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1.
Stable poly{(vinyl acetate)‐co‐[3‐dimethyl(methacryloyloxyethyl)ammonium propanesulfonate]} latexes with different compositions were synthesized by emulsifier‐free emulsion copolymerization. An unusual “overshooting” behavior of the copolymer tablets is explained based on the formation of specific clusters of oppositely oriented dipoles. The variation of their concentration with the zwitterionic monomer unit fraction, ionic strength and temperature is responsible for the differences in the swelling kinetics established. The results show that these parameters can be used to control swelling degree of copolymer matrices and their sustained drug delivery.

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A robust and effortless procedure is presented, which allows for the microstructuring of standard cell culture dishes. Cell adhesion and proliferation are controlled by three‐dimensional poly(ethylene glycol)‐dimethacrylate (PEG‐DMA) microstructures. The spacing between microwells can be extended to millimeter size in order to enable the combination with robotic workstations. Cell arrays of microcolonies can be studied under boundary‐free growth conditions by lift‐off of the PEG‐DMA layer in which the growth rate is accessible via the evolution of patch areas. Alternatively, PEG‐DMA stencils can be used as templates for plasma‐induced patterning.

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We developed a dynamic Monte Carlo model for ATRP in semibatch reactors. Semibatch reactors can be used to produce gradient copolymers even if the difference between the reactivity ratios of the comonomers is not significant by using different comonomer feed policies. The model was used to predict average molecular weights, polydispersity index, copolymer composition and complete distributions of molecular weight, chemical composition, and comonomer sequence length at any polymerization time. Two case studies, poly[styrene‐co‐(methyl methacrylate)] and poly[acrylonitrile‐co‐(methyl methacrylate)], were chosen to demonstrate the effect of comonomer feed compositions on the final chemical composition distribution of the copolymer.

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Thermoresponsive surfaces are prepared via a spin‐coating method with a block copolymer consisting of poly(N‐isopropylacrylamide) (PIPAAm) and poly(butyl methacrylate) (PBMA) on polystyrene surfaces. The PBMA block suppresses the removal of deposited PIPAAm‐based polymers from the surface. The polymer coating affects the temperature‐dependent cellular behavior of the surfaces with respect to protein adsorption. By adjusting layer thicknesses, PBMA‐b‐PIPAAm‐coated surfaces are optimized to regulate the adhesion/detachment of cells by temperature changes. Thus, thermoresponsive polymer‐coated surfaces are able to harvest contiguous cell sheets with their basal extracellular matrix proteins.

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Fluorescent‐magnetic‐biotargeting multifunctional microcapsules (FMBMMs) are designed and fabricated via layer‐by‐layer assembly. It is found that the arginine‐glycine‐aspartate‐modified FMBMMs were capable of sensitively detecting and efficiently isolating approximately 80% target cancer cells within 20 min. More importantly, FMBMMs present a general template for identifying and separating multiple types of cancer cells simply by altering the recognition motif.

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A kinetic model that considers three geometric active sites—cis, trans and vinyl—was proposed to the study polymerization reaction of high 1,4‐trans‐polybutadiene (TPBD) prepared by means of anionic living polymerization using an initiator composed of alkyl aluminium, n‐butyllithium and barium alkoxide. The conversion and dyad sequence distribution was correctly predicted; the kinetic results indicated that the microstructure and sequence distribution do not change with the conversion and temperature within the range of temperature investigated (40–80 °C). In addition, it was observed that the addition mechanism of butadiene to the active sites is entropic.

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The effects of self‐assembled polysaccharide nanogels on colloidal and thermal stability of lipase from Pseudomonas cepacia were investigated. The enzyme activity, especially kcat, drastically increased in the presence of nanogels of cholesterol‐bearing pullulan (CHP). The thermostability of lipase complex increased because the denaturation temperature of lipase increased by more than 20 °C by complexation with CHP nanogels. Lipase denaturation and aggregation upon heating was effectively prevented by complexation with CHP nanogels. Moreover, complexation with CHP nanogels protected lipase from lyophilization‐induced aggregation. Nano‐encapsulation with CHP nanogel is a useful method for colloidal and thermal stabilization of unstable enzyme.

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