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1.
The aims of this study were to encapsulate water-soluble bioactive agents into biodegradable hydrophobic polymers via emulsion electrospinning for drug delivery and tissue engineering applications and propose a simple and facile method to evaluate the bioactivity of the encapsulated protein. Proteinase K was selected as a model protein to be incorporated into poly(ethylene glycol)-poly(l-lactide) (PELA) ultrafine fibers. Core–shell structured fibers with single core or multi-core were observed. In vitro release study showed that after a burst release at the early stage, a sustained release was achieved, indicating that proteinase K was incorporated inside ultrathin fibers successfully. Results of in vitro incubation in Tris–HCl buffer at pH?8.6 and 37?°C revealed that electrospun PELA membranes containing proteinase K (PELA-P) showed obvious morphological changes, large mass loss, and slight decreases in melting temperature, melting enthalpy and relative molecular mass in 7 days. Additionally, a significant drop in pH value of the buffer after incubation of the PELA-P membrane was also observed. These findings clearly showed that encapsulation of water-soluble bioactive agents inside hydrophobic polymers could be achieved by emulsion electrospinning without compromising their bioactivity.  相似文献   

2.
In the process of preparing core–sheath fibers via coaxial electrospinning, the relative evaporation rates of core and sheath solvents play a key role in the formation of the core–sheath structure of the fiber. Both silk fibroin (SF) and poly(lactide‐co‐ε‐caprolactone) (PLCL) have good biocompatibility and biodegradability. SF has better cell affinity than PLCL, whereas PLCL has higher breaking strength and elongation than SF. In this work, hexafluoroisopropanol (HFIP)‐formic acid (volume ratio 8:2), HFIP and HFIP–dichloromethane (volume ratio 8:2) were used to dissolve PLCL as the core solutions, and HFIP was used to dissolve SF as the sheath solution. Then, core–sheath structured SF/PLCL (C‐SF/PLCL) fibers were prepared by coaxial electrospinning with the core and sheath solutions. Transmission electron microscopy images indicated the existence of the core–shell structure of the fibers, and energy dispersive X‐ray analysis results revealed that the fiber mat with the greatest content of core–shell structure fibers was obtained when the core solvent was HFIP–dichloromethane (volume ratio 8:2). Tensile tests showed that the C‐SF/PLCL fiber mat displayed improved tensile properties, with strength and elongation that were significantly higher than those of the pure SF mat. The C‐SF/PLCL fiber mat was further investigated as a scaffold for culturing EA.hy926 cells, and the results showed that the fiber mat permitted cellular adhesion, proliferation and spreading in a manner similar to that of the pure SF fiber mat. These results indicated that the coaxial electrospun SF/PLCL fiber mat could be considered a promising candidate for tissue engineering scaffolds for blood vessels. Copyright © 2014 John Wiley & Sons, Ltd.  相似文献   

3.
PolyDL-lactide (PDLLA) and the block copolymer, polyDL-lactide-b-poly(ethylene glycol)-b-polyDL-lactide (PELA) were used as the microsphere matrix to encapsulate plasmid DNA. The PDLLA, PELA, pBR322-1oaded PDLLA and pBR322-1oaded PELA microspheres were prepared by solvent extraction method based on the formation of multiple w1/o/w2 emulsion. The microspheres were characterized by surface morphology, mean particle size, particle size distribution and loading efficiency. The integrity of DNA molecules after being extracted from microspheres was determined by agarose gel electrophoresis. The result suggested that plasmid DNA molecules could retain their integrity after being encapsulated by PELA. The PELA microspheres could prevent plasmid DNA from being digested by DNase. The in vitro degradation and release profiles of plasmid DNA-loaded microspheres were measured in pH - 7.4 buffer solution at 37℃. The in vitro degradation profiles of the microspheres were evaluated by the deterioration in microspheres surface morphology, the molecular weight reduction of polymer, the mass loss of microspheres, the changes of pH values of degradation medium, and the changes of particle size. The in vitro release profiles of the microspheres were assessed by measurement of the amount of DNA presented in the release medium at determined intervals. The release profiles were correlation with the degradation profiles. The release of plasmid DNA from PELA microspheres showed a similar biphasic trend, that is, an initial burst release was followed by a slow, but sustained release.  相似文献   

4.
Wei K  Li Y  Lei X  Yang H  Teramoto A  Yao J  Abe K  Ko FK 《Macromolecular bioscience》2011,11(11):1526-1536
The effectiveness of a multifunctional scaffold produced by the electrospinning of emulsions composed of organic PLGA and aqueous collagen-like protein (denoted as Fol-8Col) solutions is demonstrated. The resultant Fol-8Col/PLGA fibrous scaffolds with homogeneous morphology have mean fiber diameters from 600 to 2,000 nm. A uniform distribution of encapsulated Fol-8Col in the fibers is observed by fluorescence microscopy. TEM is used to clarify the representative core/sheath structure of emulsion electrospun Fol-8Col/PLGA fibers. Preliminary release assessment of encapsulated Fol-8Col shows results of sustained release for more than one month from the Fol-8Col/PLGA fibrous mats. The cytocompatibility of fibroblast cell line L929 with the fibrous composite seems promosing.  相似文献   

5.
聚乙二醇-b-聚乳酸的合成及其电纺形成超细纤维研究   总被引:2,自引:2,他引:0  
为了提高聚乳酸的亲水性,以辛酸亚锡为催化剂、聚乙二醇单甲醚(mPEG)为大分子引发剂进行丙交酯(LLA)开环聚合,合成聚乙二醇-b-聚乳酸两嵌段共聚物(PELA).以红外光谱1、H核磁共振谱、接触角测试、差热扫描量热分析等方法对PELA的结构及性能进行表征.结果表明,通过调控mPEG与LLA的投料比可以控制PELA的相对分子质量,而随着mPEG组分含量或链长增加,共聚物亲水性增强,但其Tg、Tcc、Tm有所降低.由普通电纺制备PELA超细纤维,并分别由乳液电纺和同轴电纺得到以水溶性聚氧化乙烯(PEO)为芯、PELA为壳的芯/壳结构复合超细纤维(E-PEO/PELA和C-PEO/PELA).扫描电镜和透射电镜结果表明,PELA、E-PEO/PELA和C-PEO/PELA超细纤维形貌良好.随着PELA中mPEG含量的增加,电纺PELA纤维膜的吸水率增强,而由乳液电纺和同轴电纺制备的PEO/PELA芯/壳结构超细纤维膜,亲水性均好于PELA超细纤维膜.  相似文献   

6.
In this research, thermoresponsive and conductive fibers with core‐sheath structure were fabricated by coaxial electrospinning. For preparing the spinning sheath solution, poly‐(N‐isopropylacrylamide‐co‐N‐methylolacrylamide) (PNN) copolymer having thermoresponsive and cross‐linkable properties was synthesized by free‐radical polymerization using redox initiators; it was then mixed with the conductive poly(3,4‐ethylenedioxythiophene):poly(styrene sulfonate) (PEDOT:PSS) at different weight ratios in water. On the other hand, poly(butyl acrylate‐co‐styrene) (PBS) copolymer synthesized by emulsion polymerization was dissolved in chloroform and used as the spinning core solution. After electrospinning, the fibers were treated at 110 °C for 1 h to cross‐link the PNN portion in the sheath for strengthening the fibers. Well‐defined core‐sheath fibers were observed from SEM pictures; the outside and inside (core) diameters were 568 ± 24 and 290 ± 40 nm, respectively, as determined from TEM pictures. The fiber mats were further doped by DMSO to enhance their conductivity. For the fiber mat with the weight ratio of PEDOT:PSS/PNN at 0.20 in the sheath, its surface conductivity could reach 29.4 S/cm. In addition, the fiber mats exhibited thermoresponsive properties that both swelling ratio and electric resistance decreased with temperature. Furthermore, the fiber mats exhibited improved flexibility as evaluated via bending test. © 2015 Wiley Periodicals, Inc. J. Polym. Sci., Part A: Polym. Chem. 2016 , 54, 1299–1307  相似文献   

7.
Biodegradable fibers for the controlled delivery of anti‐inflammatory agent dexamethasone were developed and studied. Mono and core–shell structure fiber are prepared by wet‐spinning solutions of hydrophobic poly (lactide‐co‐glycolide) and hydrophilic alginic acid shell. The two model drugs, dexamethasone and dexamethasone‐21‐phosphate, were entrapped in core and shell, respectively. These fibers were characterized in terms of morphology, diameters, mechanical properties, in vitro degradation, and drug release. The optical microscopy and scanning electron microscopy photos revealed directly that fibers possessed core–shell structure. The release of dexamethasone and dexamethasone‐21‐phosphate was investigated, and the results showed that alginate shell retarded dexamethasone release significantly in both early and late stages. The core–shell structure fiber release shows a two stage release of dexamethasone and dexamethasone‐21‐phosphate with distinctly different release rates, and minimal initial burst release is observed. The results indicated that the prepared fibers are efficient carrier for both types of dexamethasone. Copyright © 2016 John Wiley & Sons, Ltd.  相似文献   

8.
Proteinase K was successfully loaded inside ultrafine fibers of poly(ethylene glycol)-poly(l-lactide) (PELA) by emulsion electrospinning. A core/shell fiber structure was formed and verified by a transmission electron microscope. In vitro biodegradation of electrospun PELA membranes containing proteinase K (PELA-P) was examined in Tris-HCl buffer solution at pH 8.6 and 37 °C in comparison with electrospun PELA membranes without proteinase K. During biodegradation, mass loss, water absorption, pH value of the incubated buffer, fibrous morphology and thermal properties were monitored. Results suggested that PELA-P membranes degraded significantly faster than PELA membranes. A significant drop in pH value of the buffer after incubation of PELA-P membranes for 1 d was observed, and after 7 d, PELA-P membranes lost their fibrous appearance and masses almost completely. In contrast, electrospun PELA membranes did not show any obvious changes. The obtained electrospun PELA-P membranes exhibited self-accelerated biodegradability and could benefit drug controlled release and tissue regeneration.  相似文献   

9.
Poly-DL-lactide-poly(ethylene glycol) (PELA) microspheres containing Hepatitis B surface antigen (HBsAg) were elaborated by a solvent extraction method based on the formation of a double water/oil/water (w/o/w) emulsion. Microspheres were characterized in terms of morphology, size and size distribution, encapsulation efficiency, and the efficiency of microsphere formation (EMF). Transmission electron microscopy (TEM) and polyacrylamide gel electrophoresis (PAGE) were used to investigate the structural integrality of HBsAg encapsulated in PELA microspheres. The release profile was investigated by the measurement of antigen present in the release medium at various intervals. The PELA-10 microspheres displayed the highest antigen encapsulation efficiency (about 80%), and antigen molecules could be stabilized in the PELA-10 microspheres during the preparation process. It suggested that the PELA microspheres had a great potential as a new polymer adjuvant for HBsAg. The release of Hepatitis B surface antigen from poly-DL-lactide-poly(ethylene glycol) microspheres.  相似文献   

10.
Functional PLA scaffolds are created with single component, core–sheath, or porous fiber morphology and doped with TCP nanoparticles to study the release profiles for use in bone tissue engineering applications. Pharmacokinetic analyses are performed for the three different nanofibrous structures after doping with TCP. Results indicate that single component and porous fiber scaffolds exhibit an initial‐burst release profile whereas core–sheath fibers show a steady release. All scaffolds are then seeded with human adipose‐derived stem cells (hASC), which remain viable and continue proliferation on all nanofibrous morphologies for up to 21 d. Osteogenic differentiation of hASC and cell‐mediated calcium accretion are largest on porous fibers.

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