Figure 5.
CALRdel/delmice develop an extreme myeloproliferative disease with MF. (A) CALRdel/del mice develop marked thrombocytosis. Bar graphs showing significantly increased platelets, elevated WBC counts, and reduced hematocrit (Hct) in CALRdel/del mice at 3 to 4 months after poly I:C. The CALRdel/del mice were CALRfl/fl Mx1Cre+, the CALRdel/+ mice were CALRfl/+ Mx1Cre+, and the control mice (CALRwt/+) were CALRfl/+ Mx1Cre– or CALR+/+ Mx1Cre+. (B) CALRdel/del mice show splenomegaly. (C) CALRdel/del mice show striking megakaryocytic hyperplasia. Tissues from mice at 7 to 8 months after poly C:I were taken for histologic analysis. (Left panel) H&E staining of BM showing almost complete effacement of normal hematopoiesis by megakaryocytes and displaying nuclear atypia in CALRdel/del mice. (Middle panel) Silver staining for reticulin showing BM fibrosis in CALRdel/del mice. (Right panel) H&E staining of spleen showing destruction of splenic architecture in CALRdel/del mice. (D) CALRdel/del mice show markedly increased frequencies of HSCs. Flow cytometry was performed and HSCs were defined as Lin–Sca1+cKit+CD150+CD48–. (E) CALRdel/del mice show markedly increased frequencies of megakaryocytic progenitors (MkPs) (Lin–Sca1−cKit+CD150+CD41+). (F) CALRdel/del mice show markedly increased frequencies of myeloid progenitors (Prog) in spleen. Flow cytometry was performed, and myeloid progenitors were defined as the Lin–Sca1−cKit+ population. (G) CALRdel/del mice show significantly reduced numbers of erythroblasts. Flow cytometry was performed and erythroblasts were defined as CD71+Ter119+. Data are shown as mean ± SEM. *P < .05; **P < .01; ***P < .001.

CALRdel/delmice develop an extreme myeloproliferative disease with MF. (A) CALRdel/del mice develop marked thrombocytosis. Bar graphs showing significantly increased platelets, elevated WBC counts, and reduced hematocrit (Hct) in CALRdel/del mice at 3 to 4 months after poly I:C. The CALRdel/del mice were CALRfl/fl Mx1Cre+, the CALRdel/+ mice were CALRfl/+ Mx1Cre+, and the control mice (CALRwt/+) were CALRfl/+ Mx1Cre or CALR+/+ Mx1Cre+. (B) CALRdel/del mice show splenomegaly. (C) CALRdel/del mice show striking megakaryocytic hyperplasia. Tissues from mice at 7 to 8 months after poly C:I were taken for histologic analysis. (Left panel) H&E staining of BM showing almost complete effacement of normal hematopoiesis by megakaryocytes and displaying nuclear atypia in CALRdel/del mice. (Middle panel) Silver staining for reticulin showing BM fibrosis in CALRdel/del mice. (Right panel) H&E staining of spleen showing destruction of splenic architecture in CALRdel/del mice. (D) CALRdel/del mice show markedly increased frequencies of HSCs. Flow cytometry was performed and HSCs were defined as LinSca1+cKit+CD150+CD48. (E) CALRdel/del mice show markedly increased frequencies of megakaryocytic progenitors (MkPs) (LinSca1cKit+CD150+CD41+). (F) CALRdel/del mice show markedly increased frequencies of myeloid progenitors (Prog) in spleen. Flow cytometry was performed, and myeloid progenitors were defined as the LinSca1cKit+ population. (G) CALRdel/del mice show significantly reduced numbers of erythroblasts. Flow cytometry was performed and erythroblasts were defined as CD71+Ter119+. Data are shown as mean ± SEM. *P < .05; **P < .01; ***P < .001.

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