Aizman Irina, Tirumalashetty Brenna J, McGrogan Michael, Case Casey C
Stem Cell Res Ther. 2014 Feb 26;5(1):29. doi: 10.1186/scrt418.
Transplanting mesenchymal stromal cells (MSCs) or their derivatives into a neurodegenerative environment is believed to be beneficial because of the trophic support, migratory guidance, immunosuppression, and neurogenic stimuli they provide. SB623, a cell therapy for the treatment of chronic stroke, currently in a clinical trial, is derived from bone marrow MSCs by using transient transfection with a vector encoding the human Notch1 intracellular domain. This creates a new phenotype, which is effective in experimental stroke, exhibits immunosuppressive and angiogenic activity equal or superior to parental MSCs in vitro, and produces extracellular matrix (ECM) that is exceptionally supportive for neural cell growth. The neuropoietic activity of SB623 and parental MSCs has not been compared, and the SB623-derived neuropoietic mediators have not been identified.
SB623 or parental MSCs were cocultured with rat embryonic brain cortex cells on cell-derived ECM in a previously characterized quantitative neuropoiesis assay. Changes in expression of rat neural differentiation markers were quantified by using rat-specific qRT-PCR. Human mediators were identified by using expression profiling, an enzymatic crosslinking activity, and functional interference studies by means of blocking antibodies, biologic inhibitors, and siRNA. Cocultures were immunolabeled for presynaptic vesicular transporters to assess neuronal specialization.
Among six MSC/SB623 pairs, SB623 induced expression of rat neural precursor, oligodendrocyte, and astrocyte markers on average 2.6 to 3 times stronger than did their parental MSCs. SB623 expressed significantly higher FGF2, FGF1, and BMP4, and lower FGFR1 and FGFR2 levels; and human FGF1, FGF2, BMPs, and HGF were implicated as neuropoietic mediators. Neural precursors grew faster on SB623- than on MSC-derived ECM. SB623 exhibited higher expression levels and crosslinking activity of tissue transglutaminase (TGM2). TGM2 silencing reduced neural precursor growth on SB623-ECM. SB623 also promoted the induction of GABA-ergic, but not glutamatergic, neurons more effectively than did MSCs.
These data demonstrate that SB623 cells tend to support neural cell growth more effectively than their parental MSCs and identify both soluble and insoluble mediators responsible, at least in part, for enhanced neuropoietic potency of SB623. The neuropoiesis assay is a useful tool for identifying beneficial factors produced by MSCs and their derivatives.
将间充质基质细胞(MSC)或其衍生物移植到神经退行性环境中被认为是有益的,因为它们能提供营养支持、迁移引导、免疫抑制和神经源性刺激。SB623是一种用于治疗慢性中风的细胞疗法,目前正处于临床试验阶段,它是通过用编码人Notch1细胞内结构域的载体进行瞬时转染,从骨髓MSC中衍生而来。这创造了一种新的表型,在实验性中风中有效,在体外表现出与亲代MSC相当或更强的免疫抑制和血管生成活性,并产生对神经细胞生长特别有支持作用的细胞外基质(ECM)。尚未比较SB623和亲代MSC的神经生成活性,也未鉴定出SB623衍生的神经生成介质。
在先前已表征的定量神经生成测定中,将SB623或亲代MSC与大鼠胚胎脑皮质细胞在细胞衍生的ECM上共培养。使用大鼠特异性qRT-PCR对大鼠神经分化标志物的表达变化进行定量。通过表达谱分析、酶促交联活性以及使用阻断抗体、生物抑制剂和siRNA进行的功能干扰研究来鉴定人类介质。对共培养物进行突触前囊泡转运体免疫标记以评估神经元特化。
在六对MSC/SB623中,SB623诱导大鼠神经前体、少突胶质细胞和星形胶质细胞标志物的表达,平均比其亲代MSC强2.6至3倍。SB623表达的FGF2、FGF1和BMP4水平显著更高,而FGFR1和FGFR2水平更低;并且人FGF1、FGF2、骨形态发生蛋白(BMP)和肝细胞生长因子(HGF)被认为是神经生成介质。神经前体在SB623衍生的ECM上比在MSC衍生的ECM上生长得更快。SB623表现出更高的组织转谷氨酰胺酶(TGM2)表达水平和交联活性。TGM2沉默降低了神经前体在SB623-ECM上的生长。SB623还比MSC更有效地促进GABA能神经元而非谷氨酸能神经元的诱导。
这些数据表明,SB623细胞比其亲代MSC更倾向于有效地支持神经细胞生长,并确定了至少部分负责增强SB623神经生成能力的可溶性和不可溶性介质。神经生成测定是鉴定MSC及其衍生物产生的有益因子的有用工具。
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