Figure 7
Figure 7. Modulation of Mcl-1 by BLyS, rapamycin and Pim; reduction of peripheral B-cell populations in Pim 1 and 2 doubly deficient mice receiving rapamycin in vivo; and a minimal molecular model of BLyS-dependent growth and survival. (A) Modulation of Mcl-1 protein by BLyS, rapamycin, and Pim. Extracts of small resting wild-type or Pim 1−/−2−/− B cells either freshly isolated (*) or cultured for 2 days in CM with or without rhuBLyS (50 ng/mL) and with vehicle or rapamycin (50 nM) were electrophoretically separated and transferred to nitrocellulose membranes. Membranes were probed with anti–Mcl-1 antibody, stripped, and reprobed with anti-actin antibody. (B) Peripheral B-cell survival in rapamycin-treated mice; 5- to 8-week-old Pim 1−/−2−/− doubly deficient or normal littermates were injected intraperitoneally with 2.5 mg/kg of rapamycin or diluent every other day for 6 days and killed on day 7. The number of viable spleen cells from individual mice was determined by counting and trypan blue exclusion. Peripheral B-cell subpopulations were identified by flow cytometry of viable lymphocytes stained for B220, CD 21/35 and CD23. Total B lymphocytes (B220+; □ represents rapamycin-treated donors; ■, diluent-treated donors) were subdivided into marginal zone (MZ: B220+, CD21/35hi, and CD23lo; ◇ represents rapamycin-treated donors; ♦, diluent-treated donors) or follicular (Fo: B220+, CD21/35int, CD23hi; △ represents rapamycin-treated donors; ▲, diluent-treated donors) B-cell subpopulations, and their number in each donor spleen was determined by reference to the splenocyte counts. Data pooled from 2 independent experiments are shown. (C) BLyS-mediated signaling pathways regulating B-cell growth and survival. Stimulation of B cells by BLyS leads to the activation of PI3-kinase, which phosphorylates Akt on T30842 (current study) and by a separate pathway, the processing and nuclear localization of NF-κB2 with the subsequent induction of pim 2 mRNA and production of constitutively active Pim 2 protein.15,17,34 (current study). Akt is fully activated by phosphorylation on S473 mediated by the rictor containing TOR complex mTORC230 (current study). Akt and the raptor containing TOR complex mTORC1 converge to promote rapamycin-sensitive cell growth31,32 (current study) by inducing glucose uptake and use and up-regulating amino acid and iron transporters, which maintain cell size and promote atrophy resistance28,31,47 (current study). Pim 2 also increases glycolysis and promotes maintenance of cell size by a rapamycin-independent, glucose-dependent mechanism34,35 (current study). BLyS-induced survival requires the antiapoptotic Bcl-2 family member Mcl-122 (current study). Akt induces the activation of CREB and NF-κB1,44 which promote mcl-1 transcription.73,74 Akt also inactivates FOXO3a,48,56 (current study), suppressing the transcription of the proapoptotic protein Bim, a major regulator of B-cell homeostasis.55,57 Mcl-1 protein levels are controlled at the level of translation by mTORC1 and Pim 2, which inactivate the translational repressor 4E-BP1 by rapamycin-dependent and -independent processes; Mcl-1 protein is stabilized by Erk,76 reported to be induced by BLyS stimulation,20 whereas Mcl-1 turnover is enhanced by the action of Gsk-3b,75 which is inhibited by active Akt48 (current study). Mcl-1 protein is reduced by rapamycin treatment54 (current study). Reference citations in this legend for activities induced by BLyS stimulation are in bold. AA indicates amino acid.

Modulation of Mcl-1 by BLyS, rapamycin and Pim; reduction of peripheral B-cell populations in Pim 1 and 2 doubly deficient mice receiving rapamycin in vivo; and a minimal molecular model of BLyS-dependent growth and survival. (A) Modulation of Mcl-1 protein by BLyS, rapamycin, and Pim. Extracts of small resting wild-type or Pim 1−/−2−/− B cells either freshly isolated (*) or cultured for 2 days in CM with or without rhuBLyS (50 ng/mL) and with vehicle or rapamycin (50 nM) were electrophoretically separated and transferred to nitrocellulose membranes. Membranes were probed with anti–Mcl-1 antibody, stripped, and reprobed with anti-actin antibody. (B) Peripheral B-cell survival in rapamycin-treated mice; 5- to 8-week-old Pim 1−/−2−/− doubly deficient or normal littermates were injected intraperitoneally with 2.5 mg/kg of rapamycin or diluent every other day for 6 days and killed on day 7. The number of viable spleen cells from individual mice was determined by counting and trypan blue exclusion. Peripheral B-cell subpopulations were identified by flow cytometry of viable lymphocytes stained for B220, CD 21/35 and CD23. Total B lymphocytes (B220+; □ represents rapamycin-treated donors; ■, diluent-treated donors) were subdivided into marginal zone (MZ: B220+, CD21/35hi, and CD23lo; ◇ represents rapamycin-treated donors; ♦, diluent-treated donors) or follicular (Fo: B220+, CD21/35int, CD23hi; △ represents rapamycin-treated donors; ▲, diluent-treated donors) B-cell subpopulations, and their number in each donor spleen was determined by reference to the splenocyte counts. Data pooled from 2 independent experiments are shown. (C) BLyS-mediated signaling pathways regulating B-cell growth and survival. Stimulation of B cells by BLyS leads to the activation of PI3-kinase, which phosphorylates Akt on T30842  (current study) and by a separate pathway, the processing and nuclear localization of NF-κB2 with the subsequent induction of pim 2 mRNA and production of constitutively active Pim 2 protein.15,17 ,34  (current study). Akt is fully activated by phosphorylation on S473 mediated by the rictor containing TOR complex mTORC230  (current study). Akt and the raptor containing TOR complex mTORC1 converge to promote rapamycin-sensitive cell growth31,32  (current study) by inducing glucose uptake and use and up-regulating amino acid and iron transporters, which maintain cell size and promote atrophy resistance28,31,47  (current study). Pim 2 also increases glycolysis and promotes maintenance of cell size by a rapamycin-independent, glucose-dependent mechanism34,35  (current study). BLyS-induced survival requires the antiapoptotic Bcl-2 family member Mcl-122  (current study). Akt induces the activation of CREB and NF-κB1,44  which promote mcl-1 transcription.73,74  Akt also inactivates FOXO3a,48,56  (current study), suppressing the transcription of the proapoptotic protein Bim, a major regulator of B-cell homeostasis.55,57  Mcl-1 protein levels are controlled at the level of translation by mTORC1 and Pim 2, which inactivate the translational repressor 4E-BP1 by rapamycin-dependent and -independent processes; Mcl-1 protein is stabilized by Erk,76  reported to be induced by BLyS stimulation,20  whereas Mcl-1 turnover is enhanced by the action of Gsk-3b,75  which is inhibited by active Akt48  (current study). Mcl-1 protein is reduced by rapamycin treatment54  (current study). Reference citations in this legend for activities induced by BLyS stimulation are in bold. AA indicates amino acid.

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