Fig. 3.
Fig. 3. Correlation between total ferritin (ferritin), IRP, and LIP levels in K562 cells after acute iron depletion. K562 cells incubated for 30 minutes without additives (Con) or with 100 μmol/L SIH (ISAH) were allowed to “recover” for 8 hours at 37°C in bicarbonate-free DMEM containing the indicated additives: 0.1% dimethyl sulfoxide (DMSO) final (Con-DMSO, ISAH-DMSO), 20 μg/mL leupeptin (Con-Leup, ISAH-leup), or 10% FCS (ISAH-FCS). ‘Untreated’ cells (left bar) were grown in full medium without additives for 8 hours. After the 8-hour period, aliquots of cells were taken for determination of LIP levels by the calcein method as in Fig 1(lower panel, ▪), ferritin by ELISA (lower panel, □), and IRP by electromobility gel retardation assay (upper panel). LIP levels are given in micromoles per liter, ferritin values are expressed relative to control (which contained ∼130 ng/mg protein), and IRP is given in terms of densitometry tracings (OD) of gel shift bands relative to control. All samples in the gel were obtained from equivalent numbers of cells. Rec-IRP refers to recombinant IRP, which is used here as standard for identification purposes. The second row of the upper panel depicts gel shifts performed after treatment with β-mercaptoethanol (βME) representing total (fully activated) cellular IRP.

Correlation between total ferritin (ferritin), IRP, and LIP levels in K562 cells after acute iron depletion. K562 cells incubated for 30 minutes without additives (Con) or with 100 μmol/L SIH (ISAH) were allowed to “recover” for 8 hours at 37°C in bicarbonate-free DMEM containing the indicated additives: 0.1% dimethyl sulfoxide (DMSO) final (Con-DMSO, ISAH-DMSO), 20 μg/mL leupeptin (Con-Leup, ISAH-leup), or 10% FCS (ISAH-FCS). ‘Untreated’ cells (left bar) were grown in full medium without additives for 8 hours. After the 8-hour period, aliquots of cells were taken for determination of LIP levels by the calcein method as in Fig 1(lower panel, ▪), ferritin by ELISA (lower panel, □), and IRP by electromobility gel retardation assay (upper panel). LIP levels are given in micromoles per liter, ferritin values are expressed relative to control (which contained ∼130 ng/mg protein), and IRP is given in terms of densitometry tracings (OD) of gel shift bands relative to control. All samples in the gel were obtained from equivalent numbers of cells. Rec-IRP refers to recombinant IRP, which is used here as standard for identification purposes. The second row of the upper panel depicts gel shifts performed after treatment with β-mercaptoethanol (βME) representing total (fully activated) cellular IRP.

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