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Two-step sedimentation process for selection of microcapsules containing cell aggregates

机译:两步沉降过程,用于选择含细胞聚集体的微胶囊

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Microencapsulation technologies are being developed to protect transplanted islets from immune rejection, to reduce or even eliminate the need for immunosuppression. However, unencapsulated cells increase the chances of rejection and empty beads increase transplant volumes. Thus, separation processes were investigated to remove these byproducts based on density differences. The densities of islet-sized mouse insulinoma 6 (MIN6) cell aggregates and acellular 5% alginate beads generated via emulsification and internal gelation were similar to 1.065 and 1.042 g/ml, respectively. The separation of empty beads from those containing aggregates was performed by sedimentation under unit gravity in continuous gradients of polysucrose and sodium diatrizoate with density ranges of 1.032-1.045, 1.035-1.044, or 1.039-1.042 g/ml. The 1.039-1.042 g/ml gradient enabled recoveries of similar to 80% of the aggregate-containing beads while the other gradients recovered only similar to 60%. The bottom fraction of the 1.039-1.042 g/ml gradient contained beads with similar to 6% of their volume occupied by cell aggregates. Separation of unencapsulated aggregates from the aggregate-containing beads was then achieved by centrifugation of this purified fraction in a 1.055 g/ml density solution. Thus, these sedimentation-based approaches can effectively remove the byproducts of cell encapsulation.
机译:正在开发微胶囊化技术以保护移植的胰岛免受免疫排斥,以减少甚至消除对免疫抑制的需要。然而,未封装的细胞增加了排斥和空珠的机会增加移植体积。因此,研究了分离过程以基于密度差除去这些副产物。胰岛大小的小鼠胰岛素瘤6(MIN6)细胞聚集体和通过乳化和内凝胶产生的细胞5%藻酸盐珠粒的密度分别与1.065和1.042g / mL相似。通过在单位重力下在连续梯度的聚核和脱噻吩的单位重力下沉淀来进行空珠的分离,密度范围为1.032-1.045,1.035-1.044或1.039-1.042g / ml。 1.039-1.042 g / ml梯度使得具有与含聚集珠的80%相似的回收率,而另一个梯度恢复仅类似于60%。 1.039-1.042g / ml梯度的底部含有珠子,其珠子与细胞聚集体占据的6%相似。然后通过以1.055g / ml密度溶液离心该纯化的馏分来实现来自含聚集体珠子的未封闭的聚集体。因此,这些基于沉降的方法可以有效地去除细胞包封的副产物。

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