Figure 6
M-CSFR+ precursors can become NK cells but have differential developmental requirements. (A) The CD56−CD117+ cell fraction was isolated from day 18 NK-cell differentiation culture of CD34+ cells and labeled for M-CSFR (CD115) expression. FACS gates for the M-CSFR+ and M-CSFR− subsets are shown. On further culture for 2 weeks with cytokines alone (IL-15, IL-7, SCF, FLT-3L) the M-CSFR+ subset gives rise to CD56+CD94− NK cells (top plot), whereas M-CSFR− subset generates predominantly CD56+CD94+ NK cells (bottom plot). (B) The addition of HDC, stroma, or both to CD56−CD117+M-CSFR+ myeloid precursors induces increasing acquisition of CD94 (top) and KIR (bottom). (C) The CD56−CD117+M-CSFR+ subset generates increasing numbers of CD14+ cells on the addition of M-CSF (□, no M-CSF; ▩, 10 ng/mL; ■, 50 ng/mL). The number of CD14+ cells is shown after 1 week of culture with NK-supporting cytokines (IL-15, IL-7, SCF, FLT-3L) and stroma (left) or cytokines and stroma and HDC (right). (D) M-CSF at high doses abolishes NK-cell development of CD56−CD117+M-CSFR+ precursors. Shown are the number of CD56+ cells when CD56−CD117+M-CSFR+ precursors are cultured in NK-supporting cytokines (IL-15, IL-7, SCF, FLT-3L) and in stroma (left) or cytokines, stroma, and HDC (right) and cultured with/without M-CSF (□ indicates no M-CSF; ▩, 10 ng/mL; ■, 50 ng/mL). The number of NK cells at 2 weeks is shown. (E) The CD56−CD117+M-CSFR+ subset cultured with low concentrations (0, 1, 10, and 20 ng/mL) of M-CSF induces CD56+ NK cells with coexpression of CD14 (percentages of CD14+ in CD56+ fraction indicated). Cells were present in the lymphocyte gate by SSC versus FSC characteristics (not shown).Groups showing significant differences are indicated by asterisks (***P < .001, **P = .001-.01, and *P = .01-.05), 2-way analysis of variance on log-transformed values with Bonferroni posttest.

M-CSFR+ precursors can become NK cells but have differential developmental requirements. (A) The CD56CD117+ cell fraction was isolated from day 18 NK-cell differentiation culture of CD34+ cells and labeled for M-CSFR (CD115) expression. FACS gates for the M-CSFR+ and M-CSFR subsets are shown. On further culture for 2 weeks with cytokines alone (IL-15, IL-7, SCF, FLT-3L) the M-CSFR+ subset gives rise to CD56+CD94 NK cells (top plot), whereas M-CSFR subset generates predominantly CD56+CD94+ NK cells (bottom plot). (B) The addition of HDC, stroma, or both to CD56CD117+M-CSFR+ myeloid precursors induces increasing acquisition of CD94 (top) and KIR (bottom). (C) The CD56CD117+M-CSFR+ subset generates increasing numbers of CD14+ cells on the addition of M-CSF (□, no M-CSF; ▩, 10 ng/mL; ■, 50 ng/mL). The number of CD14+ cells is shown after 1 week of culture with NK-supporting cytokines (IL-15, IL-7, SCF, FLT-3L) and stroma (left) or cytokines and stroma and HDC (right). (D) M-CSF at high doses abolishes NK-cell development of CD56CD117+M-CSFR+ precursors. Shown are the number of CD56+ cells when CD56CD117+M-CSFR+ precursors are cultured in NK-supporting cytokines (IL-15, IL-7, SCF, FLT-3L) and in stroma (left) or cytokines, stroma, and HDC (right) and cultured with/without M-CSF (□ indicates no M-CSF; ▩, 10 ng/mL; ■, 50 ng/mL). The number of NK cells at 2 weeks is shown. (E) The CD56CD117+M-CSFR+ subset cultured with low concentrations (0, 1, 10, and 20 ng/mL) of M-CSF induces CD56+ NK cells with coexpression of CD14 (percentages of CD14+ in CD56+ fraction indicated). Cells were present in the lymphocyte gate by SSC versus FSC characteristics (not shown).Groups showing significant differences are indicated by asterisks (***P < .001, **P = .001-.01, and *P = .01-.05), 2-way analysis of variance on log-transformed values with Bonferroni posttest.

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