Figure 6
Figure 6. CD19− PC are detectable at sites of chronic inflammation and can secrete autoantibodies. (A) Synovial biopsies from 2 patients with rheumatoid arthritis were analyzed by immunofluorescence histology for the presence of CD138+DAPI+CD19+ and CD138+DAPI+CD19− PC (1 out of 2 cases is shown). Upper and lower panels originate from the identical staining and section. (B) Kidney tissue from 2 patients after humoral rejection was digested by collagenase V, and mononuclear cells were analyzed by flow cytometry for the presence of CD19+ and CD19− PC. PC were identified using high expression of CD38 within a wide lymphocyte gate and electronic depletion of CD3+ cells, CD14+ cells, and dead cells. In 1 of the 2 cases, CD19 expression by PC was controlled using an isotype-matched control antibody, and the PC identity was confirmed by the detection of intracellular immunoglobulin (cyt κ and λ Ab light chains). Numbers denote mean fluorescence intensities. (C) CD19+ and CD19− BMPC from 1 SLE patient (serum anti-dsDNA antibodies, 84 U/mL) were isolated and subjected to an Elispot assay detecting dsDNA-specific IgG-secreting cells among 24 000 CD19+ BMPC/well and 27 000 CD19− BMPC/well. Representative wells (from 14 dsDNA-coated replicate wells and 7 bovine serum albumin-coated replicate wells per PC subset to determine assay background) and assay controls are shown. After background subtraction, frequencies of dsDNA-specific PC were 0.8 and 1.3 PC per 10 000 total CD19+ and CD19− BMPC, respectively.

CD19 PC are detectable at sites of chronic inflammation and can secrete autoantibodies. (A) Synovial biopsies from 2 patients with rheumatoid arthritis were analyzed by immunofluorescence histology for the presence of CD138+DAPI+CD19+ and CD138+DAPI+CD19 PC (1 out of 2 cases is shown). Upper and lower panels originate from the identical staining and section. (B) Kidney tissue from 2 patients after humoral rejection was digested by collagenase V, and mononuclear cells were analyzed by flow cytometry for the presence of CD19+ and CD19 PC. PC were identified using high expression of CD38 within a wide lymphocyte gate and electronic depletion of CD3+ cells, CD14+ cells, and dead cells. In 1 of the 2 cases, CD19 expression by PC was controlled using an isotype-matched control antibody, and the PC identity was confirmed by the detection of intracellular immunoglobulin (cyt κ and λ Ab light chains). Numbers denote mean fluorescence intensities. (C) CD19+ and CD19 BMPC from 1 SLE patient (serum anti-dsDNA antibodies, 84 U/mL) were isolated and subjected to an Elispot assay detecting dsDNA-specific IgG-secreting cells among 24 000 CD19+ BMPC/well and 27 000 CD19 BMPC/well. Representative wells (from 14 dsDNA-coated replicate wells and 7 bovine serum albumin-coated replicate wells per PC subset to determine assay background) and assay controls are shown. After background subtraction, frequencies of dsDNA-specific PC were 0.8 and 1.3 PC per 10 000 total CD19+ and CD19 BMPC, respectively.

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