Biological scaffolds

生物支架
  • 文章类型: Journal Article
    伤口修复对于临床从业者和研究人员来说都是一个复杂的挑战。用于伤口修复的常规方法具有若干局限性。基于干细胞的治疗已经成为解决这个问题的一种新策略。表现出显著的提高伤口愈合率的潜力,改善伤口质量,促进皮肤再生。然而,在皮肤再生中使用干细胞提出了一些挑战。最近,干细胞和生物材料已被确定为伤口愈合过程的关键组成部分。涉及生物相容性支架开发的联合治疗,伴随细胞,多种生物学因素,和类似于天然细胞外基质(ECM)的结构已获得相当多的关注。生物支架包括一系列生物材料,用作接种干细胞的平台,为他们提供有利于成长的环境,类似于ECM。这些支架促进干细胞的递送和应用,用于组织再生和伤口愈合。本文就目前干细胞生物支架在创面愈合中的研究进展及应用作一综述。强调它们促进干细胞粘附的能力,扩散,分化,和旁分泌功能。此外,我们确定了有助于增强细胞活性的支架的关键特征。
    Wound repair is a complex challenge for both clinical practitioners and researchers. Conventional approaches for wound repair have several limitations. Stem cell-based therapy has emerged as a novel strategy to address this issue, exhibiting significant potential for enhancing wound healing rates, improving wound quality, and promoting skin regeneration. However, the use of stem cells in skin regeneration presents several challenges. Recently, stem cells and biomaterials have been identified as crucial components of the wound-healing process. Combination therapy involving the development of biocompatible scaffolds, accompanying cells, multiple biological factors, and structures resembling the natural extracellular matrix (ECM) has gained considerable attention. Biological scaffolds encompass a range of biomaterials that serve as platforms for seeding stem cells, providing them with an environment conducive to growth, similar to that of the ECM. These scaffolds facilitate the delivery and application of stem cells for tissue regeneration and wound healing. This article provides a comprehensive review of the current developments and applications of biological scaffolds for stem cells in wound healing, emphasizing their capacity to facilitate stem cell adhesion, proliferation, differentiation, and paracrine functions. Additionally, we identify the pivotal characteristics of the scaffolds that contribute to enhanced cellular activity.
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  • 文章类型: Journal Article
    背景:已经提出了来自几种组织来源的脱细胞细胞外基质(dECM)作为再生牙髓手术(REP)中使用的常规支架的有希望的替代品。本系统综述旨在评估利用dECM衍生的支架进行REP的研究的组织学结果,并分析可能影响再生组织性质的因素。
    方法:使用PRISMA2020指南。在GoogleScholar中搜索了直到2024年4月发表的文章,Scopus,PubMed和WebofScience数据库。在主要的牙髓期刊中手动搜索其他记录。原始文章包括在REP和体内研究中dECM的组织学结果,体外研究和临床试验被排除.纳入研究的质量评估采用ARRIVE指南进行分析。使用(SYRCLE)偏倚风险工具进行偏倚风险评估。
    结果:在获得的387项研究中,包括17项研究进行分析。在大多数研究中,当用作有或没有外源细胞的支架时,dECM显示出增强血管生成的潜力,牙本质发生并再生牙髓样和牙本质样组织。然而,纳入的研究显示去细胞化方法的异质性,动物模型,脚手架源,形式和交付,以及高偏倚风险和平均证据质量。
    结论:脱细胞ECM衍生的支架可以为REP中的牙本质牙髓再生提供潜在的现成支架。然而,由于本综述纳入研究的方法学异质性和平均质量,脱细胞ECM来源支架的总体有效性尚不清楚.需要更标准化的临床前研究以及构建良好的临床试验来证明这些支架用于临床翻译的功效。
    该协议已在PROSPERO数据库#CRD42023433026中注册。这篇评论是由科学资助的,技术和创新资助机构(STDF)资助编号(44426)。
    BACKGROUND: Decellularized extracellular matrix (dECM) from several tissue sources has been proposed as a promising alternative to conventional scaffolds used in regenerative endodontic procedures (REPs). This systematic review aimed to evaluate the histological outcomes of studies utilizing dECM-derived scaffolds for REPs and to analyse the contributing factors that might influence the nature of regenerated tissues.
    METHODS: The PRISMA 2020 guidelines were used. A search of articles published until April 2024 was conducted in Google Scholar, Scopus, PubMed and Web of Science databases. Additional records were manually searched in major endodontic journals. Original articles including histological results of dECM in REPs and in-vivo studies were included while reviews, in-vitro studies and clinical trials were excluded. The quality assessment of the included studies was analysed using the ARRIVE guidelines. Risk of Bias assessment was done using the (SYRCLE) risk of bias tool.
    RESULTS: Out of the 387 studies obtained, 17 studies were included for analysis. In most studies, when used as scaffolds with or without exogenous cells, dECM showed the potential to enhance angiogenesis, dentinogenesis and to regenerate pulp-like and dentin-like tissues. However, the included studies showed heterogeneity of decellularization methods, animal models, scaffold source, form and delivery, as well as high risk of bias and average quality of evidence.
    CONCLUSIONS: Decellularized ECM-derived scaffolds could offer a potential off-the-shelf scaffold for dentin-pulp regeneration in REPs. However, due to the methodological heterogeneity and the average quality of the studies included in this review, the overall effectiveness of decellularized ECM-derived scaffolds is still unclear. More standardized preclinical research is needed as well as well-constructed clinical trials to prove the efficacy of these scaffolds for clinical translation.
    UNASSIGNED: The protocol was registered in PROSPERO database #CRD42023433026. This review was funded by the Science, Technology and Innovation Funding Authority (STDF) under grant number (44426).
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  • 文章类型: Journal Article
    生物打印是一种结合活细胞的增材制造(AM)技术,生物材料,和生物分子来开发生物功能构建体。三维(3D)生物打印通常用作体外建模系统,并且与二维(2D)细胞培养相比是体内条件的更准确表示。尽管3D生物打印已被用于各种组织工程和临床应用,它只考虑打印支架或物体的初始状态。近年来出现了四维(4D)生物打印,以在打印的3D支架中纳入额外的时间维度。在4D生物打印过程中,外部刺激暴露于印刷结构,最终改变了它的形状或功能。通过研究结构和嵌入细胞对各种刺激的反应,研究人员可以更深入地了解天然组织的功能。本文将重点介绍4D生物打印新领域的生物材料突破及其在组织工程和再生中的应用。此外,讨论了将智能生物材料和4D打印机制用于组织工程应用,以展示新型4D生物打印应用的潜在见解。为了应对当前这项技术的挑战,我们将总结未来的观点,涉及生物支架和自组装纳米材料在生物打印的组织构建体的结合。
    Bioprinting is an additive manufacturing technique that combines living cells, biomaterials, and biological molecules to develop biologically functional constructs. Three-dimensional (3D) bioprinting is commonly used as anin vitromodeling system and is a more accurate representation ofin vivoconditions in comparison to two-dimensional cell culture. Although 3D bioprinting has been utilized in various tissue engineering and clinical applications, it only takes into consideration the initial state of the printed scaffold or object. Four-dimensional (4D) bioprinting has emerged in recent years to incorporate the additional dimension of time within the printed 3D scaffolds. During the 4D bioprinting process, an external stimulus is exposed to the printed construct, which ultimately changes its shape or functionality. By studying how the structures and the embedded cells respond to various stimuli, researchers can gain a deeper understanding of the functionality of native tissues. This review paper will focus on the biomaterial breakthroughs in the newly advancing field of 4D bioprinting and their applications in tissue engineering and regeneration. In addition, the use of smart biomaterials and 4D printing mechanisms for tissue engineering applications is discussed to demonstrate potential insights for novel 4D bioprinting applications. To address the current challenges with this technology, we will conclude with future perspectives involving the incorporation of biological scaffolds and self-assembling nanomaterials in bioprinted tissue constructs.
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  • 文章类型: Case Reports
    腭裂是口腔畸形,主要影响幼犬。它们通常是广泛的并且以骨和腭粘膜畸形为特征。这种畸形是一种严重的疾病,可能导致狗的死亡,因此建议手术治疗。通过应用无细胞生物支架作为移植物,组织生物工程已成为治疗c裂的有价值的选择。该病例报告提出了一种使用脱细胞支架通过移植技术手术矫正犬left裂的新方法。植入了去细胞化的皮肤部分,以纠正3个月大的雌性哈巴狗的大left裂。从狗尸体获得皮肤碎片并进行去细胞化方案。在全身麻醉下,对裂隙边缘的整个长度进行双侧粘骨膜分离,然后将支架放置在组织和骨腭之间。移植的支架与口腔粘膜和腭层的相互作用导致完全的裂隙闭合,无术后排斥反应或感染,表明该技术在狗腭裂矫正中的适用性。这是第一例证明这种新技术的报道,导致裂缝完全闭合和愈合。
    Cleft palates are oral deformities that mostly affect puppies. They are frequently extensive and characterized by bone and palatal mucosa malformation. This deformity is a serious condition that may result in the death of the dog, therefore surgical treatment is recommended. Tissue bioengineering has emerged as a valuable option to treat cleft palates by applying acellular biological scaffolds as grafts. This case report proposed a new approach for surgical correction of canine cleft palate through a grafting technique using a decellularized scaffold. A decellularized portion of skin was implanted to correct a large cleft palate in a 3-month-old female Pug dog. The skin fragment was obtained from a dog cadaver and a decellularization protocol was performed. Under general anesthesia, a bilateral mucoperiosteal separation of the entire length of cleft margins was performed, and the scaffold was then positioned between the tissue and the bone palate. The interaction of the grafted scaffold with the oral mucosa and palatine layers resulted in total cleft closure, without postsurgical rejection or infection, indicating the applicability of this technique in dog\'s cleft palate correction. This is the first reported case demonstrating this new technique, which resulted in full cleft closure and healing.
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  • 文章类型: Journal Article
    骨科四肢创伤的最佳治疗包括对骨和软组织损伤的精心护理。历史上,涉及软组织缺损的临床情况需要整形外科医生的协助.虽然他们在覆盖选项和微血管修复方面的专业知识非常宝贵,阻碍合作的障碍很常见。脱细胞真皮基质代表了骨科创伤外科医生保存在工具箱中的一种有前途且通用的工具。这些生物支架在如何使用和促进愈合方面都是独一无二的。这篇综述探讨了一些商业产品,并为在涉及创伤伤口的不同临床情况下的选择提供了指导。
    Optimal treatment of orthopaedic extremity trauma includes meticulous care of both bony and soft tissue injuries. Historically, clinical scenarios involving soft tissue defects necessitated the assistance of a plastic surgeon. While their expertise in coverage options and microvascular repair is invaluable, barriers preventing collaboration are common. Acellular dermal matrices represent a promising and versatile tool for orthopaedic trauma surgeons to keep in their toolbox. These biological scaffolds are each unique in how they are used and promote healing. This review explores some commercial products and offers guidance for selection in different clinical scenarios involving traumatic wounds.
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  • 文章类型: Journal Article
    背景:生物材料必须允许血运重建才能成功进行组织再生。由细胞外基质(ECM)配制的生物材料由于其优越的生物相容性而在组织工程中获得了普及,由于它们的流变特性,ECM-水凝胶可以很容易地应用于受损区域,允许细胞定植并整合到宿主组织中。猪膀胱ECM(pUBM)保留功能信号和结构蛋白,是再生医学的绝佳选择。甚至一些小分子,例如抗微生物的cathelicidin衍生的LL-37肽已被证明具有血管生成性质。
    目的:本研究的目的是评估用LL-37肽(pUBMh/LL37)生物功能化的源自猪膀胱(pUBMh)的ECM-水凝胶的生物相容性和血管生成潜力。
    方法:巨噬细胞,成纤维细胞,和脂肪组织间充质干细胞(AD-MSC)暴露于pUBMh/LL37,并通过MTT法评价其对细胞增殖的影响,通过定量乳酸脱氢酶释放和活/死细胞成像测定的细胞毒性。此外,巨噬细胞产生IL-6、IL-10、IL-12p70、MCP-1、INF-γ、使用基于珠子的细胞计数阵列定量TNF-α细胞因子。pUBMh/LL37通过背侧皮下注射直接植入Wistar大鼠24小时以评估生物相容性,和pUBMh/LL37负载的血管反应器植入21天以评估血管生成。
    结果:我们发现pUBMh/LL37不影响细胞增殖,并且与所有测试的细胞系细胞相容,但在巨噬细胞中诱导TNF-α和MCP-1的产生。在体内,这种ECM-水凝胶诱导材料内的成纤维细胞样细胞募集,在48小时没有组织损伤或炎症。有趣的是,在21天观察到血管反应器内部的血管系统的组织重塑。
    结论:我们的结果表明pUBMh/LL37在细胞学上是相容的,并在体内诱导血管生成,显示组织再生疗法的潜力。
    BACKGROUND: Biomaterials must allow revascularization for a successful tissue regeneration process. Biomaterials formulated from the extracellular matrix (ECM) have gained popularity in tissue engineering because of their superior biocompatibility, and due to their rheological properties, ECM-hydrogels can be easily applied in damaged areas, allowing cell colonization and integration into the host tissue. Porcine urinary bladder ECM (pUBM) retains functional signaling and structural proteins, being an excellent option in regenerative medicine. Even some small molecules, such as the antimicrobial cathelicidin-derived LL-37 peptide have proven angiogenic properties.
    OBJECTIVE: The objective of this study was to evaluate the biocompatibility and angiogenic potential of an ECM-hydrogel derived from the porcine urinary bladder (pUBMh) biofunctionalized with the LL-37 peptide (pUBMh/LL37).
    METHODS: Macrophages, fibroblasts, and adipose tissue-derived mesenchymal stem cells (AD-MSC) were exposed pUBMh/LL37, and the effect on cell proliferation was evaluated by MTT assay, cytotoxicity by quantification of lactate dehydrogenase release and the Live/Dead Cell Imaging assays. Moreover, macrophage production of IL-6, IL-10, IL-12p70, MCP-1, INF-γ, and TNF-α cytokines was quantified using a bead-based cytometric array. pUBMh/LL37 was implanted directly by dorsal subcutaneous injection in Wistar rats for 24 h to evaluate biocompatibility, and pUBMh/LL37-loaded angioreactors were implanted for 21 days for evaluation of angiogenesis.
    RESULTS: We found that pUBMh/LL37 did not affect cell proliferation and is cytocompatible to all tested cell lines but induces the production of TNF-α and MCP-1 in macrophages. In vivo, this ECM-hydrogel induces fibroblast-like cell recruitment within the material, without tissue damage or inflammation at 48 h. Interestingly, tissue remodeling with vasculature inside angioreactors was seen at 21 days.
    CONCLUSIONS: Our results showed that pUBMh/LL37 is cytologically compatible, and induces angiogenesis in vivo, showing potential for tissue regeneration therapies.
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  • 文章类型: Journal Article
    脂肪组织由具有有价值的结构和再生功能的细胞集合组成。作为自体移植物,这些细胞可用于解决软组织缺陷和不规则,同时还对周围组织提供修复作用。脂肪来源的干细胞或基质细胞通过直接分化成天然细胞和通过分泌刺激血管生成和破坏促炎途径的多种生长因子和细胞因子而主要负责这种再生作用。将脂肪组织分成组成部分,即,细胞,支架和蛋白质,为皮肤和软组织病理学提供了新的再生疗法,包括辐射造成的。最近在动物模型和临床试验中的研究已经证明了自体脂肪移植逆转辐射诱导的皮肤纤维化的能力。对RIF复杂病理机制的更好理解使研究人员能够利用ASCs的特定功能来设计富集的脂肪移植物构建体以改善AFG的治疗效果。
    Adipose tissue is composed of a collection of cells with valuable structural and regenerative function. Taken as an autologous graft, these cells can be used to address soft tissue defects and irregularities, while also providing a reparative effect on the surrounding tissues. Adipose-derived stem or stromal cells are primarily responsible for this regenerative effect through direct differentiation into native cells and via secretion of numerous growth factors and cytokines that stimulate angiogenesis and disrupt pro-inflammatory pathways. Separating adipose tissue into its component parts, i.e., cells, scaffolds and proteins, has provided new regenerative therapies for skin and soft tissue pathology, including that resulting from radiation. Recent studies in both animal models and clinical trials have demonstrated the ability of autologous fat grafting to reverse radiation induced skin fibrosis. An improved understanding of the complex pathologic mechanism of RIF has allowed researchers to harness the specific function of the ASCs to engineer enriched fat graft constructs to improve the therapeutic effect of AFG.
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  • 文章类型: Journal Article
    石墨烯复合材料在包括柔性电极在内的各个领域具有巨大的应用潜力,可穿戴传感器和生物医学设备由于其优异的机械和电气性能。然而,由于石墨烯在制造过程中的逐渐侵略效应,制造具有高一致性的基于石墨烯复合材料的器件仍然具有挑战性。在这里,我们提出了一种通过使用具有Weissenberg效应(EPFE)的电流体动力学印刷(EHD)从石墨/聚合物溶液中一步制造基于石墨烯/聚合物复合材料的器件的方法。产生具有高剪切速度的Taylor-Couette流以使用同轴设置在喷丝头管中的旋转钢制微针剥离高质量石墨烯。针的旋转速度的影响,探讨了喷丝头尺寸和前驱体成分对石墨烯浓度的影响。作为概念的证明,EPGW用于成功制造具有良好生物相容性的石墨烯/PCL生物支架和石墨烯/TPU应变传感器,用于检测最大应变系数超过2400的40至50%应变的人体运动。因此,该方法为石墨溶液低成本一步原位制备石墨烯/聚合物复合材料基器件提供了新的思路。 .
    Graphene composites possess great application potential in various fields including flexible electrodes, wearable sensors and biomedical devices owing to their excellent mechanical and electrical properties. However, it remains challenging to fabricate graphene composites-based devices with high consistency due to the gradual aggression effect of graphene during fabrication process. Herein, we propose a method for one-step fabricating graphene/polymer composite-based devices from graphite/polymer solution by using electrohydrodynamic (EHD) printing with the Weissenberg effect (EPWE). Taylor-Couette flows with high shearing speed were generated to exfoliate high-quality graphene with a rotating steel microneedle coaxially set in a spinneret tube. The effects of the rotating speed of the needle, spinneret size and precursor ingredients on the graphene concentration were discussed. As a proof of concept, EPWE was used to successfully fabricate graphene/polycaprolactone (PCL) bio-scaffolds with good biocompatibility and graphene/thermoplastic polyurethane strain sensor for detecting human motions with a maximum gauge factor more than 2400 from 40% to 50% strain. As such, this method sheds a new light on one-stepin situfabrication of graphene/polymer composite-based devices from graphite solution with low cost.
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  • 文章类型: Journal Article
    背景:制造具有优异的生物相容性和生物降解能力的支架的必要性已导致细胞外基质(ECM)支架的产生。在他们的优势中,它们允许更好的细胞定植,这使得它能够成功地整合到托管组织中,围绕要修复的区域及其配方有助于将其放置成不规则形状。来自猪膀胱的ECM(pUBM)包含蛋白质,蛋白聚糖和糖胺聚糖,为细胞提供支持和信号。这些特性使其成为生产可用于再生医学的水凝胶的绝佳选择。
    目的:本研究的目的是使用成纤维细胞在体外评估源自猪膀胱(pUBMh)的ECM水凝胶的生物相容性,巨噬细胞,和脂肪间充质干细胞(AD-MCSs),以及使用Wistar大鼠的体内生物相容性。
    方法:使用MTT测定法测量对细胞增殖/活力的影响,通过定量乳酸脱氢酶释放和活/死细胞成像分析来分析细胞毒性作用。巨噬细胞活化通过使用基于微球的细胞计数珠阵列定量IL-6、IL-10、IL-12p70、MCP-1和TNF-α来评估。对于体内分析,用pUBMh将Wistar大鼠接种到背侧真皮下。在接种后24小时处死样本用于组织学研究。
    结果:获得的pUBMh显示出良好的一致性和不存在细胞碎片。体外生物相容性测试表明,pUBMh促进细胞增殖,对三种测试细胞系没有细胞毒性,并诱导巨噬细胞产生促炎细胞因子,主要是TNF-α和MCP-1。在体内,pUBMh表现出成纤维细胞样细胞募集,没有组织损伤或炎症。
    结论:结果表明,pUBMh允许细胞增殖而没有细胞毒性作用,并且可以被认为是组织工程的出色生物材料。
    BACKGROUND: The necessity to manufacture scaffolds with superior capabilities of biocompatibility and biodegradability has led to the production of extracellular matrix (ECM) scaffolds. Among their advantages, they allow better cell colonization, which enables its successful integration into the hosted tissue, surrounding the area to be repaired and their formulations facilitate placing it into irregular shapes. The ECM from porcine urinary bladder (pUBM) comprises proteins, proteoglycans and glycosaminoglycans which provide support and enable signals to the cells. These properties make it an excellent option to produce hydrogels that can be used in regenerative medicine.
    OBJECTIVE: The goal of this study was to assess the biocompatibility of an ECM hydrogel derived from the porcine urinary bladder (pUBMh) in vitro using fibroblasts, macrophages, and adipose-derived mesenchymal stem cells (AD-MCSs), as well as biocompatibility in vivo using Wistar rats.
    METHODS: Effects upon cells proliferation/viability was measured using MTT assay, cytotoxic effects were analyzed by quantifying lactate dehydrogenase release and the Live/Dead Cell Imaging assay. Macrophage activation was assessed by quantification of IL-6, IL-10, IL-12p70, MCP-1, and TNF-α using a microsphere-based cytometric bead array. For in vivo analysis, Wistar rats were inoculated into the dorsal sub-dermis with pUBMh. The specimens were sacrificed at 24 h after inoculation for histological study.
    RESULTS: The pUBMh obtained showed good consistency and absence of cell debris. The biocompatibility tests in vitro revealed that the pUBMh promoted cell proliferation and it is not cytotoxic on the three tested cell lines and induces the production of pro-inflammatory cytokines on macrophages, mainly TNF-α and MCP-1. In vivo, pUBMh exhibited fibroblast-like cell recruitment, without tissue damage or inflammation.
    CONCLUSIONS: The results show that pUBMh allows cell proliferation without cytotoxic effects and can be considered an excellent biomaterial for tissue engineering.
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  • 文章类型: Journal Article
    超顺磁性氧化铁纳米粒子(SPION)因其奇特的物理化学性质和优越的生物相容性而被普遍运用于骨组织工程中。在磁场的作用下,负载于生物支架中的SPIONs能有效促进成骨细胞增殖,分化,血管生成,等等。SPIONS在骨修复中具有非常广阔的应用前景,骨重建,骨再生,和其他领域。在本文中,综述了通过SPIONs生物组装形成生物支架的几种方法,并讨论了这些生物支架在骨组织工程中的具体应用。
    Superparamagnetic iron oxide nanoparticles (SPION) are widely used in bone tissue engineering because of their unique physical and chemical properties and their excellent biocompatibility. Under the action of a magnetic field, SPIONs loaded in a biological scaffold can effectively promote osteoblast proliferation, differentiation, angiogenesis, and so on. SPIONs have very broad application prospects in bone repair, bone reconstruction, bone regeneration, and other fields. In this paper, several methods for forming biological scaffolds via the biological assembly of SPIONs are reviewed, and the specific applications of these biological scaffolds in bone tissue engineering are discussed.
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