Splenic proliferative lymphoid nodules distinct from germinal centers are sites of autoantigen stimulation in immune thrombocytopenia by Capucine Daridon,

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Splenic proliferative lymphoid nodules distinct from germinal centers are sites of autoantigen stimulation in immune thrombocytopenia by Capucine Daridon, Christoph Loddenkemper, Simone Spieckermann, Anja A. Kühl, Abdulgabar Salama, Gerd R. Burmester, Peter E. Lipsky, and Thomas Dörner Blood Volume 120(25):5021-5031 December 13, 2012 ©2012 by American Society of Hematology

Microscopic quantification of GCs and other lymphoid nodules in human spleens. Microscopic quantification of GCs and other lymphoid nodules in human spleens. (A) Representative photomicrograph of an H&E-stained section of an ITP spleen with GCs within a lymphoid nodule identified as an aggregate of nonhomogeneously basophilic cells with distinct DZ and LZ (black circle). An enlargement of a characteristic GC is shown on the right. Black arrows indicate lymphoid nodules and the black square indicates a typical PLN within the white pulp. An enlargement of a characteristic PLN is shown underneath. (B) The number of GCs and lymphoid nodules was counted within spleen sections from 26 patients with ITP and 35 controls. ITP patients were grouped according to the underlying treatment before splenectomy as those treated with prednisone (+Pred) or with IvIg in combination with others medications (+IvIg). Each spleen section was normalized to 3.7 cm2 as described in “Quantification of GCs in spleen sections” and visualized with an Olympus BX70 microscope (×50 magnification). Capucine Daridon et al. Blood 2012;120:5021-5031 ©2012 by American Society of Hematology

Characterization of PLNs in human spleen. Characterization of PLNs in human spleen. (A) Representative photograph of Ki67 staining of spleens from 7 controls and 7 ITP patients showing GCs with LZ/DZ polarization and PLNs with a homogeneous distribution of proliferating cells. Representative photograph of IgM staining of spleens from 8 controls and 8 ITP patients showing GCs mostly lacking the expression of IgM and PLNs exhibiting the dense presence of IgM. Sections of 9 ITP and 10 control spleens were stained for expression of Bcl6, which was mostly limited to the DZ of the GCs and absent in PLNs. Visualization with a Zeiss Axio Imager Z1 fluorescence microscope (×200 magnification). The photomicrographs shown here are from ITP spleens. (B) GCs and PLNs were identified by either Ki67 or IgM stains and the total number of these structures/3.7 cm2 of spleen sections was determined by counting 9 spleen sections from ITP and 11 sections from control. Samples of ITP spleens were divided into those who had received prednisone (Pred) and those who received IvIg just before splenectomy and the number of PLN determined. (C) Comparison of the expression of bcl6, AIDCA, and bcl2 mRNA in spleen from ITP sections versus normal spleen. Distilled water (H2O) was used as a negative control of PCR. Representative RT-PCR of 8 sections from ITP spleen is shown. Each of these sections lacked identifiable GCs. (D) Serial sections of 10 ITP and 10 controls spleens were stained to evaluate the expression of Ki67, CD21, and CD23 in both PLNs (top panels) and GCs (bottom panels). The black arrows mark the dark zone (Ki67+, CD21+/−, and CD23−) and the white arrows indicate the light zone (Ki67+/−, CD21+, CD23+) of a GC. Visualization with Zeiss Axio Imager Z1 fluorescence microscope (×200 magnification). The photomicrographs shown here are from ITP spleens. (E) Comparison of the frequency of proliferating cells in splenic GC and PLN after staining with Ki67. Data are expressed as percentage of Ki67+ cells. Capucine Daridon et al. Blood 2012;120:5021-5031 ©2012 by American Society of Hematology

Quantitative analysis of CD3+ T cells, PD-1+ TFH, and Foxp3+ cells within PLNs and GCs of ITP and control spleens. Quantitative analysis of CD3+ T cells, PD-1+ TFH, and Foxp3+ cells within PLNs and GCs of ITP and control spleens. The density of CD3+ T cells, PD-1+ TFH, and Foxp3+ cells in the PLNs and GCs were determined by counting the total number of (A) CD3+ T cells, (B) PD-1+ cells, and (C) Foxp3+ cells and normalizing to the respective area of PLNs or GCs (per 103 μm2 as described in “Quantification of cells in splenic lymphoid nodules”). At least 3 ITP and 3 control spleens were analyzed. Visualization with Zeiss Axio Imager Z1 fluorescence microscope (×200 magnification). Capucine Daridon et al. Blood 2012;120:5021-5031 ©2012 by American Society of Hematology

Detailed characterization of PLNs within spleens from ITP patients. Detailed characterization of PLNs within spleens from ITP patients. Sections from 4 spleens (3 ITP and 1 control) were examined by double immunofluorescence staining: CD20 (red) with IgD (green), CD1c (green), CD27 (green), or IgM (green). (A) PLN (ITP) and (B) GC (control). The white outline indicates the location of the structures, PLNs and GCs, determined by IgM staining. The presence of T cells in PLNs was analyzed by CD3 (green) and CD20 staining. The arrows designated a T-cell area (B). Control for nonspecific binding was performed on spleen sections using FITC-secondary antibodies and CD20 (red). The sections were analyzed by confocal microscopy using a Zeiss LSM 710 confocal or a Zeiss Axio Imager Z1 fluorescence microscope (×200 magnification; Carl Zeiss). Capucine Daridon et al. Blood 2012;120:5021-5031 ©2012 by American Society of Hematology

Detection of IgM-ICs bound to the FDC network in PLNs identified in ITP spleens. Detection of IgM-ICs bound to the FDC network in PLNs identified in ITP spleens. Sections from 2 ITP spleens were analyzed by immunofluorescence to examine the distribution of (A) DAPI to stain nuclei, CD20 (red), and CD35 (green), and (B) DAPI, IgM (red) and CD35 (green). After staining, the sections were analyzed by confocal microscopy using a Zeiss LSM 710 confocal (×200 magnification; Carl Zeiss). The white ellipse designed using Zen 2010 software represents a proliferating lymphoid nodule identified with IgM staining. (C) Detection of GPIV in ITP spleens: PLN (white arrow) and GC (black arrows); ×200 magnification. (D) The proportion of PLNs identified as containing GPIIb/IIIa was analyzed in 4 ITP spleens versus a control spleen and representative GC and PLN. At least 3 sections of 3 different spleens were analyzed from each specimen; n corresponds to the number of PLN analyzed. (E) DAPI to stain nuclei, CD20 (red), and GPIIb/IIIa (green) on the left or GPIV (green) on the right of the figure. The arrow designated 1 PLN positive from ITP spleen. Capucine Daridon et al. Blood 2012;120:5021-5031 ©2012 by American Society of Hematology

Detection of proliferating B cells and autoantigen within PLNs of ITP spleens. Detection of proliferating B cells and autoantigen within PLNs of ITP spleens. Sections from (A) 2 ITP spleens and (B) 1 control were stained for CD20 (red), Ki67 (green), or GPIIb/IIIa (green) and assessed for the presence of proliferating B cells and B cells in proximity to GPIIb/IIIa. Visualization was carried out with a Zeiss Axio Imager Z1 fluorescence microscope (×200 magnification). Capucine Daridon et al. Blood 2012;120:5021-5031 ©2012 by American Society of Hematology