Department of Oncology, Lombardi Comprehensive Cancer Center, Georgetown University Medical Center, Washington, District of Columbia, USA.
Health Research Governance Department, Ministry of Public Health, Qatar.
Cell Cycle. 2022 Apr;21(7):655-673. doi: 10.1080/15384101.2021.2020015. Epub 2022 Mar 15.
Human amniotic epithelial cells (hAECs), derived from an epithelial cell layer of the human amniotic membrane, possess embryonic stem-like properties and are known to maintain multilineage differentiation potential. Unfortunately, an inability to expand hAECs without significantly compromising their stem cell potency has precluded their widespread use for regenerative therapies. This article critically evaluates the methods used for isolation, expansion, and cryopreservation of hAECs. We assessed the impact of these methods on ex-vivo expansion and stem cell phenotype of hAECs. Moreover, the progress and challenges to optimize clinically suitable culture conditions for an efficient ex-vivo expansion and storage of these cells are highlighted. Additionally, we also reviewed the currently used hAECs isolation and characterization methods employed in clinical trials. Despite the developments made in the last decade, significant challenges still exist to overcome limitations of ex-vivo expansion and retention of stemness of hAECs in both xenogeneic and xenofree culture conditions. Therefore, optimization and standardization of culture conditions for robust ex-vivo maintenance of hAECs without affecting tissue regenerative properties is an absolute requirement for their successful therapeutic manipulation. This review may help the researchers to optimize the methods that support ex-vivo survival, proliferation, and self-renewal properties of the hAECs. AM: Human amniotic membrane; CM-HBSS: Ca and Mg free HBSS; DMEM: Dulbecco's Modified Eagle Medium; DMEM-HG: DMEM-high glucose; EMEM: Eagle's Modified Essential Medium; EMT: Epithelial-to-mesenchymal transition; EpM: Epi-life complete media; ESC: Embryonic stem cells; ESCM: Epithelial cell surface markers; hAECs: Human amniotic epithelial cells; HLA: Human leukocyte antigen; IM: Immunogenicity markers; iPSC: Induced pluripotent stem cells; KOSR; KSR: Knockout serum replacement; KSI: Key success indicators; CHM: Cell heterogeneity markers; Nanog: NANOG homeobox; Oct-4: Octamer binding transcription factor 4; OR: Operation room; P: Passage; PM: Pluripotency markers; SCM: Stem cell markers for non-differentiated cells; Sox-2: Sry-related HMG box gene 2; SSEA-4: Stage-specific embryonic antigen; TRA: Tumor rejection antigen; UC: Ultra-culture; XF: Xenogeneic free.
人羊膜上皮细胞(hAECs)来源于人羊膜的上皮细胞层,具有胚胎干细胞样特性,已知能够维持多能分化潜能。不幸的是,由于无法在不显著降低其干细胞活力的情况下扩增 hAECs,因此限制了其在再生疗法中的广泛应用。本文批判性地评估了分离、扩增和冷冻保存 hAECs 的方法。我们评估了这些方法对 hAECs 体外扩增和干细胞表型的影响。此外,还强调了优化这些细胞临床适用培养条件以实现高效体外扩增和储存的进展和挑战。此外,我们还回顾了临床试验中目前使用的 hAECs 分离和表征方法。尽管在过去十年中取得了进展,但在异种和无异种培养条件下克服 hAECs 体外扩增和维持干细胞特性的限制方面仍存在重大挑战。因此,优化和标准化培养条件,以在不影响组织再生特性的情况下实现 hAECs 的稳健体外维持,是其成功治疗操作的绝对要求。本文综述可能有助于研究人员优化支持 hAECs 体外存活、增殖和自我更新特性的方法。AM:人羊膜;CM-HBSS:无钙镁 HBSS;DMEM:杜尔贝科改良伊格尔培养基;DMEM-HG:DMEM-高葡萄糖;EMEM:Eagle's Modified Essential Medium;EMT:上皮-间充质转化;EpM:Epi-life 完整培养基;ESC:胚胎干细胞;ESCM:上皮细胞表面标志物;hAECs:人羊膜上皮细胞;HLA:人类白细胞抗原;IM:免疫原性标志物;iPSC:诱导多能干细胞;KOSR;KSR:无血清替代物;KSI:关键成功指标;CHM:细胞异质性标志物;Nanog:NANOG 同源盒;Oct-4:八聚体结合转录因子 4;OR:手术室;P:传代;PM:多能标志物;SCM:未分化细胞的干细胞标志物;Sox-2:Sry-related HMG box gene 2;SSEA-4:阶段特异性胚胎抗原;TRA:肿瘤排斥抗原;UC:超培养;XF:无异种。
