确定并优化大规模制造 iPSC 衍生胰岛素分泌 β 细胞的关键工艺参数。

IF 7.1 2区医学 Q1 CELL & TISSUE ENGINEERING

Stem Cell Research & Therapy Pub Date : 2024-11-09 DOI:10.1186/s13287-024-03973-0

Haneen Yehya, Alexandra Wells, Michael Majcher, Dhruv Nakhwa, Ryan King, Faruk Senturk, Roshan Padmanabhan, Jan Jensen, Michael A Bukys

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引用次数: 0

摘要

背景：1 型糖尿病是一种导致胰腺 β 细胞破坏的自身免疫性疾病，需要终生接受胰岛素治疗。胰岛移植是一种很有前景的解决方案，但面临着可用性有限和需要免疫抑制等挑战。诱导多能干细胞（iPSCs）为功能性β细胞提供了潜在的替代来源，并具有大规模生产的能力。然而，目前的分化方案主要在混合或二维环境中进行，缺乏可扩展性和悬浮培养的最佳条件：方法：我们研究了一系列可能影响分化过程的生物反应器放大工艺参数和目标产品质量曲线。这项研究采用了优化的高维实验设计（HD-DoE）方案，该方案是为可扩展性而设计的，并在 0.5 升（PBS-0.5 Mini）垂直轮式生物反应器中实施：结果：开发了一种三阶段悬浮制造工艺，从粘附培养过渡到悬浮培养，在扩展过程中使用 TB2 培养基支持 iPSC 生长。采用分阶段优化方法和延长分化时间，以提高 iPSC 衍生的小岛状集群的标记表达和成熟度。连续生物反应器运行用于研究营养和生长限制以及对分化的影响。连续生物反应器与控制介质变化生物反应器进行了比较，结果显示了新陈代谢的变化和更类似于β细胞的分化特征。从运行中收获的低温保存聚合体被回收，并在回收后保持了活力和胰岛素分泌能力，这表明它们具有储存和未来移植疗法的潜力：本研究表明，阶段时间的增加和乳酸盐积累的有限培养基补充可提高在大规模悬浮环境中培养的胰岛素分泌细胞的分化能力。

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Identifying and optimizing critical process parameters for large-scale manufacturing of iPSC derived insulin-producing β-cells.

Background: Type 1 diabetes, an autoimmune disorder leading to the destruction of pancreatic β-cells, requires lifelong insulin therapy. Islet transplantation offers a promising solution but faces challenges such as limited availability and the need for immunosuppression. Induced pluripotent stem cells (iPSCs) provide a potential alternative source of functional β-cells and have the capability for large-scale production. However, current differentiation protocols, predominantly conducted in hybrid or 2D settings, lack scalability and optimal conditions for suspension culture.

Methods: We examined a range of bioreactor scaleup process parameters and quality target product profiles that might affect the differentiation process. This investigation was conducted using an optimized High Dimensional Design of Experiments (HD-DoE) protocol designed for scalability and implemented in 0.5L (PBS-0.5 Mini) vertical wheel bioreactors.

Results: A three stage suspension manufacturing process is developed, transitioning from adherent to suspension culture, with TB2 media supporting iPSC growth during scaling. Stage-wise optimization approaches and extended differentiation times are used to enhance marker expression and maturation of iPSC-derived islet-like clusters. Continuous bioreactor runs were used to study nutrient and growth limitations and impact on differentiation. The continuous bioreactors were compared to a Control media change bioreactor showing metabolic shifts and a more β-cell-like differentiation profile. Cryopreserved aggregates harvested from the runs were recovered and showed maintenance of viability and insulin secretion capacity post-recovery, indicating their potential for storage and future transplantation therapies.

Conclusion: This study demonstrated that stage time increase and limited media replenishing with lactate accumulation can increase the differentiation capacity of insulin producing cells cultured in a large-scale suspension environment.

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来源期刊

Stem Cell Research & Therapy CELL BIOLOGY-MEDICINE, RESEARCH & EXPERIMENTAL

CiteScore

13.20

自引率

8.00%

发文量

525

审稿时长

1 months

期刊介绍： Stem Cell Research & Therapy serves as a leading platform for translational research in stem cell therapies. This international, peer-reviewed journal publishes high-quality open-access research articles, with a focus on basic, translational, and clinical research in stem cell therapeutics and regenerative therapies. Coverage includes animal models and clinical trials. Additionally, the journal offers reviews, viewpoints, commentaries, and reports.