Calibrating Thrombin Generation in Different Samples: Less Effort with a Less Efficient Substrate

Tapp, Hans Jürgen; Grundmann, Claudia; Kusch, Manuela; König, Herbert

doi:10.2174/1876506800902010006

Cited by 4 publications

(5 citation statements)

References 26 publications

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“…Plasma concentration: The plasma concentration in commercial fluorogenic TGA varies between 67 % and 40 % [33], but also 25 % plasma has been successfully used [40]. Here 25 % plasma was selected, because optimum FSAP activation was seen at this dilution (Figure 1 A), similar to reports that in TGA the highest AUC values were seen at 20 % to 30 % plasma [41].…”

Section: Development Of An Fsap Generation Assay (Fga)supporting

confidence: 53%

Development of a Factor VII Activating Protease (FSAP) generation assay and its application in studying FSAP in venous thrombosis

Etscheid¹,

Hanschmann²,

Sandset³

et al. 2022

Thrombosis Research

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Section: Development Of An Fsap Generation Assay (Fga)supporting

confidence: 53%

Development of a Factor VII Activating Protease (FSAP) generation assay and its application in studying FSAP in venous thrombosis

Etscheid¹,

Hanschmann²,

Sandset³

et al. 2022

Thrombosis Research

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“…Attempts to get even closer to the in vivo situation by performing analogous experiments according to our TGT were less successful. In these experiments, FIXa was replaced by 1 p m tissue factor and the FXa specific substrate Glut‐GR‐AMC was exchanged against the thrombin specific substrate B‐VR‐AMC .…”

Section: Resultsmentioning

confidence: 95%

“…We employed thrombin generation test (TGT) as a global test to demonstrate that the ‘peripheral’ inhibitors, CTI and BPTI do not exhibit noticeable interfere with the events leading to coagulation and beyond. This test was performed with CTI/BPTI plasma from four donors with different coagulation characteristics: One represents a normal donor, one was carrier of the FV‐Leiden mutation, causing activated protein C (APC) resistance, another donor has prothrombin overload due to an as yet unknown defect (this donor had a history of two thrombotic events, but G20210A mutation had been excluded by sequencing), and a fourth donor was carrier of FV‐Leiden mutation and was under phenprocoumon therapy (INR ~ 2.5) at the time of blood donation.…”

Section: Resultsmentioning

confidence: 99%

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Factor VIII assay mimicking in vivo coagulation conditions

et al. 2013

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Under certain circumstances, the determination of coagulation factor VIII (FVIII) is hampered by assay discrepancies between clotting and chromogenic approaches. These are observed in certain patients' plasma as well as in certain concentrates. We intended to develop a novel assay for the quantification of coagulation FVIII which reflects the physiological situation better than the established assays. It is based on plasma without chelation of divalent cations and simultaneously minimizes the generation of activated factors which could function as uncontrolled triggers of coagulation. FVIII deficient plasma is prepared with the aid of biotinylated antibodies against FVIII from normal plasma in presence of inhibitors of contact activation. To start the assay only tiny amounts of activated FIX serve as trigger. The FVIII determination is performed in a kinetic experiment and is based on the cleavage of a fluorogenic substrate for activated FX. FVIII concentrations between 0.01 and 1 IU mL(-1) are easily determined. Plasma-derived and recombinant FVIII concentrates were compared. All plasma-derived concentrates were found to contain FVIII activities within the specification of the manufacturer. Recombinant concentrates yielded only 35-50% of the claimed potency. The novel in vivo-like assay avoids the undue advantage or disadvantage of certain product characteristics by eliminating unphysiological assay conditions. Its usefulness could turn out in future experiments with plasma from haemophilia A patients.

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“…The materials as well as the methods used for this study are described in the Supporting Information. The authors have cited additional references within the Supporting Information [29,39,40,43,[59][60][61][62][63][64][65][66][67][68][69][70][71][72]. Supplementary Figures of the protein similarity calculation (Figure S1), fluorometric inhibition assays (Figures S2 and S3), absorption spectra (Figure S4), stability studies (Figure S5), NMR-spectra and HPLC-chromatograms (Figures S6a-S21c) and Table S1 of the computation of physicochemical parameters can be accessed in the supporting information.…”

Section: Methodsmentioning

confidence: 99%

Ligand-Based Design of Selective Peptidomimetic uPA and TMPRSS2 Inhibitors with Arg Bioisosteres

Müller,

Zimmer,

Frey

et al. 2024

IJMS

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Trypsin-like serine proteases are involved in many important physiological processes like blood coagulation and remodeling of the extracellular matrix. On the other hand, they are also associated with pathological conditions. The urokinase-pwlasminogen activator (uPA), which is involved in tissue remodeling, can increase the metastatic behavior of various cancer types when overexpressed and dysregulated. Another member of this protease class that received attention during the SARS-CoV 2 pandemic is TMPRSS2. It is a transmembrane serine protease, which enables cell entry of the coronavirus by processing its spike protein. A variety of different inhibitors have been published against both proteases. However, the selectivity over other trypsin-like serine proteases remains a major challenge. In the current study, we replaced the arginine moiety at the P1 site of peptidomimetic inhibitors with different bioisosteres. Enzyme inhibition studies revealed that the phenylguanidine moiety in the P1 site led to strong affinity for TMPRSS2, whereas the cyclohexylguanidine derivate potently inhibited uPA. Both inhibitors exhibited high selectivity over other structurally similar and physiologically important proteases.

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Calibrating Thrombin Generation in Different Samples: Less Effort with a Less Efficient Substrate

Cited by 4 publications

References 26 publications

Development of a Factor VII Activating Protease (FSAP) generation assay and its application in studying FSAP in venous thrombosis

Development of a Factor VII Activating Protease (FSAP) generation assay and its application in studying FSAP in venous thrombosis

Factor VIII assay mimicking in vivo coagulation conditions

Ligand-Based Design of Selective Peptidomimetic uPA and TMPRSS2 Inhibitors with Arg Bioisosteres

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