.^25,26 In addition, chromatographic post-treatment of as-made CDs plays a critical role in obtaining different colored fractions, using techniques such as anion-exchange column chromatography,²⁶ normal phase silica chromatography,²⁷ and reversed phase silica chromatography.¹⁵ Compared with high performance liquid chromatography (HPLC), the aforementioned column chromatography techniques help to separate CDs on a larger scale. These separations are based on charge²⁶ or polarity,²¹ and are efficient in isolating the desired fractions with distinct colors so that detailed structural characterization can be performed.To gain insight into the fluorescence mechanism of these multicolor CDs, researchers have considered three hypotheses: quantum size effects,²⁸ the inclusion of molecular fluorophores,²⁹ and surface state-induced emission.³⁰ For example, Rogach and coworkers developed solid-state CDs with tunable fluorescence via the seeded growth method. They attributed the tunable emission to the size of π-conjugated domains.³¹ Yang and coworkers synthesized CDs by hydrothermal treatment of citric acid and ethylenediamine. They identified a small molecule fluorophore, IPCA (1,2,3,5-tetrahydro-5-oxo-imidazo[1,2-α]pyridiine-7-carboxylic acid) from CD column separation fractions, which contributed to the blue fluorescence.¹³ Xiong and coworkers synthesized CDs from urea and p-phenylenediamine that emitted a range of colors and separated them with silica column chromatography. They found the degree of carbon oxidation increased as the emission redshifted and thus, they endorsed the surface state hypothesis.²¹ In addition to the above mechanisms, computational methods such as density functional theory (DFT) have also been applied to analyze the fluorescence origins of CDs. The charge transfer between functional groups on the polymeric unit of CDs made from citric acid and ethylenediamine was found to facilitate blue emission.¹⁶The goal of present work is to understand the fluorescence origin of multicolor CDs. The model multicolor CDs were obtained by reacting citric acid and urea in formamide via a microwave-assisted hydrothermal treatment. An automated chromatographic apparatus was employed to separate as-made CD mixtures into distinct color fractions. The individual separation process took around 20 minutes, and the obtained CD fractions exhibit discrete illumination-induced emission throughout the visible region of the spectrum. Interestingly, the sizes of separated CD fractions are not statistically different from one another, suggesting that the quantum size effects are not the source of differential emission. Solvatochromism experiments showed that the blue and green fractions have similar fluorescence behavior as a function of solvent polarity, but the red fraction behaved differently. Using computational simulations, three models of the fluorescence origin were constructed and evaluated, showing that the formation of small blue fluorescent molecules is likely and pyrene analogs could be the origins for various emission colors. Moreover, two representative CD fractions, the blue- and red-emitting fractions, were chosen for subsequent cell imaging experiments. The localization pattern for the CD fractions differed: blue-emitting CDs were observed in a wide range of organelles, while red-emitting CDs were primarily enclosed in lysosomes. Understanding the origin and the sensitivity of CD emission will improve their utility in bioimaging applications.