Induced differentiation of peripheral blood hematopoietic stem cells into mature erythrocytes in vitro

doi:10.3969/j.issn.2095-4344.1800

Abstract

Abstract:

BACKGROUND: With the aging of the population and the continuous updating of medical technology, the demand for red blood cells is increasing and blood supply intends to be increasingly tight. The preparation of blood products for clinical application in vitro has become a hot spot of many experts, and hematopoietic stem cells differentiating into mature red blood cells in vitro may be an approach for new blood sources.
OBJECTIVE: To explore the practicability of using three-stage suspension culture system to induce the differentiation of peripheral blood hematopoietic stem cells from the abandoned buffy-coat into mature erythrocytes in vitro.
METHODS: The study protocol was approved by the ethics committee of Henan Red Cross Blood Center, China. CD34+ cells were isolated from peripheral blood buffy-coat, and were subsequently induced to differentiate into mature red blood cells in vitro by 21-day three-stage suspension culture system. Cell counts were performed on 4, 7, 9, 11, 13, 15, 17, 19, and 21 days of culture, and cell growth curves were then drawn. Cell smear and May-Giemsa staining were performed on 7, 11, 15, 19, and 21 days of culture, for cell morphology observation under a microscope. Flow cytometry was used to detect early erythroid differentiation on 7 days of culture and to detect terminal erythroid differentiation on 7, 11, 15, and 17 days of culture. Denucleation rate of erythroblasts was measured on 15, 17, and 19 days of culture.
RESULTS AND CONCLUSION: (1) With the increase of culture days, the number of cells showed an increasing trend, reaching a peak on 17 days of culture. The cells expanded to about 1 300 times, and then tended to be stable. (2) With the increase of culture days, the cells differentiated from proerythrocytes to basophilic erythrocytes, polychromatic erythrocytes and positive-stained erythrocytes, and almost all of the cells differentiated into denucleated erythrocytes on 21 days of culture. (3) The percentage of IL-3R/GPA double-negative cells was (15.8±0.21)%, of which erythroid burst-forming units accounted for (0.98±0.21)% and colony-forming units accounted for (8.13±1.42)%. (4) The GPA expression increased gradually with the increase of cell culture days, and about 90% of cells expressed GPA on 17 days of culture, indicating a successful erythroid differentiation of hematopoietic stem cells. (5) With the increase of culture days, the non-nuclear red blood cells increased in number, and accounted for over 80% of the cells until the 19th day of culture. To conclude, in the 21-day three-stage suspension culture system, peripheral blood hematopoietic stem cells from the abandoned buffy-coat can be induced to differentiate into mature red blood cells in vitro, with a high denucleation rate.

Key words: hematopoietic stem cells, peripheral blood, abandoned buffy-coat, mature erythrocyte, differentiation

CLC Number:

Wang Jiaojie, An Huijuan, Shan Hong, Han Xiaogai, Bie Lili, Li Jianbin. Induced differentiation of peripheral blood hematopoietic stem cells into mature erythrocytes in vitro[J]. Chinese Journal of Tissue Engineering Research, 2019, 23(29): 4662-4667.

Figures/Tables 1

2.1 细胞在三阶段悬浮培养体系中生长情况采用三阶段21 d悬浮培养体系，模拟红系发育过程，观察外周造血干细胞向成熟红细胞分化扩增情况。如图1所示，随着培养天数的增加，细胞呈增加趋势，第17天达高峰，细胞扩增到约1 300倍，之后趋于平稳。 2.2 外周血造血干细胞向成熟红细胞分化过程的形态学变化第7，11，15，19，21天取出细胞，用瑞氏-吉姆萨染色，显微镜下观察并拍照。如图2所示，随着培养天数的增加，细胞从原幼红细胞向嗜碱性幼红细胞、多染幼红细胞、正染幼红细胞分化，培养至21 d时，几乎全部分化为脱核的红细胞。整个培养体系的脱核率达到90%以上。 2.3 红系早期分化情况用流式分析仪检测样本，首先选取7AAD阴性群细胞(活细胞)，在活细胞的基础上选取IL-3R-GPA-细胞，然后在这群双阴性的细胞群中选取CD34+CD36-和CD34-CD36+细胞群，即为红系爆发集落形成单位(BFU-E)和红系祖细胞克隆形成单位(CFU-E)细胞群。培养至第7天时，IL-3R/GPA双阴性细胞占(15.8±0.21)%，其中红系爆发集落形成单位(BFU-E)占(0.98±0.21)%，红系祖细胞克隆形成单位(CFU-E)占(8.13±1.42)%，见图3。 2.4 红系终末分化情况第7天开始流式细胞仪检测红系终末分化情况，第7，11，15，17天细胞GPA表达率分别为(62.90±6.17)%，(90.40±6.44)%，(92.70±5.79)%，(96.10±2.63)%；随着细胞培养天数的增加，GPA表达也逐渐增加，培养至第17天时，接近90%的细胞表达GPA，表明造血干细胞定向红系分化较为成功。为进一步了解红系终末分化情况，在GPA阳性细胞的基础上，检测细胞膜表面分子Band3和α4-integrin的表达。结果发现膜表面标记分子Band3的表达逐渐升高，α4-integrin的表达逐渐降低，至第17天时，α4-integrinlowband3hi细胞数达90%左右，见图4。 2.5 红系晚期脱核情况 Syto16是一种核酸染料，能够透过完整的细胞膜将细胞核染上颜色。为了解细胞增殖分化过程中细胞脱核情况，在红系分化的第15，17，19天，通过流式细胞仪检测Syto16阳性细胞比例来判定红系晚期细胞脱核情况，第15，17，19天的脱核率分别为(53.98±3.49)%，(82.5±3.56)%，(91.8±2.18)%，表明随着培养天数的增加，无核红细胞越来越多，至第19天80%以上均为无核红细胞，见图5。"

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