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Pulp EGM-derived macroporous scaffolds for stimulation of dental-pulp regeneration process

机译:纸浆EGM衍生的大孔支架刺激牙髓再生过程

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摘要

Objective. Recent studies suggest xenogeneic extracellular matrices as potential regenerative tools in dental pulp regeneration. This study aimed to fabricate and characterize a novel three-dimensional macroporous pulp-derived scaffold that enables the attachment, penetration, proliferation and differentiation of mesenchymal stem cells.Method. Bovine pulp was decellularized and characterized with histological and DNA content methods. This scaffold was prepared using finely milled lyophilized decellularized pulp extracellular matrix (ECM) digested with pepsin. Three different concentrations of ECM (1.50, 2.25 and 3.00 mg/ml) were freeze-dried and were tested with/without chemical crosslinking. The specimens were subjected to physicochemical characterization, cell viability and quantitative real time polymerase chain reaction assessments with human bone marrow mesenchymal stem cells (hBMMSCs). All scaffolds were subcutaneously implanted in rats for two weeks and histological and immunostaining analyses were performed.Results. Histological and DNA analysis confirmed complete decellularization. All samples demonstrated more than 97% porosity and 1.50 mg/ml scaffold demonstrated highest water absorption. The highest cell viability and proliferation of hBMMSCs was observed on the 3.00 mg/ml crosslinked scaffolds. The gene expression analysis showed a significant increase of dmp-1 and collagen-I on 3.00 mg/ml crosslinked scaffolds compared to the other scaffolds. Histological examination of subcutaneous implanted scaffolds revealed low immunological response, and enhanced angiogenesis in cross-linked samples compared to non-crosslinked samples.Significance. The three-dimensional macroporous pulp-derived injectable scaffold developed and characterized in this study displayed potential for regenerative therapy. While the scaffold biodegradability was decreased by crosslinking, the biocompatibility of post-crosslinked scaffold was significantly improved. (C) 2019 The Academy of Dental Materials. Published by Elsevier Inc. All rights reserved.
机译:目的。最近的研究表明异种细胞外基质是牙髓再生中潜在的再生工具。这项研究旨在制造和表征新颖的三维大孔髓衍生的支架,使间充质干细胞的附着,渗透,增殖和分化成为可能。将牛牙髓脱细胞,并用组织学和DNA含量方法进行表征。使用经胃蛋白酶消化的细磨的冻干脱细胞果肉细胞外基质(ECM)制备该支架。将三种不同浓度的ECM(1.50、2.25和3.00 mg / ml)冷冻干燥,并在有/无化学交联的情况下进行测试。用人骨髓间充质干细胞(hBMMSC)对标本进行理化鉴定,细胞活力和实时定量聚合酶链反应评估。将所有支架皮下植入大鼠体内两周,并进行组织学和免疫染色分析。组织学和DNA分析证实完全脱细胞。所有样品均显示出超过97%的孔隙率,而1.50 mg / ml支架显示出最高的吸水性。在3.00 mg / ml的交联支架上观察到了hBMMSC的最高细胞活力和增殖。基因表达分析表明,与其他支架相比,在3.00 mg / ml交联支架上dmp-1和I型胶原蛋白显着增加。皮下植入的支架的组织学检查显示,与未交联的样品相比,交联的样品免疫应答低,血管生成增强。在这项研究中开发和表征的三维大孔纸浆衍生的可注射支架展示了再生疗法的潜力。尽管通过交联降低了支架的生物降解性,但后交联支架的生物相容性却得到了显着改善。 (C)2019牙科材料学院。由Elsevier Inc.出版。保留所有权利。

著录项

  • 来源
    《Dental materials》 |2020年第1期|76-87|共12页
  • 作者

  • 作者单位

    Islamic Azad Univ Tehran Med Sci Fac Dent Dept Endodont Tehran Iran|Univ Toronto Fac Dent 124 Edward St Toronto ON M5G 1G6 Canada|Islamic Azad Univ Tehran Cent Branch Tissue Engn & Regenerat Med Inst Stem Cell Res Ctr Tehran Iran;

    Iran Univ Med Sci Burn Res Ctr Tehran Iran;

    Islamic Azad Univ Tehran Cent Branch Tissue Engn & Regenerat Med Inst Stem Cell Res Ctr Tehran Iran;

    ACECR Royan Inst Stem Cell Biol & Technol Cell Sci Res Ctr Dept Cell Engn Tehran Iran;

    Univ Tehran Med Sci Fac Pharm Dept Pharmacol Toxicol Tehran Iran;

    Univ Hosp Regensburg Dept Conservat Dent & Periodontol Regensburg Germany;

    Univ Toronto Fac Dent 124 Edward St Toronto ON M5G 1G6 Canada;

    Univ Toronto Fac Dent 124 Edward St Toronto ON M5G 1G6 Canada|Univ Toronto Inst Hlth Policy Management & Evaluat Clin Epidemiol & Hlth Care Res Toronto ON Canada|Mt Sinai Hosp Dept Dent Toronto ON Canada;

    Univ Toronto Fac Dent 124 Edward St Toronto ON M5G 1G6 Canada|Mt Sinai Hosp Dept Dent Toronto ON Canada;

  • 收录信息 美国《科学引文索引》(SCI);美国《工程索引》(EI);美国《化学文摘》(CA);
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类
  • 关键词

    Tissue engineering; Dentin-pulp complex; Pulp ECM; Crosslinked scaffold;

    机译:组织工程;牙本质浆复合物;纸浆ECM;交联支架;
  • 入库时间 2022-08-18 05:19:14

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