One step visual detection of PCR products with gold nanoparticles and a nucleic acid lateral flow (NALF) device

Specific PCR products are detected with an antibody-free lateral-flow device by sandwiching them between reporter oligonucleotides covalently attached to gold nanoparticles (GNPs) and capture oligonucleotides covalently attached to a nitrocellulose chromatographic strip.     

共价嫁接Ru(Ⅱ)配合物杂化材料的制备及氧气传感性能研究

利用十六烷基三甲基溴化铵制备了一种具有MSU型蠕虫状孔道结构, 同时共价嫁接了Ru(Ⅱ)配合物的介孔杂化功能材料, 并研究了其氧气传感性能. 双功能有机改性硅酸酯Bpy-Si不仅是配合物Ru(bpy)2Cl2·2H2O的一个配体, 而且通过与正硅酸乙酯的水解和共聚反应, 把Ru(bpy)2(bpy-Si)Cl2配合物通过Si—C共价键嫁接到二氧化硅的骨架上. 研究结果表明, Ru(Ⅱ)分子在杂化材料中的发光受氧气猝灭明显, 而且具有较快的响应时间, 所得材料具有作为性能优良的氧气传感材料研究的潜质. 由于介孔材料的独特孔道结构有利于氧气在载体中的扩散, 介孔样品表现出比无定形样品更高的灵敏度.     

Two-dimensional optimization using different pairs of variables for the reversed-phase high-performance liquid chromatographic separation of a mixture of acidic compounds

A cryptand-based anion exchanger has been developed in which the capacity and to a lesser degree, selectivity are adjustable simply by the choice of the mobile phase. Although much work has been done in the past using cryptand-based anion exchangers, these stationary phases were based on adsorbed cryptands rather than covalently bound cryptands. These phases suffered from the usual problems associated with adsorbed systems. A novel styrene-based cryptand has been synthesized which can be covalently attached to a solid support. A brief review of cryptands and binding constants as well as comparisons of adsorbed phases versus covalently bound phases will be discussed. Some of the unique chromatographic properties of this prototype column will be illustrated as well.     

Novel covalently coated diazoresin/polyvinyl alcohol capillary column for the analysis of proteins by capillary electrophoresis

A novel method for the preparation of covalently linked capillary coatings of PVA was demonstrated using photosensitive diazoresin (DR) as coupling agents. Layer‐by‐layer self‐assembly film of DR and PVA based on hydrogen bonding was first fabricated on the inner wall of capillary, then the hydrogen bonding was converted into covalent bonding after treatment with UV light through the unique photochemistry reaction of DR. The covalently bonded coatings suppressed basic protein adsorption on the inner surface of capillary, and thus a baseline separation of lysozyme, cytochrome c and BSA was achieved using CE. Compared with bare capillary or noncovalently bonded DR/PVA coatings, the covalently linked DR/PVA capillary coatings not only improved the CE separation performance for proteins, but also exhibited good stability and repeatability. Due to the replacement of highly toxic and moisture‐sensitive silane coupling agent by DR in the covalent coating preparation, this method may provide a green and easy way to make the covalently coated capillaries for CE.     

Affinity Covalent Immobilization of Glucoamylase onto ρ-Benzoquinone-Activated Alginate Beads: II. Enzyme Immobilization and Characterization

A novel affinity covalent immobilization technique of glucoamylase enzyme onto ρ-benzoquinone-activated alginate beads was presented and compared with traditional entrapment one. Factors affecting the immobilization process such as enzyme concentration, alginate concentration, calcium chloride concentration, cross-linking time, and temperature were studied. No shift in the optimum temperature and pH of immobilized enzymes was observed. In addition, K _m values of free and entrapped glucoamylase were found to be almost identical, while the covalently immobilized enzyme shows the lowest affinity for substrate. In accordance, V _m value of covalently immobilized enzyme was found lowest among free and immobilized counter parts. On the other hand, the retained activity of covalently immobilized glucoamylase has been improved and was found higher than that of entrapped one. Finally, the industrial applicability of covalently immobilized glucoamylase has been investigated through monitoring both shelf and operational stability characters. The covalently immobilized enzyme kept its activity over 36 days of shelf storage and after 30 repeated use runs. Drying the catalytic beads greatly reduced its activity in the beginning but recovered its lost part during use. In general, the newly developed affinity covalent immobilization technique of glucoamylase onto ρ-benzoquinone-activated alginate carrier is simple yet effective and could be used for the immobilization of some other enzymes especially amylases.     

A novel diazoresin/poly(N‐vinyl aminobutyric acid) covalent capillary coating for the analysis of proteins by capillary electrophoresis

A novel method for the preparation of covalently linked capillary coatings of poly(N‐vinyl aminobutyric acid) (PVAA) obtained from hydrolyzed polyvinylpyrrolidone was demonstrated using photosensitive diazoresin (DR) as a coupling agent. A layer‐by‐layer self‐assembled film of DR and PVAA based on ionic bonding was first fabricated on the inner wall of capillary, then ionic bonding was converted into covalent bonding after treatment with UV light through a unique photochemical reaction of DR. The covalently bonded coatings suppressed protein adsorption on the inner surface of the capillary, and thus a baseline separation of lysozyme, cytochrome c, BSA, amyloglucosidase, and myoglobin was achieved using CE. Compared with bare capillary or noncovalently bonded DR/PVAA coatings, the covalently linked DR/PVAA capillary coatings not only improved the CE separation performance for proteins, but also exhibited good stability and repeatability. Due to the replacement of the highly toxic and moisture‐sensitive silane coupling agent by DR in the covalent coating preparation, this method may provide a green and easy way to make covalently coated capillaries for CE.     

Direct electron transfer in immobilized flavoenzyme chemically modified graphite electrodes

Direct electron transfer between covalently immobilized flavoenzymes and a cyanuric chloride-modified graphite electrode is observed via differential pulse voltammetry. L-Amino acid oxidase and xanthine oxidase display peaks arising from the reduction of flavin adenine dinucleotide. Peak current enhancements are observed for both covalently attached enzymes compared to their free and adsorbed state voltammograms. Studies concerning flavin removal and reconstitution indicate that xanthine oxidase contains multiple flavin chromophores which are nonequivalent.     

Covalent VEGF protein immobilization on resorbable polymeric surfaces

Vascular endothelial growth factor type protein (VEGF), a potent angiogenic effector molecule, was successfully covalently immobilized onto the surfaces of the resorbable polymers poly(L‐lactic acid) (PLLA) and poly(ε‐caprolactone) (PCL) through a three‐step strategy. The surfaces were first covalently grafted with poly(acrylic acid) using non‐destructive and solvent free vapor‐phase grafting. A diamine spacer was coupled to the carboxylic acid pendant groups on the graft chains using EDC/NHS chemistry and VEGF was finally covalently attached to the amine linkers. The chemistry and topography of the modified substrates were quantitatively and qualitatively verified with XPS, ATR‐FTIR, UV–VIS, SEM, and ELISA. Copyright © 2010 John Wiley & Sons, Ltd.     

Unprecedented covalently attached ATRP initiator onto OH-functionalized mica surfaces

Mica substrates were activated by a plasma method leading to OH-functionalized surfaces to which an atom transfer radical polymerization (ATRP) radical initiator was covalently bound using standard siloxane protocols. The unprecedented covalently immobilized initiator underwent radical polymerization with tert-butyl acrylate, yielding for the first time end-grafted polymer brushes that are covalently linked to mica. The initiator grafting on the mica substrate was confirmed by time-of-flight secondary ion mass spectrometry (TOF-SIMS), while the change in the water contact angle of the OH-activated mica surface was used to follow the change in surface coverage of the initiator on the surface. The polymer brush and initiator film thicknesses relative to the virgin mica were confirmed by atomic force microscopy (AFM). This was done by comparing the atomic step-height difference between a protected area of freshly cleaved mica and a zone exposed to plasma activation, initiator immobilization, and then ATRP.     

Photoinitiators with functional groups. VI. Chemically bound sensitizers

Several benzophenone‐ and thioxanthone‐based photosensitizers (PSs) were covalently bonded to hydroxyalkylphenone‐ and aminoalkylphenone‐based photoinitiators (PIs) to enhance the rate of the excitation‐transfer effect due to the close vicinity of the PS to the PI. The properties of these new systems were investigated with UV spectroscopy and photo‐differential scanning calorimetry. Broadband irradiation experiments and selective excitation of the PS were carried out for the physical mixtures and covalently bonded PI/PS combinations to investigate the effect of excitation transfer. Selective excitation of the PS chromophore revealed that the energy transfer was significantly increased in covalently bonded initiators in comparison with the physical mixtures. This effect was most pronounced for the hydroxyalkylphenones that were sensitized by suitable benzophenone derivatives, especially at low PI concentrations. © 2004 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 42: 2285–2301, 2004     

The anticancer natural product pironetin selectively targets Lys352 of alpha-tubulin

Pironetin is a potent inhibitor of tubulin assembly and arrests cell cycle progression in M phase. Analyses of its structure-activity relationships suggested that pironetin covalently binds tubulin. To determine the binding site of pironetin, we synthesized biotinylated pironetin, which inhibited tubulin assembly both in vitro and in situ. The biotinylated pironetin selectively and covalently bound with tubulin. Partial digestion of biotinylated pironetin-treated tubulin by several proteases revealed that the binding site is the C-terminal portion of alpha-tubulin. By systematic alanine scanning, the pironetin binding site was determined to be Lys352 of alpha-tubulin. Lys352 is located at the entrance of a small pocket of alpha-tubulin, and this pocket faces the beta-tubulin of the next dimer. This is the first compound that covalently binds to the alpha subunit of tubulin and Lys352 of alpha-tubulin and inhibits the interaction of tubulin heterodimers.     

Photoreactive stapled BH3 peptides to dissect the BCL-2 family interactome

Defining protein interactions forms the basis for discovery of biological pathways, disease mechanisms, and opportunities for therapeutic intervention. To harness the robust binding affinity and selectivity of structured peptides for interactome discovery, we engineered photoreactive stapled BH3 peptide helices that covalently capture their physiologic BCL-2 family targets. The crosslinking α helices covalently trap both static and dynamic protein interactors, and enable rapid identification of interaction sites, providing a critical link between interactome discovery and targeted drug design.     

Orientational Ordering of Dyes in the Glassy State of Liquid-Crystalline Side Group Polymers

Liquid-crystalline side group copolymers containing dyes can be macroscopic-ally oriented and the orientation can be locked-in below the glass transition temperature. The order parameters of anthraquinone dyes and a trisazo dye in nematic and smectic glasses were determined by optical absorption measurements. The dyes have higher degrees of order in the smectic glass than in the nematic glass. A comparison of order parameters of covalently bonded dyes with order parameters of monomeric dyes dissolved in the corresponding homopolymers demonstrates the influence of covalently anchoring the dye to the polymer.     

Investigation of covalently colored polyurethane latexes based on novel anthraquinone polyurethane chain extenders

Novel red and yellow polyurethane (PU) chain extenders with one anthraquinone chromophore and two hydroxyls were synthesized, and then used to fabricate covalently colored PU latexes with pendent chromophores on the PU backbone. The chemical structures of the chain extenders were characterized by ¹H-NMR and FTIR, and the properties of PU latexes and their films were investigated by UV-Vis absorption spectra, particle size analysis, FTIR, Soxhlet's extraction and xenon arc aging testing. Results showed that the covalently colored PUs had the same UV-Vis absorption behavior as the corresponding chain extenders, and amount of the chain extenders had no obvious influence on the latex preparation process and the resulted latex colloidal properties. Compared with the corresponding non-covalently colored PU latex films, both the light fastness and the solvent fastness of the covalently colored PU latex films were significantly enhanced by the covalent incorporation of chromophores with PU matrix.     

Bulk production of a strong covalently linked (C60H(x))2 dimer

The high-pressure treatment of C60 in an H2 atmosphere at high temperatures leads to the efficient formation of a covalently bound dimer and some oligomeric species. The resulting hydrogenated C120 is an example of the bulk production of covalently bound derivatized fullerene cores. Matrix-assisted laser desorption/ionization in conjunction with reflectron time-of-flight mass spectrometry has been applied to the product analysis. The dissociation pattern of selected C120H(2x)+ ions (x > 30) indicates the dimeric structure of (C60H(x))2, as opposed to a giant hydrofullerene species possessing a fused C120 core. However, the results also clearly indicate a much stronger bonding (multiple sigma bonding) between the C60H(x) units than present in cycloaddition products. Evidence of a covalently linked dimer was obtained in labeling experiments, on the basis of which any laser-induced gas-phase aggregation of the C60H(x) monomer during the analysis is discounted.     

Covalent attachment and hybridization of DNA oligonucleotides on patterned single-walled carbon nanotube films

DNA oligonucleotides were covalently immobilized to prepatterned single-walled carbon nanotube (SWNT) multilayer films by amidation. SWNT multilayer films were constructed via consecutive condensation reactions creating stacks of functionalized SWNT layers linked together by 4,4'-oxydianiline. Aminated- or carboxylated-DNA oligonucleotides were covalently immobilized to the respective carboxylated or aminated SWNT multilayer films through amide bond formation using 1-ethyl-3-(3-dimethylaminopropyl)carbodiimide hydrochloride. UV-vis-NIR spectroscopic analysis indicated that the SWNT film surface density increased uniformly according to the number of reaction cycles. Scanning electron microscopy and contact angle measurements of the SWNT multilayer film revealed a uniform coverage over the substrate surface. The covalent attachment of DNA oligonucleotides to the SWNT multilayer films and their subsequent hybridization with complementary oligonucleotides were verified using X-ray photoelectron spectroscopy and fluorescence-based measurements. This is the first report demonstrating that DNA oligonucleotides can be covalently attached to immobilized SWNT multilayer films. The anchored DNA oligonucleotides were shown to exhibit excellent specificity, realizing their potential in future biosensor applications.     

A covalent capillary coating of diazoresin and polyglycerol dendrimer for protein analysis using capillary electrophoresis

Overcoming proteins adsorption on the inner surface of capillary has attracted increasing attention recently. By using the unique photochemistry reaction of diazoresin (DR), a new covalent capillary coating was prepared on the fused‐silica capillary through layer‐by‐layer self‐assembly of DR with polyglycerol (PG) dendrimer. The separation performance of covalently DR/PG‐dendrimer coated capillary noticeably exceeded the bare capillary and the noncovalently linked DR/PG‐dendrimer capillary. A baseline separation of lysozyme, myoglobin, bovine serum albumin, and ribonuclease A was achieved using CE within 20 min. Besides, the covalently linked DR/PG‐dendrimer coating has the remarkable stability and reproducibility. Especially, compared with the traditional method which use highly toxic and moisture‐sensitive silane coupling agent, this method seems to be a simple and environmental friendly way to prepare the covalently coated capillaries for CE.     

Kinetics of enzyme attack on substrates covalently attached to solid surfaces: influence of spacer chain length, immobilized substrate surface concentration and surface charge

The use of alpha-chymotrypsin to cleave covalently bound N-acetyl- l-tryptophan (Ac-Trp-OH) from the surfaces of aminopropylated controlled pore glass (CPG) and the polymer PEGA 1,900 was investigated. Oligoglycine spacer chains were used to present the covalently attached Ac-Trp-OH substrate to the aqueous enzyme. In the absence of the oligoglycine spacer chain, the rate of release was relatively slow, especially from the PEGA 1,900. These slow rates reflect the position of the amino group to which Ac-Trp-OH is covalently attached. On the glass there was a clear optimum with a chain of four glycine residues. For PEGA 1,900 there is no real apparent change beyond two glycine residues. The decline in rate beyond these optima are a possible result of changes in oligoglycine structure. Comparing different surface loadings of bound substrate the rate of release of Ac-Trp-OH from CPG with a pore diameter of 1,200 A was optimal when using 83% of the maximum that can be coupled, then fell again at higher loading. The rate of Ac-Trp-OH release from CPG was the same for surface coverages of 0.4 and 1.0. The introduction of permanent surface charges on CPG 1,200 exhibits a distinct influence on enzymatic cleavage with an increase in the rate of biocatalysis at the surface. Optimal presentation of covalently immobilized substrate on different supports by use of appropriate linkers leads to favorable biocatalysis from the support.     

Covalent adlayer growth on a diamond thin film surface

The surface of boron-doped diamond thin films can be modified by exposure to a strong oxidizing agent, resulting in the formation of -OH and =O terminated diamond. The -OH groups are reacted with an acid chloride to produce a covalently bound, modified diamond thin film surface. The demonstration of these reactions allows for the facile modification of diamond surfaces using techniques well established for oxide surfaces. Characterization of the covalently bound species shows submonolayer coverage, and time-resolved fluorescence measurements are reflective of the highly featured nature of the diamond film.     

Short peptides enhance single cell adhesion and viability on microarrays

Single cell patterning holds important implications for biology, biochemistry, biotechnology, medicine, and bioinformatics. The challenge for single cell patterning is to produce small islands hosting only single cells and retaining their viability for a prolonged period of time. This study demonstrated a surface engineering approach that uses a covalently bound short peptide as a mediator to pattern cells with improved single cell adhesion and prolonged cellular viability on gold patterned SiO2 substrates. The underlying hypothesis is that cell adhesion is regulated by the type, availability, and stability of effective cell adhesion peptides, and thus covalently bound short peptides would promote cell spreading and, thus, single cell adhesion and viability. The effectiveness of this approach and the underlying mechanism for the increased probability of single cell adhesion and prolonged cell viability by short peptides were studied by comparing cellular behavior of human umbilical cord vein endothelial cells on three model surfaces whose gold electrodes were immobilized with fibronectin, physically adsorbed Arg-Glu-Asp-Val-Tyr, and covalently bound Lys-Arg-Glu-Asp-Val-Tyr, respectively. The surface chemistry and binding properties were characterized by reflectance Fourier transform infrared spectroscopy. Both short peptides were superior to fibronectin in producing adhesion of only single cells, whereas the covalently bound peptide also reduced apoptosis and necrosis of adhered cells. Controlling cell spreading by peptide binding domains to regulate apoptosis and viability represents a fundamental mechanism in cell-materials interaction and provides an effective strategy in engineering arrays of single cells.