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在流动灌注条件下双层血管移植物中的层特异性细胞分化。

Layer-specific cell differentiation in bi-layered vascular grafts under flow perfusion.

机构信息

Department of Oral and Maxillofacial Surgery & Special Dental Care, UMC Utrecht, Utrecht University, Utrecht, The Netherlands. Regenerative Medicine Center Utrecht, Utrecht, The Netherlands.

出版信息

Biofabrication. 2019 Nov 18;12(1):015009. doi: 10.1088/1758-5090/ab47f0.

Abstract

Bioengineered grafts have the potential to overcome the limitations of autologous and non-resorbable synthetic vessels as vascular substitutes. However, one of the challenges in creating these living grafts is to induce and maintain multiple cell phenotypes with a biomimetic organization. Our biomimetic grafts with heterotypic design hold promises for functional neovessel regeneration by guiding the layered cellular and tissue organization into a native-like structure. In this study, a perfusable two-compartment bioreactor chamber was designed for the further maturation of these vascular grafts, with a compartmentalized exposure of the graft's luminal and outer layer to cell-specific media. We used the system for a co-culture of endothelial colony forming cells and multipotent mesenchymal stromal cells (MSCs) in the vascular grafts, produced by combining electrospinning and melt electrowriting. It was demonstrated that the targeted cell phenotypes (i.e. endothelial cells (ECs) and vascular smooth muscle cells (vSMCs), respectively) could be induced and maintained during flow perfusion. The confluent luminal layer of ECs showed flow responsiveness, as indicated by the upregulation of COX-2, KLF2, and eNOS, as well as through stress fiber remodeling and cell elongation. In the outer layer, the circumferentially oriented, multi-layered structure of MSCs could be successfully differentiated into vSM-like cells using TGFβ, as indicated by the upregulation of αSMA, calponin, collagen IV, and (tropo)elastin, without affecting the endothelial monolayer. The cellular layers inhibited diffusion between the outer and the inner medium reservoirs. This implies tightly sealed cellular layers in the constructs, resulting in truly separated bioreactor compartments, ensuring the exposure of the inner endothelium and the outer smooth muscle-like layer to cell-specific media. In conclusion, using this system, we successfully induced layer-specific cell differentiation with a native-like cell organization. This co-culture system enables the creation of biomimetic neovessels, and as such can be exploited to investigate and improve bioengineered vascular grafts.

摘要

生物工程移植物有潜力克服自体和不可吸收的合成血管替代物的局限性。然而,在创造这些活移植物时,面临的挑战之一是诱导和维持具有仿生组织的多种细胞表型。我们具有异型设计的仿生移植物通过引导分层的细胞和组织形成类似于天然的结构,为功能性新血管再生提供了希望。在这项研究中,设计了一个可灌注的两室生物反应器室,以进一步成熟这些血管移植物,将移植物的内腔和外层分别暴露于细胞特异性培养基中。我们使用该系统对电纺丝和熔融静电纺丝相结合产生的血管移植物中的内皮集落形成细胞和多能间充质基质细胞(MSCs)进行共培养。结果表明,在流动灌注过程中可以诱导和维持靶向细胞表型(即分别为内皮细胞(ECs)和血管平滑肌细胞(vSMCs))。ECs 的腔层达到了融合状态,表现出对流动的反应性,这表现为 COX-2、KLF2 和 eNOS 的上调,以及应力纤维重塑和细胞伸长。在外层,使用 TGFβ可以将多层层状结构的 MSC 成功分化为 vSM 样细胞,这表现为αSMA、钙调蛋白、IV 型胶原和(原)弹性蛋白的上调,而不会影响内皮单层。细胞层抑制了外层和内层中间储液之间的扩散。这意味着构建物中的细胞层紧密密封,导致真正分隔的生物反应器隔室,确保内层内皮和外层平滑肌样层暴露于细胞特异性培养基中。总之,使用该系统,我们成功地诱导了具有类似天然细胞组织的层特异性细胞分化。这种共培养系统能够创建仿生新血管,并可用于研究和改进生物工程血管移植物。

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