CD19 can also associate with the BCR in
the absence of CD21 to promote BCR HSP inhibitor cancer signalosome assembly upon recognition of membrane-associated antigens 4. The cytoplasmic tail of CD19 contains two canonical motifs for recruitment of PI3K (YXXM), and these are required for CD19 function 5. Genetic evidence supports a functional role for AKT downstream of CD19, in that combined deletion of two AKT genes (Akt1 and Akt2) in mouse B cells confers a defect in marginal zone (MZ) B-cell development 6 similar to the phenotype of CD19-deficient mice 5, 7. However, it is not yet clear which AKT substrates regulate MZ-cell development. Forkhead box subgroup O (Foxo) transcription factors activate or suppress target genes in a cell type-specific and context-dependent manner 8, 9. In resting lymphocytes, Foxo proteins are localized to the nucleus and activate genes that maintain quiescence as well as proper homing and recirculation 1. Phosphorylation by AKT causes cytoplasmic sequestration and degradation of Foxo factors, inhibiting the Foxo gene expression program. The Foxo1 family member has been studied in lymphocytes by conditional deletion using Cre-lox systems. This work has identified unique roles
for Foxo1 MG-132 in several aspects of B-cell function 10. Deletion of the Foxo1 gene in early B-cell progenitors using Mb1Cre caused a block at the pro-B cell stage. Deletion at a later stage with Cd19Cre caused a partial block at the pre-B-cell stage. Deletion
of Foxo1 in late transitional B cells with Cd21Cre blocked class-switch recombination. We have examined in more detail the phenotype of mature B cells in mice with Cd19Cre-mediated deletion of Foxo1. We find that these mice have fewer FO B cells and a higher percentage of MZ cells. In mice homozygous for the Cd19Cre knock-in allele, which lack CD19 protein, MZ cells are absent as reported previously 5, 7 but this defect is reversed by the concomitant Bcl-w deletion of Foxo1. This genetic epitasis analysis suggests the possibility that CD19 negatively regulates Foxo1 to promote MZ B-cell development. We generated a conditional Foxo1 allele by inserting LoxP sites flanking the first exon of Foxo111. Mice homozygous for the Foxo1-flox allele are denoted Foxo1f/f herein. We bred Foxo1f/f mice with Cd19Cre mice in which the Cre recombinase is knocked into the Cd19 locus 12. Splenic B cells from Foxo1f/fCd19Cre mice expressed no detectable Foxo1 protein as determined by immunoblot, whereas Foxo3a expression was unchanged (Supporting Information Fig. 1A). Several aspects of B-cell development in these mice were altered in a manner similar to the phenotype of another strain of Foxo1f/fCd19Cre mice reported by Dengler et al.10. In particular, our Foxo1f/fCd19Cre mice had fewer IgM+ bone marrow B cells (Supporting Information Fig. 1B), and a population of peripheral B220+ cells lacking surface expression of IgM or IgD (Supporting Information Fig.
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