Zhao Sheng-ming, Gu Xi-chun, Chang Nai-bai, Clackson Tim, Blau C Anthony
Department of Hematology, Beijing Hospital, Beijing 100730, China.
Zhonghua Xue Ye Xue Za Zhi. 2004 Feb;25(2):65-9.
To explore the feasibility of regulated expansion and committed differentiation potential of JAK2 gene modified hematopoietic stem/progenitor cells in vitro.
A murine stem cell virus (MSCV) based retroviral vector MGI-F2Jak2, which encodes a green fluorescent protein (GFP) and a fusion protein containing two copies of modified FK506 binding protein (F36v) linked tyrosine kinase JAK2 was cloned. F36v served as a high-affinity binding site for dimerizer AP20187. GpE + 86 packaging cell was transfected with this vector. Bone marrow cells from C57BL/6 mice were transduced by co-cultured with irradiated (1500 cGy) GpE + 86 producer clone for 48 h. Transduced marrow cells were expanded in X-VIVO 15 and divided into four groups as follows: (1) control group; (2) AP20187 alone group; (3) SCF alone group and (4) AP20187 + SCF group. The phenotypes of the expanded cells were analyzed by directly phycoerythrin-labeled anti-Sca1, c-kit, CD(34), Gr1, CD(11b), TER119, CD(41), B220 and CD(3) monoclonal antibodies for flow cytometry. Committed differentiation, progenitor colony assay and spleen colony forming units (CFU-S) were further evaluated.
A significant sustained outgrowth of transduced marrow cells was obtained only in the AP20187 + SCF group. Cells expanded up to 10(14)-fold after 80 days culture. The doubling time was about 30 hs. The phenotypes of the expanded cells were homogeneously strong positive for CD(34), c-kit and Sca1, while were almost negative for Gr1, CD(11b), TER119, CD(41), B220 and CD(3). Functional assay demonstrated that the expanded cells had multipotential to differentiate into granulocyte, macrophage, erythrocyte, or B-cells under different cytokines combinations. A prominent megakaryocytic differentiation was observed when cultured with SCF/Tpo/IL-11 combination. The expanded cells were also capable of forming BFU-E, CFU-GM and CFU-Mix in methylcellulose colony assay. The expanded cells over three months could still form CFU-S.
AP20187 combined SCF mediated activation of JAK2 signaling domain can dramatically expand hematopoietic stem/progenitor cells, and the expanded cells can be regulated and committed to differentiate into multilineage cells. This system may provide important insights into stem cell biology and may be promising for gene and cell therapy.
探讨JAK2基因修饰的造血干/祖细胞在体外定向扩增及定向分化潜能的可行性。
克隆基于小鼠干细胞病毒(MSCV)的逆转录病毒载体MGI-F2Jak2,其编码绿色荧光蛋白(GFP)和含两个拷贝修饰的FK506结合蛋白(F36v)与酪氨酸激酶JAK2的融合蛋白。F36v作为二聚体AP20187的高亲和力结合位点。用该载体转染GpE + 86包装细胞。将C57BL/6小鼠的骨髓细胞与经1500 cGy照射的GpE + 86产生克隆共培养48小时进行转导。转导后的骨髓细胞在X-VIVO 15中扩增,并分为以下四组:(1)对照组;(2)单独AP20187组;(3)单独SCF组;(4)AP20187 + SCF组。通过直接用藻红蛋白标记的抗Sca1、c-kit、CD(34)、Gr1、CD(11b)、TER119、CD(41)、B220和CD(3)单克隆抗体进行流式细胞术分析扩增细胞的表型。进一步评估定向分化、祖细胞集落测定和脾集落形成单位(CFU-S)。
仅在AP20187 + SCF组获得了转导骨髓细胞的显著持续生长。培养80天后细胞扩增至10(14)倍。倍增时间约为30小时。扩增细胞的表型对CD(34)、c-kit和Sca1呈均匀强阳性,而对Gr1、CD(11b)、TER119、CD(41)、B2
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