Figure 6.
Fibrin(ogen) supports tumor cell survival in the lungs by a mechanism coupled to NK cell function. (A-B) Quantitative analysis of metastatic foci within the lungs of mice with single and combined genetic deficits in fibrinogen and NK cells 14 days after intravenous injection of LLCGFP cells. Note that with natural killer cell function intact (A), Fib–/– mice developed significantly fewer metastatic foci than control animals challenged in parallel with 4 × 105 LLCGFP (*P < .01). In contrast, in transgenic mice with a life-long genetic deficit in NK cells (B), fibrinogen deficiency did not significantly alter metastatic potential (8 × 104 cells injected/mouse; P > .5). (C-D) Quantitative analysis of residual radiolabeled LLCGFP cells within the lung tissue 24 hours after intravenous injection of 8 × 104 cells into mice with and without NK cells. Note that in mice with intact natural killer function (NK+), fibrinogen deficiency (n = 15) resulted in a significant diminution in lung-associated tumor cells relative to control animals (n = 18; C). (*P < .008). However, in transgenic mice with a life-long genetic deficit in NK cells (D), no significant diminution in lung-associated tumor cells was observed in Fib–/– mice (n = 12) relative to control animals (n = 19). All P values were generated using a Mann-Whitney U test.