![Figure 5. PF4-coated E coli LPS mutants are recognized by anti-PF4/heparin IgG from sera of patients with HIT. (A) PF4-coated E coli LPS mutants ΔwaaC (KPM53) or ΔwaaA (KPM121) were incubated with sera of 3 patients with HIT known to contain anti-PF4/heparin antibodies, and bound IgG was affinity purified. Symbols represent reactivities of IgG antibodies eluted from PF4-coated E coli KPM53 (squares) or KPM121 (triangles); means are presented as horizontal lines. Binding of the purified antibodies to PF4/heparin complexes (first column) was inhibited by excess heparin (100 IU/mL unfractionated heparin [UFH], column 2), which disrupts PF4/heparin complexes. Antibodies did not react with PF4 alone (column 3). PF4-untreated bacteria served as control for unspecific binding of the antibodies to bacteria alone (column 4). (B) E coli K12 wild-type strain BW30270 and its isogenic ΔwaaA mutant KPM121 were labeled with FITC and preincubated with PF4 and additionally with heat-inactivated human serum containing anti-PF4/heparin IgG (preadsorbed with bacteria alone). After preincubation, the bacteria were subjected to phagocytosis. The figure shows the MFI multiplied by the percentage of FITC-positive polymorphonuclear leukocytes (PMNs) as a measure for bacterial phagocytosis. Data are mean ± SD of 4 different sera.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/120/16/10.1182_blood-2012-06-434985/4/zh89991298070005.jpeg?Expires=1724262387&Signature=jpvT5EPKntcJQALmVxttjT-fDZORav7iKpUbpbIbY83ivoj3G~uNryo6hp6FU833RuyjhDzqvLpwD4QUEHL786z7g5FJmOXklNaiYEQDUdhlvzpAOYGWThOu~T22NH~t44eaPUfgkNC0fcC59jpwVHRyWIy7RBeh7kLHNBNUbd7lEh6~vpRQPrDYj0YPL6AGl9pBNrRzY5jT-uxVwWfN2W8g4BrjX-uxQa4bXTVEnVX6QLvGuv9lyfAer84boo2UnNhI6BmzVMxrBfgmjQ2w7wDaISDS9FohARt0ADgu9aOB14p7T0tY45PsrVhGyERaUVuTKHnhYaanP0-YPHmLsQ__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
PF4-coated E coli LPS mutants are recognized by anti-PF4/heparin IgG from sera of patients with HIT. (A) PF4-coated E coli LPS mutants ΔwaaC (KPM53) or ΔwaaA (KPM121) were incubated with sera of 3 patients with HIT known to contain anti-PF4/heparin antibodies, and bound IgG was affinity purified. Symbols represent reactivities of IgG antibodies eluted from PF4-coated E coli KPM53 (squares) or KPM121 (triangles); means are presented as horizontal lines. Binding of the purified antibodies to PF4/heparin complexes (first column) was inhibited by excess heparin (100 IU/mL unfractionated heparin [UFH], column 2), which disrupts PF4/heparin complexes. Antibodies did not react with PF4 alone (column 3). PF4-untreated bacteria served as control for unspecific binding of the antibodies to bacteria alone (column 4). (B) E coli K12 wild-type strain BW30270 and its isogenic ΔwaaA mutant KPM121 were labeled with FITC and preincubated with PF4 and additionally with heat-inactivated human serum containing anti-PF4/heparin IgG (preadsorbed with bacteria alone). After preincubation, the bacteria were subjected to phagocytosis. The figure shows the MFI multiplied by the percentage of FITC-positive polymorphonuclear leukocytes (PMNs) as a measure for bacterial phagocytosis. Data are mean ± SD of 4 different sera.
