Fig. 2.
Fig. 2. Effect of myeloma cells on RANKL secretion by activated T lymphocytes. / Aliquots of conditioned media were assessed for sRANKL by ELISA. Activated CD3+ T lymphocytes (A) or CD4+/CD8+ subsets (B) were cocultured with HMCL RPMI-8266 or U266 placed in a transwell insert. Autologous CD3+ T cells were cocultured with fresh MM cells (panel C). (C indicates activated CD3+ T cells.) Graphs represent the mean levels ± SE of 3 repeated experiments. *P < .05. Secretion of RANKL into conditioned medium was checked by immunoprecipitation with RANK-Fc followed by gel electrophoresis. RANKL protein was detected either by gel staining with silver stain plus in conditioned medium of activated T cells cocultured with HMCL (D) or by immunoblot analysis using anti-RANKL mAb (E). Data are representative of 3 independent experiments. C indicates activated CD3+ lymphocytes).

Effect of myeloma cells on RANKL secretion by activated T lymphocytes.

Aliquots of conditioned media were assessed for sRANKL by ELISA. Activated CD3+ T lymphocytes (A) or CD4+/CD8+ subsets (B) were cocultured with HMCL RPMI-8266 or U266 placed in a transwell insert. Autologous CD3+ T cells were cocultured with fresh MM cells (panel C). (C indicates activated CD3+ T cells.) Graphs represent the mean levels ± SE of 3 repeated experiments. *P < .05. Secretion of RANKL into conditioned medium was checked by immunoprecipitation with RANK-Fc followed by gel electrophoresis. RANKL protein was detected either by gel staining with silver stain plus in conditioned medium of activated T cells cocultured with HMCL (D) or by immunoblot analysis using anti-RANKL mAb (E). Data are representative of 3 independent experiments. C indicates activated CD3+ lymphocytes).

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