脐血源 CD34 阳性细胞中间充质基质细胞来源对其造血支持能力的影响。
Influence of the mesenchymal stromal cell source on the hematopoietic supportive capacity of umbilical cord blood-derived CD34-enriched cells.
机构信息
Department of Bioengineering and iBB - Institute for Bioengineering and Biosciences, Instituto Superior Técnico, Universidade de Lisboa, Lisboa, Portugal.
Associate Laboratory i4HB - Institute for Health and Bioeconomy, Instituto Superior Técnico, Universidade de Lisboa, Lisboa, Portugal.
出版信息
Stem Cell Res Ther. 2021 Jul 13;12(1):399. doi: 10.1186/s13287-021-02474-8.
BACKGROUND
Umbilical cord blood (UCB) is a clinically relevant alternative source of hematopoietic stem/progenitor cells (HSPC). To overcome the low cell number per UCB unit, ex vivo expansion of UCB HSPC in co-culture with mesenchymal stromal cells (MSC) has been established. Bone marrow (BM)-derived MSC have been the standard choice, but the use of MSC from alternative sources, less invasive and discardable, could ease clinical translation of an expanded CD34 cell product. Here, we compare the capacity of BM-, umbilical cord matrix (UCM)-, and adipose tissue (AT)-derived MSC, expanded with/without xenogeneic components, to expand/maintain UCB CD34-enriched cells ex vivo.
METHODS
UCB CD34-enriched cells were isolated from cryopreserved mononuclear cells and cultured for 7 days over an established feeder layer (FL) of BM-, UCM-, or AT-derived MSC, previously expanded using fetal bovine serum (FBS) or fibrinogen-depleted human platelet lysate (HPL) supplemented medium. UCB cells were cultured in serum-free medium supplemented with SCF/TPO/FLT3-L/bFGF. Fold increase in total nucleated cells (TNC) as well as immunophenotype and clonogenic potential (cobblestone area-forming cells and colony-forming unit assays) of the expanded hematopoietic cells were assessed.
RESULTS
MSC from all sources effectively supported UCB HSPC expansion/maintenance ex vivo, with expansion factors (in TNC) superior to 50x, 70x, and 80x in UCM-, BM-, and AT-derived MSC co-cultures, respectively. Specifically, AT-derived MSC co-culture resulted in expanded cells with similar phenotypic profile compared to BM-derived MSC, but resulting in higher total cell numbers. Importantly, a subpopulation of more primitive cells (CD34CD90) was maintained in all co-cultures. In addition, the presence of a MSC FL was essential to maintain and expand a subpopulation of progenitor T cells (CD34CD7). The use of HPL to expand MSC prior to co-culture establishment did not influence the expansion potential of UCB cells.
CONCLUSIONS
AT represents a promising alternative to BM as a source of MSC for co-culture protocols to expand/maintain HSPC ex vivo. On the other hand, UCM-derived MSC demonstrated inferior hematopoietic supportive capacity compared to MSC from adult tissues. Despite HPL being considered an alternative to FBS for clinical-scale manufacturing of MSC, further studies are needed to determine its impact on the hematopoietic supportive capacity of these cells.
背景
脐带血(UCB)是一种具有临床相关性的造血干/祖细胞(HSPC)替代来源。为了克服每个 UCB 单位细胞数量低的问题,已经建立了 UCB HSPC 在与间充质基质细胞(MSC)共培养中的体外扩增。骨髓(BM)来源的 MSC 一直是标准选择,但使用来自替代来源的 MSC,侵入性更小且可丢弃,可能会促进 CD34 细胞产品的临床转化。在这里,我们比较了 BM、脐带基质(UCM)和脂肪组织(AT)来源的 MSC,在添加/不添加异种成分的情况下,体外扩增/维持 UCB CD34 富集细胞的能力。
方法
从冷冻保存的单核细胞中分离出 UCB CD34 富集细胞,并在已建立的 BM、UCM 或 AT 来源的 MSC 饲养层(FL)上培养 7 天,这些 MSC 之前使用胎牛血清(FBS)或纤维蛋白原 depleted human platelet lysate(HPL)补充培养基进行了扩增。UCB 细胞在补充有 SCF/TPO/FLT3-L/bFGF 的无血清培养基中培养。评估总核细胞(TNC)的倍增倍数以及扩增造血细胞的免疫表型和克隆形成潜力(鹅卵石形成细胞和集落形成单位测定)。
结果
所有来源的 MSC 均有效地支持 UCB HSPC 体外扩增/维持,在 UCM-、BM-和 AT 衍生 MSC 共培养中,TNC 的扩增倍数分别超过 50x、70x 和 80x。具体而言,AT 衍生的 MSC 共培养产生的扩增细胞与 BM 衍生的 MSC 具有相似的表型特征,但产生的总细胞数更高。重要的是,在所有共培养物中都维持了一个更原始细胞(CD34CD90)的亚群。此外,MSC FL 的存在对于维持和扩增祖 T 细胞(CD34CD7)的一个亚群是必不可少的。在建立共培养之前使用 HPL 扩增 MSC 并不会影响 UCB 细胞的扩增潜力。
结论
AT 是 BM 的一种有前途的替代来源,可作为用于体外扩增/维持 HSPC 的 MSC 共培养方案的来源。另一方面,与成人组织来源的 MSC 相比,UCM 衍生的 MSC 表现出较差的造血支持能力。尽管 HPL 被认为是 FBS 的替代品,用于 MSC 的临床规模制造,但需要进一步研究来确定其对这些细胞的造血支持能力的影响。
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