一种用于细胞微模式系统的无异种培养基,作为潜在临床应用的细胞指导性生物材料。

Hui Che, Melanie L Hart, Jasmin C Lauer, Mischa Selig, Marita Voelker, Bodo Kurz, Bernd Rolauffs
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引用次数: 0

摘要

细胞微模式控制着细胞的命运和功能,并有可能产生具有精确功能的可用于治疗的间充质基质细胞(MSC)群体。然而,到目前为止,在翻译环境中人类细胞的微模式是不可能的,因为只有反刍动物培养基补充剂,例如胎牛血清(FBS),被确定用于微模式(MPs)。因此,目前没有符合GMP的介质可用于微图案(MPs)。本研究测试了一种不含异种的人血浆和血小板裂解液(hP+PL)培养基补充剂,以确定其与MPs的相容性。未经过滤的hP+PL培养基导致大量蛋白质沉积,形成“地毯状”层,使MPs无效。过滤(3×/5×)消除了这种影响。重要的是,使用微滴数字PCR的定量比较显示,所有培养基类型的人间充质干细胞表现出相似的图谱,具有强肌(CNN1/TAGLN2)和弱成骨(ALPL/RUNX2)标记表达,以及更弱的脂肪(LPL/PPARG)和软骨(COL2A1/ACAN)表达,且图谱以肌源性标记为主。在这些相似的谱中,与含fbs的培养基相比,所有hP+PL-对肌源性标记TAGLN2的诱导作用更强。总的来说,这表明FBS可以用hP+PL代替,而不会改变分化特征。然而,评估个体MSC对各种MP类型的反应并定义分类显示未过滤的hP+PL培养基是不可用的。重要的是,FBS-和3x过滤的hP+PL培养基在每个分化类别中具有可比性。综上所述,本研究推荐3倍过滤的hP+PL作为基础和转化研究中微模式细胞群的培养基补充,作为无异种和潜在的GMP符合FBS的替代品,以确保一致和可靠的MSC微模式用于治疗。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A xenogenic-free culture medium for cell micro-patterning systems as cell-instructive biomaterials for potential clinical applications.

Cell micro-patterning controls cell fate and function and has potential for generating therapeutically usable mesenchymal stromal cell (MSC) populations with precise functions. However, to date, the micro-patterning of human cells in a translational context has been impossible because only ruminant media supplements, e.g. fetal bovine serum (FBS), are established for use with micro-patterns (MPs). Thus, there are currently no good manufacturing practice (GMP)-compliant media available for MPs. This study tested a xenogenic-free human plasma and platelet lysate (hP + PL) medium supplement to determine its compatibility with MPs. Unfiltered hP + PL medium resulted in significant protein deposition, creating a 'carpet-like' layer that rendered MPs ineffective. Filtration (3×/5×) eliminated this effect. Importantly, quantitative comparison using droplet digital PCR revealed that human MSCs in all media types exhibited similar profiles with strong myogenic Calponin 1/Transgelin 2 (TAGLN2) and weaker osteogenic alkaline phosphatase/Runt-related transcription factor 2 marker expression, and much weaker adipogenic (lipoprotein lipase/peroxisome proliferator-activated receptor gamma) and chondrogenic (collagen type II/aggrecan) expression, with profiles being dominated by myogenic markers. Within these similar profiles, an even stronger induction of the myogenic marker TAGLN2 by all hP + PL- compared to FBS-containing media. Overall, this suggested that FBS can be replaced with hP + PL without altering differentiation profiles. However, assessing individual MSC responses to various MP types with defined categories revealed that unfiltered hP + PL medium was unusable. Importantly, FBS- and 3× filtered hP + PL media were comparable in each differentiation category. Summarized, this study recommends 3× filtered hP + PL as a xenogenic-free and potentially GMP-compliant alternative to FBS as a culture medium supplement for micro-patterning cell populations in both basic and translational research that will ensure consistent and reliable MSC micro-patterning for therapeutic use.

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