Definition of a multiple myeloma progenitor population in mice driven by enforced expression of XBP1s
Joshua Kellner, Caroline Wallace, Bei Liu, Zihai Li
Joshua Kellner, Caroline Wallace, Bei Liu, Zihai Li
View: Text | PDF
Research Article Hematology Immunology

Definition of a multiple myeloma progenitor population in mice driven by enforced expression of XBP1s

Abstract

Multiple myeloma (MM) is an incurable plasma cell malignancy with frequent treatment failures and relapses, suggesting the existence of pathogenic myeloma stem/progenitor populations. However, the identity of MM stem cells remains elusive. We used a murine model of MM with transgenic overexpression of the unfolded protein response sensor X-box binding protein 1 (XBP1s) in the B cell compartment to define MM stem cells. We herein report that a post–germinal center, pre–plasma cell population significantly expands as MM develops. This population has the following characteristics: (a) cell surface phenotype of B220+CD19+IgM–IgD–CD138–CD80+sIgG–AA4.1+FSChi; (b) high expression levels of Pax5 and Bcl6 with intermediate levels of Blimp1 and XBP1s; (c) increased expression of aldehyde dehydrogenase, Notch1, and c-Kit; and (d) ability to efficiently reconstitute antibody-producing capacity in B cell–deficient mice in vivo. We thus have defined a plasma cell progenitor population that resembles myeloma stem cells in mice. These results provide potentially novel insights into MM stem cell biology and may contribute to the development of novel stem cell–targeted therapies for the eradication of MM.

Authors

Joshua Kellner, Caroline Wallace, Bei Liu, Zihai Li

×

Figure 5

The PCPC population differentiates into PCs.

Options: View larger image (or click on image) Download as PowerPoint
The PCPC population differentiates into PCs. (A–C) Naive B cells (B220+C...
(AC) Naive B cells (B220+CD19+IgM+CD138AA4.1), PCPCs, and PCs (B220CD138+) were sorted from XBP1-Tg mice and adoptively transferred into μMT mice (n = 4 mice/group). (A) FACS staining profile of nucleated cells before sorting. (B) Characterization of naive, PCPC, and PC populations after sorting but before the adoptive transfer. The percentages of each population in the final sorted cellular products are indicated. (C) Total IgG1 and IgM concentrations in the sera of recipient mice were measured by ELISA 4 months after the adoptive transfer. *P < 0.05 and error bars denote ± SEM. (D) PCs (B220CD138+), BCPCs, PCPCs, and memory-like B cells (PCPC sIgG+) were sorted to over 90% purity and placed into PC-culturing conditions for 7 days. The total numbers of PCs generated from 300,000 total cells are shown (n = 4). In C and D, 1-way ANOVA with Tukey’s multiple-comparisons test was used to calculate *P < 0.05. All error bars denote ± SEM.