(A and B) Humanized chimeras were constructed by infusing NSG mice intraperitoneally with PBMCs (1 × 10⁷cells/per mouse) isolated from patients with SLE or healthy donors. A total of 4 chimeras were included in each experimental group. (A) The proliferation of MCs was demonstrated by dual-color immunostaining of DESIN (green) and KI67 (red). The nuclei were marked with DAPI, which produced a blue fluorescence. (B) Transmission electron microscopy was employed to observe the glomerular ultrastructure of humanized chimeras. (C) MCs were conditioned with SLE plasma that had been pretreated with pepsin (pepsin/IgG = 1:60) or papain (papain/IgG = 1:60) and DnaseI (50 μL working buffer for 5 μg DNA) in order to eliminate IgG and DNA component (papain cleaves the hinge region of IgG into Fab/Fc fragments, while pepsin degrades Fc regions). The proliferation of MCs was detected by the CCK-8 assay. MCs were stimulated with DNA-IC (80 IU/mL) isolated from plasma of patients with SLE or IgG from healthy donors for 1 day. MCs were stimulated with DNA-IC isolated from plasma of patients with SLE (IC group) or healthy donors (HC group). (D) Effect of DNA-IC on proliferative activity of MCs detected by CCK-8 assay (n = 10). (E and F) EdU assay revealed that the percentage of EdU⁺ cells was significantly higher in LN MCs. (G) Cell cycle detection was analyzed in LN MCs and HC MCs by the cell cycle assay kit (n = 7 for each group). (H) Gene set enrichment analysis of single-cell data from SYD997, enriched in genes involved in cell_cycle_G1_S_phase_transition progression. NES, normalized enrichment score. Lines with whiskers show the mean ± SEM. Scale bar: 100 μm (A), 50 μm (E), 2 μm (B). *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001 with ANOVA plus Turkey’s method (C) and paired t test (D, F, and G).