Increasing Collagen to Bioink Drives Mesenchymal Stromal Cells-Chondrogenesis from Hyaline to Calcified Layers.

IF 3.5 3区 医学 Q3 CELL & TISSUE ENGINEERING Tissue Engineering Part A Pub Date : 2024-06-01 Epub Date: 2023-11-30 DOI:10.1089/ten.TEA.2023.0178
Océane Messaoudi, Christel Henrionnet, Edwin-Joffrey Courtial, Laurent Grossin, Didier Mainard, Laurent Galois, Damien Loeuille, Christophe Marquette, Pierre Gillet, Astrid Pinzano
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Abstract

The bioextrusion of mesenchymal stromal cells (MSCs) directly seeded in a bioink enables the production of three-dimensional (3D) constructs, promoting their chondrogenic differentiation. Our study aimed to evaluate the effect of different type I collagen concentrations in the bioink on MSCs' chondrogenic differentiation. We printed 3D constructs using an alginate, gelatin, and fibrinogen-based bioink cellularized with MSCs, with four different quantities of type I collagen addition (0.0, 0.5, 1.0, and 5.0 mg per bioink syringe). We assessed the influence of the bioprinting process, the bioink composition, and the growth factor (TGF-ꞵ1) on the MSCs' survival rate. We confirmed the biocompatibility of the process and the bioinks' cytocompatibility. We evaluated the chondrogenic effects of TGF-ꞵ1 and collagen addition on the MSCs' chondrogenic properties through macroscopic observation, shrinking ratio, reverse transcription polymerase chain reaction, glycosaminoglycan synthesis, histology, and type II collagen immunohistochemistry. The bioink containing 0.5 mg of collagen produces the richest hyaline-like extracellular matrix, presenting itself as a promising tool to recreate the superficial layer of hyaline cartilage. The bioink containing 5.0 mg of collagen enhances the synthesis of a calcified matrix, making it a good candidate for mimicking the calcified cartilaginous layer. Type I collagen thus allows the dose-dependent design of specific hyaline cartilage layers.

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增加胶原到生物墨水驱动MSCs软骨形成从透明层到钙化层。
直接接种在生物墨水中的间充质基质细胞(MSC)的生物挤出能够产生3D构建体,促进其软骨分化。我们的研究旨在评估生物墨水中不同I型胶原浓度对MSCs软骨分化的影响。我们使用用MSC细胞化的基于藻酸盐、明胶和纤维蛋白原的生物墨水打印3D构建体,添加了四种不同量的I型胶原(每个生物墨水注射器0.0、0.5、1.0和5.0 mg)。我们评估了生物打印过程、生物墨水成分和生长因子(TGF-ꞵ1) 对MSC的存活率的影响。我们确认了该工艺的生物相容性和生物墨水的细胞相容性。我们评估了转化生长因子的软骨形成作用-ꞵ1和胶原添加对MSCs软骨形成特性的影响,通过宏观观察、收缩率、RT-PCR、糖胺聚糖合成、组织学和II型胶原免疫组织化学。含有0.5毫克胶原蛋白的生物墨水产生了最丰富的透明质样细胞外基质,是重建透明质软骨表层的一种很有前途的工具。含有5.0毫克胶原蛋白的生物墨水可以增强钙化基质的合成,使其成为模拟钙化软骨层的良好候选者。因此,I型胶原允许特定透明软骨层的剂量依赖性设计。
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来源期刊
Tissue Engineering Part A
Tissue Engineering Part A Chemical Engineering-Bioengineering
CiteScore
9.20
自引率
2.40%
发文量
163
审稿时长
3 months
期刊介绍: Tissue Engineering is the preeminent, biomedical journal advancing the field with cutting-edge research and applications that repair or regenerate portions or whole tissues. This multidisciplinary journal brings together the principles of engineering and life sciences in the creation of artificial tissues and regenerative medicine. Tissue Engineering is divided into three parts, providing a central forum for groundbreaking scientific research and developments of clinical applications from leading experts in the field that will enable the functional replacement of tissues.
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