Sanofi, Waltham, Massachusetts.
J Thromb Haemost. 2019 Jul;17(7):1044-1052. doi: 10.1111/jth.14430. Epub 2019 Apr 26.
Essentials Non-factor VIII (FVIII) therapies for hemophilia A, such as bispecific antibodies (bsAbs), are in development. Bispecific antibodies are intrinsically different from FVIII and lack many of the same regulatory mechanisms. These differences complicate assignment and interpretation of FVIII-equivalent activity. Inability to assign FVIII equivalence compromises our capacity to assess hemostatic potential of bsAb therapies.
Activated factor VIII (FVIIIa) mimetic bsAbs aim to enable prophylactic treatment of hemophilia A patients with and without inhibitors. With different mechanisms of action, benchmarking their activity against FVIII to determine efficacious yet safe dosage is difficult.
To compare the activities of sequence identical emicizumab (SI-Emi) and another bsAb, BS-027125, to recombinant FVIII (rFVIII) using clinical and nonclinical assays and to evaluate our ability to assign a FVIII-equivalent value to bsAbs and implications thereof.
Activities of SI-Emi, BS-027125, and rFVIII were measured by one-stage clotting assay, chromogenic factor Xa generation assay, and thrombin generation assay. We also assessed the activity of anti-FIXa and anti-FX bivalent homodimers of each bsAb and probed the effect of different reagents in thrombin generation assay (TGA).
The FVIII-like activity of SI-Emi and BS-027125 ranged greatly across each assay, varying both by parameter measured within an assay and by reagents used. Notably, SI-Emi anti-FIXa bivalent homodimer had meaningful activity in several assays, whereas BS-027125 anti-FIXa bivalent homodimer only had activity in the chromogenic assay. Surprisingly, SI-Emi displayed activity in the absence of phospholipids, while BS-027125 had minimal phospholipid-independent activity.
Bispecific antibodies demonstrate little consistency between assays tested here owing to intrinsic differences between FVIII and bsAbs. While some trends are shared, the bsAbs also differ in mechanism. These inconsistencies complicate assignment of FVIII-equivalent values to bsAbs. Ultimately, a deeper mechanistic understanding of bsAbs as well as bsAb-tailored assays are needed to monitor and predict their hemostatic potential and long-term efficacy and safety confidently.
使用临床和非临床检测方法比较序列相同的emicizumab(SI-Emi)和另一种 bsAb、BS-027125 与重组 FVIII(rFVIII)的活性,并评估我们为 bsAb 赋值 FVIII 等效值的能力及其影响。
通过一期凝血检测、显色因子 Xa 生成检测和凝血酶生成检测来测量 SI-Emi、BS-027125 和 rFVIII 的活性。我们还评估了每种 bsAb 的抗 FIXa 和抗 FX bivalent 同型二聚体的活性,并研究了不同试剂在凝血酶生成检测(TGA)中的作用。
SI-Emi 和 BS-027125 的 FVIII 样活性在每个检测中差异很大,在检测内的参数和使用的试剂上均有不同。值得注意的是,SI-Emi 的抗 FIXa bivalent 同型二聚体在几个检测中具有有意义的活性,而 BS-027125 的抗 FIXa bivalent 同型二聚体仅在显色检测中具有活性。令人惊讶的是,SI-Emi 在没有磷脂的情况下显示出活性,而 BS-027125 的磷脂非依赖性活性很小。
由于 FVIII 和 bsAb 之间存在内在差异,这里测试的 bsAb 之间在检测上显示出很少的一致性。虽然有些趋势是共享的,但 bsAb 在机制上也存在差异。这些不一致性使得为 bsAb 赋值 FVIII 等效值变得复杂。最终,需要更深入地了解 bsAb 的机制以及专门用于监测和预测其止血潜力以及长期疗效和安全性的 bsAb 检测方法。
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