A further parameter, index velocity, is defined as peak thrombin

A further parameter, index velocity, is defined as peak thrombin concentration divided by the difference between lag time

and time to peak. In brief, thrombin generation assays are able to detect and describe conditions associated with enhanced or impaired coagulation. A CAT thrombin generation curve characterized by a short lag time, high peak, short time-to-peak and high ETP is indicative of a hypercoagulable state, whereas a curve indicating prolonged lag times and decreased peak heights/ETP reflects a hypocoagulable or ‘prohaemorrhagic’ state (Table 5) [14]. In patients with haemophilia, the thrombin generation assay has been shown to detect and correlate with levels of FVIII and RG-7388 supplier factor IX [15]. Importantly, in patients with severe haemophilia but no inhibitors, the thrombin generation assay was able to distinguish among clinical phenotypes, with higher ETP values being measured in patients with a mild bleeding phenotype compared with controls whose

bleeding tendency was more typical for patients with FVIII levels below 1% (Fig. 2) [16]. The major role for thrombin generation assays is expected to be in haemophilia patients with inhibitors, specifically to monitor treatment regimens with bypassing agents and to assess the coagulation profile during ITI therapy and/or high-dose FVIII replacement therapy. Bypassing agents do not restore normal pathways of haemostasis in haemophilia but, rather, they boost the generation of thrombin [17]; this is not reflected in traditional clinical coagulation assays such as prothrombin time (PT) and activated partial thromboplastin Doramapimod nmr time [14, 17, 18]. Ongoing laboratory investigations are attempting to identify whether a correlation exists between thrombin generation assay results and the clinical MCE公司 efficacy of bypassing agents. Likewise, efforts are underway to determine whether a correlation exists between assay results and the clinical outcome of ITI therapy and/or the incidence of breakthrough bleeds and bleeding phenotype. A considerable amount of in vitro data supports the concept that anti-FVIII inhibitor activity in patients with

severe haemophilia A is variable and complex. Epitope mapping has revealed that most FVIII inhibitors have multiple rather than single epitope specificities and that inhibitor patterns differ according to FVIII source [19]. An analysis of patient plasma samples detected major inhibitors directed against C2 and another light chain epitope in about one-third (8/23) of haemophiliacs treated with plasma-derived FVIII (pdFVIII), whereas none (0/11) of the patients treated with rFVIII showed a similar pattern. The combination of anti-A2 and anti-C2 inhibitors was detected in 45% of patients treated with rFVIII and in only 17% of those treated with pdFVIII [19]. In addition, substantial in vitro data indicate a protective role for VWF on inhibitor reactivity with FVIII [20-24].

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