Fig. 1.
Fig. 1. Autoimmune antibodies bound to the RBC membranes. / RBC membranes were prepared as described in “Materials and methods.” Aggregates that formed during the band 3(−/−) mouse membrane preparations were homogenized (see “Materials and methods”). Proteins were separated on 10% SDS-PAGE gels and were immunoblotted with HRP-conjugated, antimouse (A), or antihuman (B) secondary antibody. H and L indicate the positions of the immunoglobulin H and L chains. Mouse RBC membranes are shown in panel A. Loading: C1, C2, controls 1 and 2, respectively; M1, M2, band 3(−/−) mice 1 and 2, respectively; A1, A2, aggregates 1 and 2 from band 3(−/−) mice 1 and 2 preparations, respectively. C1 were C57BL/6 strain; M1, M2, and C2 were B6.129 strain. (B) Human RBC membranes. Loading: C1, C2, controls 1 and 2, respectively. P indicates proband. Molecular weight markers (kDa) are indicated to the left of the blots.

Autoimmune antibodies bound to the RBC membranes.

RBC membranes were prepared as described in “Materials and methods.” Aggregates that formed during the band 3(−/−) mouse membrane preparations were homogenized (see “Materials and methods”). Proteins were separated on 10% SDS-PAGE gels and were immunoblotted with HRP-conjugated, antimouse (A), or antihuman (B) secondary antibody. H and L indicate the positions of the immunoglobulin H and L chains. Mouse RBC membranes are shown in panel A. Loading: C1, C2, controls 1 and 2, respectively; M1, M2, band 3(−/−) mice 1 and 2, respectively; A1, A2, aggregates 1 and 2 from band 3(−/−) mice 1 and 2 preparations, respectively. C1 were C57BL/6 strain; M1, M2, and C2 were B6.129 strain. (B) Human RBC membranes. Loading: C1, C2, controls 1 and 2, respectively. P indicates proband. Molecular weight markers (kDa) are indicated to the left of the blots.

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