Development of a recombinant anti-Vel immunoglobulin M to identify Vel-negative donors

Fig. S1. Flow cytometry analysis of Vel expression. Comparison of immunopurified anti-Vel antibodies from serum of the immunized patient and reference MB46 serum with Vel-positive and Vel-negative RBCs, detected with anti-IgM (a) or -IgG (b). MB46 eluate Vel-positive RBCs (dashed), MB46 eluate Vel-negative RBCs (dotted), patient eluate Vel-positive RBCs (solid), and patient eluate Vel-negative RBCs (filled).

Fig. S2. Sorting single B-cells bound to Vel-positive ghosts labeled with PKH26 probe. Gating strategy: CD19-positive B-cell were purified by MACS and dot plot shows the FSC/SSC distribution and gating of B-cells (a), forward scatter to include only single cells (b), side scatter to include only single cells (c). d) depicts the gate used to single cell sort B-cells bound to Vel-positive ghosts (RBC labeled with PKH26, PE-channel; x-axis) into a 96 wells plate.

Fig. S3. Vel specific clone with 1st PCR and nested PCR amplified VH and VL bands on agarose gel. Detection of heavy chains-IgM (M) and IgG (G) and light chains Kappa (κ) and Lambda (λ).

Fig.S4. Anti-Vel M3F5S-IgM can mediate deposition of C3b and C4b on RBCs. a) histogram depicting specific antigen detection using anti-Vel M3F5S-IgM (left), anti-D (middle) and anti-A (right) (solid lines) and isotype controls (gray). RBCs were treated with anti-Vel M3F5S-IgM (left), anti-D (middle) and anti-A (right) in presence of serum and with or without 20 mM EDTA (to block the calcium-dependent complement deposition) for 30 minutes. Complement deposition on RBCs was detected using anti-C3b and anti-C4b as indicated. Note the absence of C3b and C4b deposition upon incubation with anti-D IgM (middle, negative control) and upon treatment with EDTA.

Table S1. PCR primers. A First PCR primers B. Nested PCR primers

Table S2. RBC panel for antibody identification in 4 different agglutination assays