Abstract
Abstract 1446
Currently, there is no single assay that will detect platelet function abnormalities in all individuals. We prospectively studied 369 patients with a strong history of bruising and mucosal membrane bleeding for possible platelet dysfunction following documentation of normal Von Willebrand antigen and activity levels. In an effort to evaluate platelet function under more diverse conditions we chose to simultaneously evaluate 1) aggregation using platelet rich plasma and light transmission aggregometry (LTA), 2) adhesion under high shear using the Platelet Function Analyzer (PFA-100, ADP-collagen, and Epinephrine-collagen cartridges) and 3) platelet initiated clot formation using heparinized whole blood and the two standard mapping agonists, arachadonic acid (AA) and ADP (Hemascope Thromboelastograph Analyzer).
Of the 369 platelet evaluations performed, 87 patients (24%) were found to be normal in all three assays with all agonists. On repeated assays with increased attention to medication and food history, an additional 152 patients were felt to have a transient or acquired dysfunction which improved or normalized on further testing. Leaving 130 patients with persistent bleeding and documented abnormalities on one or more of the assays used. There were no patients with only Collagen (CN) or arachadonic acid (AA) aggregation alone on LTA. Using LTA, there was one patient with combined CN and ADP aggregation defect only, another with AA and EPI absent aggregation only, and one with only AA and Thrombin receptor agonist peptide (TRAP) aggregation abnormalities. A summary of the remaining 127 patients are displayed in the table below:
| Abnormal Assay . | LTA EPI . | LTA ADP . | LTA ADP + EPI . | LTA ADP, EPI CN . | LTA ADP, EPI, AA . | LTA ADP, EPI CN, AA . | PFA and PLT Mapping ONLY . |
|---|---|---|---|---|---|---|---|
| Number | 20 | 12 | 40 | 8 | 4 | 18 | 25 |
| M/F | 3M/17F | 6M/6F | 16M/24F | 1M/7F | 1M/3F | 8M/10F | 12M/13F |
| PFA | 1M/2F | 4M | 7M/4F | 0 | 1M | 0 | 1M/3F |
| Plt Mapping | 2M/2F | 1M/2F | 3F | 1F | 0 | 0 | 9M/7F |
| Both PFA and Mapping | 1M | 0 | 0 | 0 | 1F | 2M/9F | 2M/3F |
| Abnormal Assay . | LTA EPI . | LTA ADP . | LTA ADP + EPI . | LTA ADP, EPI CN . | LTA ADP, EPI, AA . | LTA ADP, EPI CN, AA . | PFA and PLT Mapping ONLY . |
|---|---|---|---|---|---|---|---|
| Number | 20 | 12 | 40 | 8 | 4 | 18 | 25 |
| M/F | 3M/17F | 6M/6F | 16M/24F | 1M/7F | 1M/3F | 8M/10F | 12M/13F |
| PFA | 1M/2F | 4M | 7M/4F | 0 | 1M | 0 | 1M/3F |
| Plt Mapping | 2M/2F | 1M/2F | 3F | 1F | 0 | 0 | 9M/7F |
| Both PFA and Mapping | 1M | 0 | 0 | 0 | 1F | 2M/9F | 2M/3F |
Summary: By using a combination of three assays, we were able to identify 25 additional patients with significant platelet dysfunction detected with abnormal platelet mapping or PFA-100 despite normal light transmission aggregometry. Patients with the most abnormalities on aggregation, also demonstrated abnormal adhesion and platelet initiated clot formation. However, the use of PFA-100 and/or platelet mapping alone would miss the majority of patients with aggregation defects. In the future, the unique combination of platelet function defects as measured by these assays, and future technologies, will not only improve detection, but also facilitate phenotype to genotype associations and expedite mutational analysis.
Off Label Use: Rituximab to treat ITP.
Author notes
Asterisk with author names denotes non-ASH members.
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