![Figure 1. Loss of sialic acids on the erythrocyte membrane activates Lu/BCAM. (A) Representative micrograph of adhesion of healthy erythrocytes (top panel; original magnification ×10) and sickle erythrocytes (lower panel) to a laminin-α5–coated ibidi chamber at 0.2 dyn/cm. (B) Quantification of adhesion frequency of old and young erythrocytes to laminin-α5 at 0.2 dyn/cm2 (n = 3). Percoll dilutions were stacked in a 15-mL tube; erythrocytes isolated from the fraction denser than 1.096 g/mL Percoll were defined as dense and old erythrocytes (roughly 3% of total red blood cell [RBC]), whereas erythrocytes lighter than 1.060 g/mL Percoll are here defined as light and young erythrocytes (roughly 0.75% of total RBC). (C) Biotinylated Maackia amurensis lectin type II (MA) was used to quantify α2,3-linked sialic acid (SIA) by flow cytometry (Data shown as mean fluorescence intensity [MFI] and normalized [Norm.] to control erythrocytes [aaRBC].). (D) Membrane sialic acid was removed from control erythrocytes by V cholerae neuraminidase (N'ase RBC), and adhesion frequency was assessed at 0.2 dyn/cm2 (n = 5). Specificity was addressed using an Lu/BCAM blocking polyclonal antibody. (E) Sickle erythrocyte (ssRBC) adhesion frequency to laminin-α5 at 0.2 dyn/cm2, either treated or not treated with neuraminidase for 30 minutes at 37°C (n = 5). *P < .05; ***P < .001.](https://ash.silverchair-cdn.com/ash/content_public/journal/bloodadvances/2/1/10.1182_bloodadvances.2017013094/3/advances013094f1.jpeg?Expires=1724965121&Signature=w-ICIpMLOfssPLuwpKnaoz9IsrAX34l3~qqLDcvj1gv6GPs5HBw4zge2Rjq3lKK2oOgb0evgVAsaZ96nlrdG-~NSwfKJPHVodsJ7rDFaE4NfO6mTlOL0cj1ZhdjjgRQ~1vAhFqzz6Bd-vwjNNWSBdBu9XnPgqq1wwesN1Go8c-EjiWrKABY4p0YB5T8n6xeNVczQJTZfYFLzNOBdwQVMBDGFNTa8BFT5-HIMGAdVByk~q6VMyn3hOxqlsbk5vXWgNnBxXNM93tINBeZL3xE6kqVJQdIo~kvcl69BQNNKIDiGm625SSJwTejeBOKI4CJr6AwHv0AJfOi7j05sgl0NJg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Loss of sialic acids on the erythrocyte membrane activates Lu/BCAM. (A) Representative micrograph of adhesion of healthy erythrocytes (top panel; original magnification ×10) and sickle erythrocytes (lower panel) to a laminin-α5–coated ibidi chamber at 0.2 dyn/cm. (B) Quantification of adhesion frequency of old and young erythrocytes to laminin-α5 at 0.2 dyn/cm2 (n = 3). Percoll dilutions were stacked in a 15-mL tube; erythrocytes isolated from the fraction denser than 1.096 g/mL Percoll were defined as dense and old erythrocytes (roughly 3% of total red blood cell [RBC]), whereas erythrocytes lighter than 1.060 g/mL Percoll are here defined as light and young erythrocytes (roughly 0.75% of total RBC). (C) Biotinylated Maackia amurensis lectin type II (MA) was used to quantify α2,3-linked sialic acid (SIA) by flow cytometry (Data shown as mean fluorescence intensity [MFI] and normalized [Norm.] to control erythrocytes [aaRBC].). (D) Membrane sialic acid was removed from control erythrocytes by V cholerae neuraminidase (N'ase RBC), and adhesion frequency was assessed at 0.2 dyn/cm2 (n = 5). Specificity was addressed using an Lu/BCAM blocking polyclonal antibody. (E) Sickle erythrocyte (ssRBC) adhesion frequency to laminin-α5 at 0.2 dyn/cm2, either treated or not treated with neuraminidase for 30 minutes at 37°C (n = 5). *P < .05; ***P < .001.
