Colloidal crystallization kinetics is studied in the shear flow of a suspension of colloidal silica spheres (110 nm in diameter), using a continuously-circulating type of stopped flow cell system. The crystallization rate from a suspension containing a small amount of nuclei and/or single crystals is high compared with that from a suspension containing no nuclei and/or single crystals. Crystal growth takes place at shear rates smaller than 3.4 s–1 and at sphere concentrations higher than a volume fraction of 0.004. 相似文献
A novel immunoassay strategy based on combination of chitosan (CHIT) and a gold nanoparticle (GNP) label has been developed. The susceptibility of CHIT to further chemical modifications due to the abundant amino groups is explored in order to covalently immobilize antibody (Ab) onto the (3-aminopropyl) triethoxysilane derivatized glass slide by cross-linking with glutaraldehyde (GA). After incubating in antigen (Ag) solution, the obtained substrate is immersed in GNP labeled antibody solution for signal generation. The two steps were repeated alternatively for three times, forming multilayer of gold nanoparticles via antigen-antibody specific reaction. Ultraviolet-visible (UV-vis) absorption spectrum is recorded to obtain quantitative information about the specific antigen. The presented immunoassay strategy is applied for determination of human serum albumin (HSA) as a model analyte. The immunoassay of HSA is specific. Compared to previous correlative work, the proposed immunosensing strategy shows some advantages, such as improved sensitivity as much more gold nanoparticles can be coupled to the functionalized surface making use of the abundant amino groups of CHIT. Moreover, a significantly extended linear detection range of 8.0-512.0 μg/mL is gained under the optimized experimental conditions. In particular, the presented biosensing method shows low cost and simplicity, and only a conventional UV-vis detector is involved. 相似文献
A disposable sensor for the determination of cotinine in human serum was developed based on immunochromatographic test strip and quantum dot label. In this assay, cotinine linked with quantum dot competes with cotinine in sample to bind to anti-cotinine antibody in the test strip and the quantum dots serve as signal vehicles for electrochemical readout. Some parameters governing the performance of the sensor were optimized. The sensor shows a wide linear range from 1 ng mL?1 to 100 ng mL?1 cotinine with a detection limit of 1.0 ng mL?1. The sensor was validated with spiked human serum samples and it was found that this method was reliable in measuring cotinine in human serum. The results demonstrate that this sensor is rapid, accurate, and less expensive and has the potential for point of care (POC) detection of cotinine and fast screening of tobacco smoke exposure. 相似文献
In this study, colloidal systems with SiO2 nanoparticle as viscosity modifier additive were synthesized in the lubricating oil via an in situ Stober sol-gel method. The fluid characters of lubricating oil and viscosity variation were carefully investigated via rheological methods. The results showed that the lubricating oil transformed from Newtonian fluid to non-Newtonian fluid with increasing the concentration of nanoparticles, and smaller particles displayed better thickening effect toward lubricating oil. For the system with highly concentrated nanoparticle (20?wt%), the rheological behavior mainly depends on the size of nano-SiO2. The lubricating oil with smaller nano-SiO2 particles displayed higher structural strength and response rate, resulting in good recoverability after high-speed shear. The viscosity changed with temperature and also displayed a thermo-responsive behavior, which significantly alleviated the effect of shear thinning on the viscosity under high temperature. This study presented a new strategy for effectively tuning the fluid characters and modifying the viscosity of lubricating oils by adding highly concentrated inorganic nanoparticles. 相似文献
Nanoparticle labels have enhanced the performance of diagnostic, screening, and other measurement applications and hold further promise for more sensitive, precise, and cost-effective assay technologies. Nevertheless, a clear view of the biomolecular interactions on the molecular level is missing. Controlling the ratio of molecular recognition over undesired nonspecific adhesion is the key to improve biosensing with nanoparticles. To improve this ratio with an aim to disallow nonspecific binding, a more detailed perspective into the kinetic differences between the cases is needed. We present the application of two novel methods to determine complex binding kinetics of bioconjugate nanoparticles, interferometry, and force spectroscopy. Force spectroscopy is an atomic force microscopy technique and optical interferometry is a direct method to monitor reaction kinetics in second-hour timescale, both having steadily increasing importance in nanomedicine. The combination is perfectly suited for this purpose, due to the high sensitivity to detect binding events and the ability to investigate biological samples under physiological conditions. We have attached a single biofunctionalized nanoparticle to the outer tip apex and studied the binding behavior of the nanoparticle in a sandwich-type immunoassay using dynamic force spectroscopy in millisecond timescale. Utilization of the two novel methods allowed characterization of binding kinetics in a time range spanning from 50 ms to 4 h. These experiments allowed detection and demonstration of differences between specific and nonspecific binding. Most importantly, nonspecific binding of a nanoparticle was reduced at contact times below 100 ms with the solid-phase surface.
Figure A single biofunctionalized nanoparticle was attached to the outer tip apex and the binding behavior of the nanoparticle in a sandwich-type immunoassay, A) without analyte, B) with analyte and C) saturating analyte concentration, was recorded using dynamic force spectroscopy in millisecond timescale. The setting allowed measurement of the association speed of nonspecific binding.
A very simple and fast method for the direct determination of atrazine in food samples based on the use of stopped-flow fluorescence polarization immunoassay is described. Unlike other immunoassay methods where the analytical signal is obtained when the immunochemical reaction has reached or is close to the equilibrium, this method uses the initial rate of this reaction as the analytical parameter, which is measured in only 4-5 s. This approach minimizes the static signal from the sample matrix, allows the direct analysis of the samples and can be easily adapted to the routine automatic determination of atrazine. The dynamic range of the calibration graph was 0.7-100 ng ml(-1) and the detection limit was 0.2 ng ml(-1). The precision and selectivity of the method were also studied. The analytical recoveries obtained by applying the method to white and red wine, orange juice and tea samples ranged from 80 to 104%. 相似文献
A facile and sensitive immunoassay protocol for the detection of alpha-fetoprotein (AFP) was developed using gold-coated iron oxide magnetic nanoclusters and dynamic light scattering (DLS) methods. The increase in the average particle size due to AFP-mediated aggregation was measured using DLS, and the detection limit was better than 0.01 ng mL(-1). 相似文献
In this protocol, a fluorescent aptasensor based on magnetic separation for simultaneous detection thrombin and lysozyme was proposed. Firstly, one of the anti-thrombin aptamer and the anti-lysozyme aptamer were individually immobilized onto magnetic nanoparticles, acting as the protein captor. The other anti-thrombin aptamer was labeled with rhodamine B and the anti-lysozyme aptamer was labeled with fluorescein, employing as the protein report. By applying the sandwich detection strategy, the fluorescence response at 515 nm and 578 nm were respectively corresponding to lysozyme and thrombin with high selectivity and sensitivities. The fluorescence intensity was individually linear with the concentration of thrombin and lysozyme in the range of 0.13-4 nM and 0.56-12.3 nM, and the detection limits were 0.06 nM of thrombin and 0.2 nM of lysozyme, respectively. The preliminary study on simultaneous detection of thrombin and lysozyme in real plasma samples was also performed. It shows that the proposed approach has the good character for simultaneous multiple protein detection. 相似文献
We report on a highly sensitive competitive immunoassay for the mycotoxin Ochratoxin (OTA) using magnetic silica nanoparticles (NPs) fluorescently labeled with rhodamine 123 (Rho123) as signal intensifier. The method is based on the measurement of fluorescence resonance energy transfer (FRET) that occurs from CdTe quantum dots covered with anti-OTA antibody to the dye Rho123 on the surface of the NPs. The immunoreaction between anti-OTA antibody and OTA brings the fluorophore (acting as the acceptor) in close proximity of the QDs (acting as the donor), and this causes FRET to occur upon photo-excitation of the QDs. The size and polydispersity of the silica coated magnetic NPs was studied via TEM. The method has a detection limit of 0.8 pg of OTA per mL. It was applied to the determination of OTA in spiked human serum. A linear relationship is found between the increase in the fluorescence intensity of Rho 123 at 580 nm and the concentration of OTA in spiked samples over the 8 to 48 pg?mL?1 concentration range. This highly sensitive homogeneous competitive detection scheme is simple, rapid and efficient. It does not require multiple separation steps and excessive washing.
Graphical abstract Following photoexcitation of immobilized quantum dots (QDs), FRET occurs between the QDs and Rhodamine 123. The close proximity of Rho 123 and the magnetic silica core/shell particles leads to strongly intensified emission to result in an assay for Ochratoxin A that has a detection limit as low as 0.8 pg?mL-1
We report on a highly sensitive aptameric assay system for the determination of IgE, where a special chemiluminescence (CL) reagent, 3,4,5-trimethoxylphenylglyoxal (TMPG), acts as the signaling molecule and polystyrene beads as the amplification platform. Briefly, a "sandwich-type" detection strategy is employed in our design, where magnetic beads functionalized with a capture antibody were reacted with the target protein IgE, and then sandwiched with the aptamer-barcodes which were prepared by assembling polystyrene beads with IgE aptamer. The target immunoreaction event could be sensitively detected via an instantaneous derivatization reaction between TMPG and the guanine (G) nucleotides within the aptamer-barcodes to form an unstable CL intermediate for the generation of light. Further signal amplification is achieved by extending the G nucleotide-rich domain on the aptamer backbone for second amplification. Such simple amplified CL transduction allows the detection of IgE down to the 4.6 pM level, which is better than most previous aptameric methods for IgE detection. This new protocol also provides a good capability in discriminating IgE from nontarget proteins such as IgG, IgA, IgM, interferon and thrombin. The practical application of the proposed aptamer-barcode based immunoassay was successfully carried out for the determination of IgE in 20 human serum samples. It is straightforward to adapt this strategy to detect a spectrum of other proteins by using different aptamers, thus this method may offer a new direction in designing high-performance CL aptasensors for early diagnoses of diseases. 相似文献
A signal due to coherently excited vibrational motion has been observed in polydisperse silver nanoparticle samples. The particles were synthesized via a wet chemistry seed mediated method, which yields different particle shapes, including spheres, rods, and irregular triangular-shaped particles. The measured vibrational periods were compared to the results from continuum mechanics calculations. This analysis shows that the observed signal arises from the triangular-shaped particles, rather than the rods or spheres. The period of vibration increases as the dimensions of the triangular-shaped particles increase; specifically, we find that the period is given by 2h/c(l), where h is the bisector of the triangle and c(l) is the longitudinal speed of sound in silver. 相似文献
Co@Pt nanoparticles as a bifunctional nanoplatform system for the hydrogenation of various unsaturated organic molecules under mild conditions and also for magnetic separation and recycling are demonstrated. 相似文献
We describe a sensitive sandwich immunoassay for alpha-fetoprotein (AFP). It is making use of gold nanoparticles (GNPs) and magnetic beads (MBs) as labels, and of resonance Rayleigh scattering for detection. Two antibodies were labeled with GNPs and MBs, respectively, and MB-antigen-GNP complexes were formed in the presence of antigens. The MB labels also serve as solid phase carriers that can be used to magnetically separate the immuno complex. The GNP labels are used as optical probes, and Rayleigh scattering was used to determine the concentration of free GNPs-antibody after separation of the MB-antigen-GNP complexes. The concentration of AFP is related to the intensity of light scattered by free GNPs in the 13.6 pM to 436 pM concentration range, and the limit of detection is 13.6 pM. The method was applied to the determination of AFP in sera of cancer patients, and the results agree well with those obtained by conventional ELISA.
Figure
A sensitive sandwich immunoassay for alpha-fetoprotein (AFP) was reported in this paper. It was based on high resonance Rayleigh scattering light of gold nanoparticles (GNPs) and rapid separation of magnetic beads (MBs). Rayleigh scattering intensity of free GNPs was reduced strongly after immunoassay. Under optimized conditions, we got good relationship between resonance Rayleigh scattering (RRS) of free GNPs and the AFP concentration to determine AFP concentration efficiently. 相似文献
A polyclonal antibody against ochratoxin A (OTA) was produced from rabbits immunized with the OTA–BSA conjugate. A competitive
direct enzyme-linked immunosorbent assay (cdELISA) and a membrane-base colloidal gold immunoassay in flow-through format were
developed for the rapid detection of OTA in various food matrices. In the cdELISA, the concentration causing 50% inhibition
was 0.07 ng mL−1, and the effects of different chemical conditions (ionic strength, pH value, and organic solvent) were studied. The sensitivity
of the assay was higher than those previously reported. A simple, rapid, and efficient extraction method was developed and
74–110% recoveries of spiked samples were obtained. Fifty percent methanol extracts of some food samples such as barley, wheat,
oat, corn, rice, and raisins could be analyzed directly by immunoassay after dilution in PBS; grape juice and beer samples
could be analyzed directly after dilution with PBS; for coffee samples, a more complex method was used to remove the matrix
effect effectively. Membrane-based colloidal gold immunoassays had a visual detection limit of 1.0 ng mL−1 for OTA with a detection time of less than 10 min. For the validation of the cdELISA and membrane-based colloidal gold immunoassay,
samples were analyzed by high-performance liquid chromatography. The correlation between data obtained using the microwell
assay and HPLC was good (R2 = 0.984). The developed immunoassay methods are suitable for the rapid quantitative or qualitative determination of OTA in
food samples. 相似文献
A multianalyte lateral-flow technique using colloidal gold-labeled monoclonal antibodies was developed for the rapid simultaneous
detection of deoxynivalenol (DON) and zearalenone (ZEA). The results of this qualitative one-step test were interpreted visually.
A very simple and fast sample preparation was used, and the assay procedure could be accomplished within 10 min. When applied
to spiked wheat samples, the technique gave accurate and reproducible results. Cut-off levels of 1500 and 100 μg kg−1 for DON and ZEA, respectively, were observed. The described multianalyte format can be used as a reliable, rapid and cost-effective
on-site screening technique for the simultaneous determination of mycotoxins in grain samples. 相似文献
An ultrasensitive electrochemical immunoassay method based on counting single magnetic nanobead (MNB) with combined amplification of nanobead and enzyme. Carcinoembryonic antigen (CEA) and MNB were initially immobilized on substrate at 1:1 molar ratio through sandwich immunoreactions. The MNBs were then labeled with alkaline phosphatase (AP) and continuously introduced to capillary with disodium phenyl phosphate (DPP). APs convert DPPs into a phenol zone around each moving MNB, i.e., one CEA. The phenol zones can be electrochemically detected as peaks and counted for CEA quantification. The detection limit for CEA is 5.0 × 10?17 mol/L. 相似文献
We demonstrate the dispersion free digital transport of emulsion droplets and biological cells in an aqueous solution using paramagnetic colloidal particles above a uniaxial magnetic garnet film. Magnetic modulations above the stripe domain pattern induce a step-wise transport of paramagnetic particles dispersed in water and deposited on the surface of the film. Capillary or hydrodynamic interactions are then used to couple the cargo to the paramagnetic beads. We achieve full control of the cargo motion up to velocities in the 100 microm/s range. 相似文献
Sensitive biomarker detection techniques are beneficial for both disease diagnosis and postoperative examinations. In this study, we report an integrated microfluidic chip designed for the immunodetection of prostate-specific antigens (PSAs). The microfluidic chip is based on the three-dimensional structure of quartz capillaries. The outlet channel extends to 1.8 cm, effectively facilitating the generation of uniform droplets ranging in size from 3 to 50 μm. Furthermore, we successfully immobilized the captured antibodies onto the surface of magnetic beads using an activator, and we constructed an immunosandwich complex by employing biotinylated antibodies. A key feature of this microfluidic chip is its integration of microfluidic droplet technology advantages, such as high-throughput parallelism, enzymatic signal amplification, and small droplet size. This integration results in an exceptionally sensitive PSA detection capability, with the detection limit reduced to 7.00 ± 0.62 pg/mL. 相似文献
Monodisperse magnetic nanoparticles conjugated with complementary oligonucleotide sequences self-assemble into stable magnetic nanoassemblies resulting in a decrease of the spin-spin relaxation times (T2) of neighboring water protons. When these nanoassemblies are treated with a DNA cleaving agent, the nanoparticles become dispersed, switching the T2 of the solution back to original values. These qualities render the developed nanoparticles and their nanoassemblies as magnetic relaxation switches capable of screening for DNA-cleaving compounds by magnetic resonance methods such as MRI and NMR. 相似文献
