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首页> 外文期刊>Biomacromolecules >Synthesis and Characterization of Photo-Cross-Linkable Keratin Hydrogels for Stem Cell Encapsulation
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Synthesis and Characterization of Photo-Cross-Linkable Keratin Hydrogels for Stem Cell Encapsulation

机译:用于干细胞包封的光交联角蛋白水凝胶的合成与表征

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摘要

The objective of this work was to synthesize an injectable and photopolymerizable hydrogel based on keratin extracted from poultry feather for encapsulation and delivery of stem cells in tissue regeneration. Since feather keratin is rich in cysteine residue, allylation of sulfhydryl groups was used for functionalization of keratin. Keratin was extracted from feather barbs by reducing the disulfide bonds in cysteine residues to sulfhydryl groups (-SH). Next, the free thiol groups were converted to dehydroalanine (Dha) by oxidative elimination using O-(2,4,6-trimethylbenzenesulfonyl) hydroxylamine. Then, the Dha moieties were converted to s-allyl cysteine by reaction with allyl mercaptan to produce keratin allyl thioether (KeratATE) biopolymer. Human mesenchymal stem cell (hMSCs) were suspended in the aqueous solution of KeratATE, injected into a mold, and photopolymerized to generate a KeratATE hydrogel encapsulating hMSCs. The freeze-dried photo-cross-linked KeratATE hydrogels had a porous, interconnected, honeycomb microstructure with pore sizes in the 20-60 mu m range. The compressive modulus of the hydrogels ranged from 1 to 8 kPa depending on KeratATE concentration. KeratATE hydrogels had <5% mass loss in collagenase solution after 21 days of incubation, whereas the mass loss was 15% in trypsin solution. Degradation of KeratATE hydrogel was strongly dependent on trypsin concentration but independent of collagenase. hMSCs proliferated and adopted an elongated spindle-shape morphology after seeding on KeratATE hydrogel. KeratATE hydrogel supported differentiation of the encapsulated hMSCs to the osteogenic and chondrogenic lineages to the same extent as those hMSCs encapsulated in gelatin methacryloyl hydrogel. The results suggest that keratin allyl thioether hydrogel with controllable degradation is a viable matrix for encapsulation and delivery of stem cells in tissue regeneration.
机译:本作作品的目的是在基于从家禽羽羽中提取的角蛋白来合成可注射和可光聚合的水凝胶,以进行组织再生在组织再生中的干细胞。由于羽毛蛋白富含半胱氨酸残基,因此巯基的烯丙基化用于角蛋白的官能化。通过将半胱氨酸残基中的二硫键降低至巯基(-SH),从羽毛玻璃中从羽毛玻璃中提取角蛋白。接下来,通过使用O-(2,4,4,6-三甲基苯磺酰基)羟胺通过氧化消除将自由硫醇基团转化为脱氢碱(DHA)。然后,通过与烯丙基硫醇的反应将DHA部分转化为S-烯丙基半胱氨酸,以产生角蛋白烯丙基硫醚(角酸)生物聚合物。将人的间充质干细胞(HMSCs)悬浮在角酸盐水溶液中,注入模具中,并光聚合以产生包装HMSC的角酸水凝胶。冷冻干燥的光交联角酸盐水凝胶具有多孔,相互连接的蜂窝微观结构,其中孔径在20-60μm范围内。根据角酸盐浓度,水凝胶的压缩模量范围为1至8kPa。在孵育21天后,角膜酸盐水凝胶在胶原酶溶液中具有<5%的质量损失,而胰蛋白酶溶液中的质量损失为15%。角酸盐水凝胶的降解强烈依赖于胰蛋白酶浓度,而是依赖于胶原酶。 HMSCs在播种后在角酸盐水凝胶后采用细长的主轴形态。角酸盐水凝胶支持将包封的HMSCs的分化为骨质发生和软骨内谱系,与那些在明胶甲基丙烯酰水凝胶中包封的那些HMSCs相同程度。结果表明,具有可控降解的角蛋白烯丙基硫醚水凝胶是用于在组织再生中封装和递送干细胞的活性基质。

著录项

  • 来源
    《Biomacromolecules》 |2017年第2期|共15页
  • 作者单位

    Univ South Carolina Biomimet Mat &

    Tissue Engn Lab Dept Chem Engn Columbia SC 29208 USA;

    Univ South Carolina Biomimet Mat &

    Tissue Engn Lab Dept Chem Engn Columbia SC 29208 USA;

    Univ South Carolina Biomimet Mat &

    Tissue Engn Lab Dept Chem Engn Columbia SC 29208 USA;

    Univ South Carolina Biomimet Mat &

    Tissue Engn Lab Dept Chem Engn Columbia SC 29208 USA;

    Univ South Carolina Dept Sci Biol Columbia SC 29208 USA;

    Univ South Carolina Biomimet Mat &

    Tissue Engn Lab Dept Chem Engn Columbia SC 29208 USA;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分子生物学;
  • 关键词

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