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Macroporous scaffolds: Molecular brushes based on oligo(lactic acid)-amino acid-indomethacin conjugated poly(norbornene)s

机译:大孔支架:基于寡核苷酸(乳酸) - 氨基酸 - 吲哚美辛共轭聚(降冰片烯)的分子刷

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Leucine-derived norbornene monomer (1), oligo(lactic acid)-derived norborne macromonomer (2) and indomethacin-conjugated norbomene (3) were synthesized and polymerized using the Grubbs ruthenium complex as a catalyst. Macromonomer 2 was synthesized by the ring-opening polymerization of lactide using 5-norbornene-2,3-exo,exo-dimethanol as an initiator and 1,8-diazabicyclo[5.4.0]undec-7-ene (DBU) as a catalyst. The corresponding polymers, poly(1), poly(2), poly(3) and copolymers with number-average molecular weights (M-n) ranging from 14 000 to 360 000 were obtained in 73-95% yields. Poly(2) formed scaffolds by simply drying under reduced pressure presumably due to the brush-like structure causing entanglement of the polymer chains. The compressive strength of poly(2) scaffold increased as increasing the polylactide chain length. The compressive strength of the scaffolds obtained from the copolymers ranged from 0.222 to 0.587 MPa in accordance with the monomer unit ratios. SEM revealed the presence of pores around 5-10 mu m diameters, together with larger pores dispersed in the range of 50-300 mu m diameters. TEM demonstrated the presence of polymer networks. The conjugated indomethacin was gradually released by incubation under acidic condition (pH 5.7) at 37 degrees C. The results of % cell viability, release of LDH activity and cell morphology assays revealed that the obtained scaffolds did not exhibit cytotoxicity toward HEK 293 cells.
机译:亮氨酸衍生的降冰片烯单体(1),寡核苷酸(乳酸)的降低的降冰片型大分子单体(2)和吲哚美辛蛋白 - 共轭的降血烯(3)合成并使用GRUBBS钌配合物作为催化剂聚合。通过使用5-降冰片烯-2,3-EXO,EXO-二甲醇作为引发剂和1,8-二氮杂双环[5.4.0] UDEC-7-ENE(DBU)作为引发剂的开环聚合,通过丙交酯的开环聚合合成。催化剂。在73-95%的产率下,获得相应的聚合物,聚(1),聚(2),聚(3)和具有14 000至360 000的分子量(M-N)的共聚物。通过在减压下简单地干燥,通过引起聚合物链缠结的刷状结构,通过简单地干燥来形成支架。聚(2)支架的抗压强度随着增加聚物链长度而增加。根据单体单元比,从共聚物获得的支架的压缩强度范围为0.222至0.587MPa。 SEM揭示了大约5-10μm直径约为5-10μm的孔的存在,以及分散在50-300 mu m的范围内的较大孔。 TEM证明了聚合物网络的存在。通过在37℃下在酸性条件(pH5.7)下孵育逐渐释放缀合的吲哚美甘油。%细胞活力的结果,LDH活性的释放和细胞形态学测定显示,所获得的支架未对HEK 293细胞表现出细胞毒性。

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