We have established a cell culture system without stromal cells that allows the CD34+ hematopoietic progenitor cells (HPC) to differentiate into natural killer (NK) cells. CD34+Lin (CD3, CD16, CD56)-cells were purified using fluorescence-activated cell sorting from normal adult bone marrow (BM) and cultured for 28 days in medium supplemented with interleukin-2 (IL-2) and stem cell factor (SCF). NK (CD3-CD16-CD56+) cells were generated in a dose-dependent manner in response to SCF. NK cells originated from CD34+CD33+Lin- cells, but they were barely detectable in cultures of CD34+CD33-Lin- cells. However, on addition of IL-3, an induced differentiation of NK cells from CD34+CD33-Lin- cells was observed, although at a lower frequency. Supplementing of the cell cultures with SCF alone or both SCF and IL-3 for the first 7 days followed by IL-2 for the next 21 days is essential for production of NK cells from CD34+CD33+Lin- cells and from CD34+CD33-Lin- cells, respectively. These data provide direct evidence that NK cells arise from CD34+HPC and show the minimum lymphokine requirement for their differentiation.
ARTICLES|
June 15, 1995
Lymphokine requirement for the generation of natural killer cells from CD34+ hematopoietic progenitor cells
A Shibuya,
A Shibuya
Division of Hematology, University of Tsukuba, Japan.
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K Nagayoshi,
K Nagayoshi
Division of Hematology, University of Tsukuba, Japan.
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K Nakamura,
K Nakamura
Division of Hematology, University of Tsukuba, Japan.
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H Nakauchi
H Nakauchi
Division of Hematology, University of Tsukuba, Japan.
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Blood (1995) 85 (12): 3538–3546.
Citation
A Shibuya, K Nagayoshi, K Nakamura, H Nakauchi; Lymphokine requirement for the generation of natural killer cells from CD34+ hematopoietic progenitor cells. Blood 1995; 85 (12): 3538–3546. doi: https://doi.org/10.1182/blood.V85.12.3538.bloodjournal85123538
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