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无辅助细胞的造血干细胞和祖细胞向成熟红细胞的分化。

Accessory-cell-free differentiation of hematopoietic stem and progenitor cells into mature red blood cells.

机构信息

Medical Affairs and Innovation, Héma-Qubec, Québec, Quebec, Canada; Centre Hospitalier Universitaire de Québec Research Center, Université Laval, Québec, Quebec, Canada.

Medical Affairs and Innovation, Héma-Qubec, Québec, Quebec, Canada.

出版信息

Cytotherapy. 2023 Nov;25(11):1242-1248. doi: 10.1016/j.jcyt.2023.07.007. Epub 2023 Aug 17.

Abstract

BACKGROUND AIMS

The culture and ex vivo engineering of red blood cells (RBCs) can help characterize genetic variants, model diseases, and may eventually spur the development of applications in transfusion medicine. In the last decade, improvements to the in vitro production of RBCs have enabled efficient erythroid progenitor proliferation and high enucleation levels from several sources of hematopoietic stem and progenitor cells (HSPCs). Despite these advances, there remains a need for refining the terminal step of in vitro human erythropoiesis, i.e., the terminal maturation of reticulocytes into erythrocytes, so that it can occur without feeder or accessory cells and animal-derived components.

METHODS

Here, we describe the near-complete erythroid differentiation of cultured RBCs (cRBCs) from adult HSPCs in accessory-cell-free and xeno-free conditions.

RESULTS

The approach improves post-enucleation cell integrity and cell survival, and it enables subsequent storage of cRBCs for up to 42 days in classical additive solution conditions without any specialized equipment.

CONCLUSIONS

We foresee that these improvements will facilitate the characterization of RBCs derived from gene-edited HSPCs.

摘要

背景目的

红细胞(RBC)的培养和体外工程有助于对遗传变异进行特征分析,建立疾病模型,最终可能会推动输血医学相关应用的发展。在过去十年中,人们对 RBC 体外生产的改进使得能够从多种造血干细胞和祖细胞(HSPC)来源中高效扩增红系祖细胞并实现高核去除水平。尽管取得了这些进展,但仍需要改进体外人红细胞生成的终末步骤,即网织红细胞向红细胞的终末成熟,使其能够在无饲养细胞或辅助细胞以及动物源性成分的情况下发生。

方法

在这里,我们描述了在无饲养细胞和无动物源条件下从成人 HSPC 中培养的 RBC(cRBC)的近乎完全红系分化。

结果

该方法提高了去核后细胞完整性和细胞存活率,并能够在没有任何特殊设备的情况下,在经典添加剂溶液条件下将 cRBC 储存长达 42 天。

结论

我们预计这些改进将有助于对基因编辑的 HSPC 衍生 RBC 进行特征分析。

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