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生物墨水的钙补充减少了生物打印过程中剪切应力引起的细胞损伤。

Calcium supplementation of bioinks reduces shear stress-induced cell damage during bioprinting.

机构信息

Department of Physics, University of Erlangen-Nuremberg, Erlangen, Germany.

Institute of Biomaterials, Department of Materials Science and Engineering, University of Erlangen-Nuremberg, Erlangen, Germany.

出版信息

Biofabrication. 2022 Aug 11;14(4). doi: 10.1088/1758-5090/ac84af.

Abstract

During bioprinting, cells are suspended in a viscous bioink and extruded under pressure through small diameter printing needles. The combination of high pressure and small needle diameter exposes cells to considerable shear stress, which can lead to cell damage and death. Approaches to monitor and control shear stress-induced cell damage are currently not well established. To visualize the effects of printing-induced shear stress on plasma membrane integrity, we add FM 1-43 to the bioink, a styryl dye that becomes fluorescent when bound to lipid membranes, such as the cellular plasma membrane. Upon plasma membrane disruption, the dye enters the cell and also stains intracellular membranes. Extrusion of alginate-suspended NIH/3T3 cells through a 200m printing needle led to an increased FM 1-43 incorporation at high pressure, demonstrating that typical shear stresses during bioprinting can transiently damage the plasma membrane. Cell imaging in a microfluidic channel confirmed that FM 1-43 incorporation is caused by cell strain. Notably, high printing pressure also impaired cell survival in bioprinting experiments. Using cell types of different stiffnesses, we find that shear stress-induced cell strain, FM 1-43 incorporation and cell death were reduced in stiffer compared to softer cell types and demonstrate that cell damage and death correlate with shear stress-induced cell deformation. Importantly, supplementation of the suspension medium with physiological concentrations of CaClgreatly reduced shear stress-induced cell damage and death but not cell deformation. As the sudden influx of calcium ions is known to induce rapid cellular vesicle exocytosis and subsequent actin polymerization in the cell cortex, we hypothesize that calcium supplementation facilitates the rapid resealing of plasma membrane damage sites. We recommend that bioinks should be routinely supplemented with physiological concentrations of calcium ions to reduce shear stress-induced cell damage and death during extrusion bioprinting.

摘要

在生物打印过程中,细胞悬浮在粘性生物墨水中,并在高压下通过小直径打印针挤出。高压和小针直径的组合会使细胞暴露在相当大的剪切应力下,从而导致细胞损伤和死亡。目前尚未建立监测和控制剪切应力诱导的细胞损伤的方法。为了观察打印诱导的剪切应力对质膜完整性的影响,我们在生物墨水中添加 FM 1-43,这是一种吖啶染料,与脂质膜(如细胞质膜)结合时会发出荧光。在质膜破裂时,染料进入细胞并染色细胞内膜。将悬浮在藻酸盐中的 NIH/3T3 细胞通过 200m 的打印针挤出会导致在高压下 FM 1-43 的结合增加,表明生物打印过程中的典型剪切应力会短暂破坏质膜。在微流控通道中的细胞成像证实,FM 1-43 的结合是由细胞应变引起的。值得注意的是,高打印压力也会损害生物打印实验中的细胞存活率。使用不同刚度的细胞类型,我们发现与较软的细胞类型相比,剪切应力诱导的细胞应变、FM 1-43 结合和细胞死亡减少,并且证明细胞损伤和死亡与剪切应力诱导的细胞变形相关。重要的是,在悬浮介质中补充生理浓度的 CaClgreatly 减少了剪切应力诱导的细胞损伤和死亡,但没有减少细胞变形。由于钙离子的突然涌入已知会诱导细胞皮层中快速的囊泡胞吐和随后的肌动蛋白聚合,我们假设钙补充剂有助于快速修复质膜损伤部位。我们建议在挤出式生物打印过程中,生物墨应常规补充生理浓度的钙离子,以减少剪切应力诱导的细胞损伤和死亡。

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