Maria C Naskou, Anna Cochran, Nikolia Darzenta, Morgane E Golan, Steven L Stice, Douglas R Martin
{"title":"从骨髓和脐带间充质基质细胞中提取的细胞外小泡的特征和功能受细胞培养条件的影响。","authors":"Maria C Naskou, Anna Cochran, Nikolia Darzenta, Morgane E Golan, Steven L Stice, Douglas R Martin","doi":"10.1089/scd.2023.0229","DOIUrl":null,"url":null,"abstract":"<p><p>Extracellular vesicles (EVs) derived from mesenchymal stromal cells (MSC-EVs) have been proposed as a novel therapeutic tool with numerous clinically related advantages. However, their characteristics and functionality are dependent on the source of MSCs and their cell culture conditions. Fetal bovine serum (FBS) provides a source of nutrients and growth factors to the cultured cells. However, certain pitfalls are associated with its supplementation to the culture media, including introduction of exogenous FBS-derived EVs to the cultured cells. Thus, recent practices recommend utilization of serum-free (SF) media or EV-depleted FBS. On the contrary, evidence suggests that the immunomodulatory ability of MSC-EVs can be improved by exposing MSCs to an inflammatory (IF) environment. The objective of this study was to (1) compare EVs isolated from two tissue sources of MSCs that were exposed to various cell culture conditions and (2) to evaluate their anti-inflammatory effects. Bone marrow-derived mesenchymal stromal cells (BM-MSCs) and umbilical cord-derived mesenchymal stromal cells (UC-MSCs) were exposed to either a SF media environment, an IF environment, or media supplemented with 5% EV-depleted FBS. Following isolation of MSC-EVs, the isolates were quantified and evaluated for particle size, phenotypic changes, and their immunomodulatory potential. A statistically significant difference was not identified on the yield and protein concentration of different isolates of EVs from BM-MSCs and UC-MSCs, and all isolates had a circular appearance as evaluated via electron microscopy. A significant difference was identified on the phenotype of different EVs isolates; however, all isolates expressed classical markers such as CD9, CD63, and CD81. The addition of BM-derived MSC-EVs from FBS environment or UC-derived MSC-EVs from IF environment resulted in statistically significant downregulation of IL-6 messenger RNA (mRNA) in stimulated leukocytes. 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引用次数: 0
摘要
从间充质基质细胞(MSCs-EVs)中提取的细胞外囊泡(EVs)被认为是一种新型的治疗工具,具有许多临床相关的优势。然而,它们的特性和功能取决于间充质干细胞的来源及其细胞培养条件。胎牛血清(FBS)可为培养细胞提供营养和生长因子。然而,在培养基中补充胎牛血清会带来一些隐患,包括向培养细胞中引入外源性胎牛血清衍生的EVs。因此,最近的实践建议使用无血清培养基或去掉 EV 的 FBS。另一方面,有证据表明,将间叶干细胞暴露在炎症环境中可提高间叶干细胞-EV 的免疫调节能力。本研究的目的是:a)比较从两种间充质干细胞组织来源中分离出来的暴露于不同细胞培养条件下的EV;b)评估它们的抗炎作用。骨髓(BM)和脐带(UC)来源的间充质干细胞分别暴露于无血清(SF)培养基环境、炎症(IF)环境或补充了 5%去除了 EV 的 FBS 的培养基中。在分离间充质干细胞-EV后,对分离物进行量化,并评估其粒径、表型变化及其免疫调节潜力。从 BM-MSCs 和 UC-MSCs 分离出的不同 EVs 在产量和蛋白质浓度上没有发现明显的统计学差异,通过电子显微镜评估,所有分离物均呈圆形外观。不同EVs分离物的表型存在明显差异,但所有分离物均表达CD9、CD63和CD81等经典标记物。加入来自 FBS 环境的 BM 间充质干细胞-EVs 或来自 IF 环境的 UC 间充质干细胞-EVs 后,受刺激白细胞的 IL-6 mRNA 在统计学上有明显下调。这项研究证实,不同间充质干细胞来源和细胞培养条件产生的EV会影响其表型及其免疫调节能力。
The Characteristics and Function of Small Extracellular Vesicles Derived from Human Bone Marrow and Umbilical Cord Mesenchymal Stromal Cells Are Influenced by Cell Culture Conditions.
Extracellular vesicles (EVs) derived from mesenchymal stromal cells (MSC-EVs) have been proposed as a novel therapeutic tool with numerous clinically related advantages. However, their characteristics and functionality are dependent on the source of MSCs and their cell culture conditions. Fetal bovine serum (FBS) provides a source of nutrients and growth factors to the cultured cells. However, certain pitfalls are associated with its supplementation to the culture media, including introduction of exogenous FBS-derived EVs to the cultured cells. Thus, recent practices recommend utilization of serum-free (SF) media or EV-depleted FBS. On the contrary, evidence suggests that the immunomodulatory ability of MSC-EVs can be improved by exposing MSCs to an inflammatory (IF) environment. The objective of this study was to (1) compare EVs isolated from two tissue sources of MSCs that were exposed to various cell culture conditions and (2) to evaluate their anti-inflammatory effects. Bone marrow-derived mesenchymal stromal cells (BM-MSCs) and umbilical cord-derived mesenchymal stromal cells (UC-MSCs) were exposed to either a SF media environment, an IF environment, or media supplemented with 5% EV-depleted FBS. Following isolation of MSC-EVs, the isolates were quantified and evaluated for particle size, phenotypic changes, and their immunomodulatory potential. A statistically significant difference was not identified on the yield and protein concentration of different isolates of EVs from BM-MSCs and UC-MSCs, and all isolates had a circular appearance as evaluated via electron microscopy. A significant difference was identified on the phenotype of different EVs isolates; however, all isolates expressed classical markers such as CD9, CD63, and CD81. The addition of BM-derived MSC-EVs from FBS environment or UC-derived MSC-EVs from IF environment resulted in statistically significant downregulation of IL-6 messenger RNA (mRNA) in stimulated leukocytes. This study confirms that EVs produced by different MSC sources and cell culture conditions affect their phenotype and their immunomodulatory capacities.