Characterization of the expression and gene promoter of CD22 in murine B cells

CD22 is a B cell-restricted surface molecule which may play an important role in interactions between B cells and other cells and in regulating signals through the B cell receptor (BCR) complex. Were we have examined whether the mouse is a suitable in vivo model for studying CD22 functions. Tn primary and secondary lymphoid organs of adult mice CD22 is on all mature B cells, including resting IgM(+)IgD(+) B cells, IgG(+) HSA(lo) memory B cells, syndecan(+) plasma cells and CD5(+) B cells, but it is not on immature IgM(+)IgD(-) B cells. Biochemical, analysis revealed that murine CD22 is associated with the IgM receptor in some, but not all, CD22(+) B leukemic and lymphoma cell lines; as with human CD22, murine CD22 is rapidly phosphorylated on tyrosine after ligation of the BCR. In the CD22(-) murine pro-B cell line, FEMCL, CD22 expression was inducible by treatment with phorbol 32-myristate 13-acetate. A genomic fragment of the cd22(b) allele containing 1.3 kb 5' of exon 1 was sequenced in order to identify potential DNA regulatory elements in the CD22 promoter region. Consensus sequences for transcription factor binding sites including PU.1, BP-1, AP-2, C/EBP and SP-1 were present, but no classical TATA elements or initiator motifs were evident at relevant positions. The 1.3-kb promoter fragment 5' of exon 1 was sufficient for directing basal promoter activity in B and T cells. There was no significant sequence similarity between the murine and human cd22 gene promoters, although both contain repetitive elements and Sp-1 and AP1 binding sites. Thus, murine CD22 shares a number of features with human CD22 and the mouse provides a suitable model system for elucidating the function of CD22 in vivo.