- Email: [email protected]
Monitoring Recombinant Factor VIIa Treatment: Efficacy Depends on High Levels of Fibrinogen in a Model of Severe Dilutional Coagulopathy
Monitoring Recombinant Factor VIIa Treatment: Efficacy Depends on High Levels of Fibrinogen in a Model of Severe Dilutional Coagulopathy Michael T. Ganter, MD,* Saskia Schmuck, MD,† Christine R. Hamiel, BS,‡ Paul E. Wischmeyer, MD,‡ Daniela Heule, MD,† Andreas Zollinger, MD,† and Christoph K. Hofer, MD† Objectives: Recombinant activated factor VII (rFVIIa) is increasingly being given to treat massive bleeding. However, there is no clear guidance on which patients are suitable for treatment and how the effects of treatment should be monitored. The aim of this in vitro study was to assess the coagulation status of severely hemodiluted blood samples before and after treatment with therapeutic doses of rFVIIa and/or fibrinogen with 2 viscoelastic point-of-care coagulation analyzers: ROTEM (Pentapharm GmbH, Munich, Germany) and Sonoclot (Sienco Inc, Arvada, CO). Design: Laboratory study. Setting: Research coagulation laboratory. Participants: Ten healthy male volunteers without hereditary or acquired coagulation disorders. Interventions: Blood samples were obtained. After severe hemodilution with albumin 5%, therapeutic doses of rFVIIa and/or fibrinogen were added, and the coagulation status was assessed with new 1:1,000 diluted tissue factor–activated tests from ROTEM and Sonoclot.
Measurements and Main Results: The administration of therapeutic doses of rFVIIa to hemodiluted samples shortened the initiation phase of coagulation only. Isolated fibrinogen administration to physiologic levels improved both the initiation of coagulation as well as clot formation and strength. Combined fibrinogen and rFVIIa administration further improved both effects. Conclusions: ROTEM and Sonoclot were able to monitor the effects of rFVIIa and fibrinogen administration with 1:1,000 diluted tissue factor–activated tests. The efficacy of rFVIIa was largely dependent on the presence of high levels of fibrinogen in reversing this severe dilutional coagulopathy. © 2008 Elsevier Inc. All rights reserved.
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and the Sonoclot analyzer; Sienco Inc, Arvada, CO). The authors’ hypothesis was that rFVIIa may only reverse severe dilutional coagulopathy in the presence of sufficient fibrinogen levels.
ECOMBINANT ACTIVATED FACTOR VII (rFVIIa) increasingly is being given on a compassionate basis to control severe bleeding1 and has been shown to result in a significant reduction in red blood cell transfusion in severe blunt trauma.2 Although consensus guidelines for use of rFVIIa have been published recently,3,4 a paucity of data from randomized controlled trials limit the strength and scope of these recommendations. No specific test is currently available to indicate the need for rFVIIa or to monitor its efficacy. Therefore, the administration of rFVIIa in patients with massive hemorrhage still depends largely on clinical judgment.5 Viscoelastic techniques like thromboelastography/ thromboelastometry or Sonoclot analysis appear to be highly desirable and have shown some promising results.6-8 Coagulation is assessed in whole blood allowing coagulation factors to interact with red cells and platelets. rFVIIa increases thrombin formation by tissue factor– dependent and –independent activation of factor X on the surface of platelets.9 To study the effects of rFVIIa, blood samples need to be activated with minute amounts of tissue factor for best sensitivity.10,11 The presence of high amounts of tissue factor may directly activate the coagulation cascade (bypassing agent), and effects of rFVIIa may no longer be monitored.11 The modern practice of coagulation management is based on rapid diagnosis of the patient’s coagulation status, specific component therapy, and monitoring of the procoagulant treatment.12 Measuring clotting factors during progressive hemodilution showed that fibrinogen is the first factor to become critically low.13,14 Fibrinogen is a key coagulation factor (substrate to form a clot), and isolated fibrinogen substitution in severe models of dilutional coagulopathy resulted in a significantly improved clot strength and reduced blood loss.15-18 The aim of this in vitro study was to determine the efficacy of rFVIIa in a model of severe dilutional coagulopathy by 2 different viscoelastic point-of-care (POC) coagulation analyzers (ROTEM system; Pentapharm GmbH, Munich, Germany;
KEY WORDS: recombinant activated factor VII, fibrinogen concentrate, hemodilution, dilutional coagulopathy, thromboelastography, thromboelastometry, ROTEM, Sonoclot analyzer
METHODS With institutional approval, blood was withdrawn from 10 healthy volunteers. Exclusion criteria were hereditary or acquired coagulation disorders including pharmacologically induced coagulopathies (ie, treatment with any anticoagulants or antiplatelet drugs 14 days before blood withdrawal). Fifty milliliters of venous blood were sampled after application of minimum stasis from the antecubital fossa via a 21-G needle. The blood was instilled into citrated tubes (sodium citrate, 0.109 mol/L; BD Vacutainer, Becton Dickinson), and the initial tube was discarded before collection of the test tubes to avoid tissue factor contamination. An extra tube (EDTA; BD Vacutainer, Becton Dickinson, Franklin Lakes, NJ) was obtained for whole blood count and platelet measurement.
From the *Institute of Anesthesiology, University Hospital Zurich, Zurich, Switzerland; †Institute of Anesthesiology and Intensive Care Medicine, Triemli City Hospital, Zurich, Switzerland; and ‡Department of Anesthesiology, University of Colorado Health Sciences Center, Denver, CO. M.T. Ganter and S. Schmuck contributed equally to this work. Supported by Pentapharm GmbH (Munich, Germany), Sienco Inc (Arvada, CO), and Novo Nordisk (Cophenhagen, Denmark). An educational grant for this study was provided by ZLB Behring (Berne, Switzerland). None of the authors is related to or has financial interests in the manufacturers of products studied. Presented in part at the annual meeting of the American Society of Anesthesiologists, Chicago, IL, October 15-17, 2006. Address reprint requests to Christoph K. Hofer, MD, Institute of Anesthesiology and Intensive Care Medicine, Triemli City Hospital Zurich, Birmensdorferstr 497, 8063 Zurich, Switzerland. E-mail: [email protected] © 2008 Elsevier Inc. All rights reserved. 1053-0770/08/2205-0005$34.00/0 doi:10.1053/j.jvca.2008.01.017
Journal of Cardiothoracic and Vascular Anesthesia, Vol 22, No 5 (October), 2008: pp 675-680
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In order to mimic a scenario of maximum dilution of clotting factors but maintaining a minimally required hemoglobin concentration and platelet count, the authors processed the samples to obtain platelet-rich plasma (PRP, centrifugation at 80g for 8 minutes). PRP was carefully collected, and the remaining sample was recentrifuged (400g for 3 minutes) to further concentrate the red blood cells (RBCs). The supernatant (remaining plasma and buffy coat) was discarded, and the RBC was washed twice with 0.9% normal saline. Then, PRP was diluted 1:20 with albumin 5% (ZLB Behring, Berne, Switzerland; sodium citrate, 0.109 mol/L was added to the albumin solution before the dilution of PRP), and washed RBCs were added to obtain a final targeted hematocrit of 20%. Albumin 5% was chosen in this hemodilution model because it has been shown previously to have the least adverse effect on hemostasis compared with other colloids.19,20 The reconstituted blood samples were treated with a therapeutic dose of rFVIIa (Novo Nordisk, Copenhagen, Denmark; final concentration 1.4 g/mL) corresponding to a clinical dose of 100 g/kg bodyweight. Furthermore, diluted blood samples were treated with fibrinogen (Calbiochem, San Diego, CA; final targeted concentration 2 g/L) alone or combined with rFVIIa. Because the maximum effect of rFVIIa was seen in blood samples treated with fibrinogen, a dose response of rFVIIa was then performed in these blood samples. Whole-blood coagulation analyses were performed with the rotation thromboelastometry ROTEM (Pentapharm GmbH) and the Sonoclot Coagulation and Platelet Function Analyzer (Sienco Inc). Both technologies have been described in detail elsewhere.21,22 Briefly, the measurements are based on the detection of viscoelastic changes of a blood sample after activation with different coagulation activators (1:1,000 diluted tissue factor was used for this study). ROTEM measures and graphically displays the time until initial fibrin formation (coagulation time [CT], denoted as clot initiation), the kinetics of fibrin formation, clot development (␣-angle, denoted as clot propagation), and the ultimate clot strength and stability (maximum clot firmness [MCF]).16,23-25 To study thrombus generation, modified ROTEM parameters (based on the original tracing) have been introduced recently including maximum velocity of clot formation (maximum rate of thrombus generation [MaxVel]), time to reach MaxVel (time to maximum thrombus generation [t-MaxVel]), and total thrombus generation (area under the curve [AUC]).11,23 These parameters are supposed to be more sensitive to rFVIIa than standard ROTEM parameters.26 The Sonoclot analyzer provides information on the entire hemostasis process both in a qualitative graph, known as Sonoclot signature, and as quantitative results including the activated coagulation time (ACT), the clot rate (CR), and the platelet function. The ACT is the time from the activation of the sample until the beginning of a fibrin formation. Besides providing information on the initiation phase of coagulation, the Sonoclot analyzer also measures the kinetics of fibrin formation and clot development, expressed as CR (ie, the maximum slope of the Sonoclot signature during initial fibrin polymerization and clot development). Furthermore, the Sonoclot analyzer analyzes the timing and quality of the clot retraction and calculates the function of the platelets accordingly.25 All analyses were performed at 37°C in duplicate using 1:1,000 diluted tissue factor–activated tests provided by the manufacturer (for ROTEM: tif-TEM; Pentapharm GmbH, Munich, Germany; and for Sonoclot: microPT; Sienco Inc, Arvada, CO). Recalcification of blood samples was done by adding 20 L of 0.25 mol/L of CaCl2 to the test cuvettes containing 20 L of coagulation activator. Subsequently, 330 L of blood specimen were dispensed with a pipette, mixed, and analyzed. Routine coagulation tests included platelet count, prothrombin time (PT), activated partial thromboplastin time, and fibrinogen concentration determined by Clauss method. StatView for Windows version 5.01 (SAS Institute Inc, Cary, NC) and SPSS for Windows Release 12.0.2 (SPSS Inc, Chicago, IL) were
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used to perform the statistical analyses. Analysis of variance with post hoc Bonferroni-Dunn correction was performed to compare the different conditions of the blood samples (p value adjusted to 5 [effect of rFVIIa and fibrinogen on hemodiluted blood samples] and 4 comparisons [dose response of rFVIIa], respectively). Test variability was calculated as the percent difference between duplicate measurements in relation to the mean of duplicate measurements. Results are given as mean ⫾ standard deviation; p ⬍ 0.05 was considered significant. RESULTS
Venous blood was obtained from 10 male donors (age, 35.5 ⫾ 7.5 years). They were nonsmokers, had no history of abnormal bleeding, and presented without a coagulation disorder or anemia (Table 1). Diluting blood samples according to the authors’ model resulted in a final hematocrit of 19% on average and significantly impaired standard coagulation values (Table 1). ROTEM and Sonoclot variables reflected the severe hemodilution; ROTEM’s CT and t-MaxVel significantly increased, whereas all other variables (angle ␣, MCF, MaxVel, and AUC) significantly decreased. The same effect was observed for the Sonoclot variables ACT and CR (Figs 1 and 2). The administration of therapeutic doses of rFVIIa to hemodiluted samples significantly shortened PT (⫺31 ⫾ 11 seconds), ROTEM’s CT (⫺180 ⫾ 90 seconds), and Sonoclot’s ACT (⫺88 ⫾ 180 seconds). However, no effects on ROTEM’s angle ␣, MCF, and Sonoclot’s CR were observed (Figs 1 and 2). Single administration of fibrinogen to diluted samples resulted in a final concentration of fibrinogen of 2.0 ⫾ 0.3 g/L as determined by the Clauss method. Compared with hemodiluted blood samples, fibrinogen substitution decreased PT significantly by ⫺12 ⫾ 7 seconds. Furthermore, all ROTEM and Sonoclot variables improved significantly (Figs 1 and 2). There was a reduction of CT, t-MaxVel, and ACT values combined with an increase of angle ␣, MCF, MaxVel, AUC, and CR values. The combined application of rFVIIa and fibrinogen further reduced PT significantly (⫺15 ⫾ 9 seconds). ROTEM’s CT and t-MaxVel significantly decreased. Angle ␣, MCF, MaxVel, and AUC significantly increased. A similar effect was observed for the Sonoclot variables ACT and CR (Figs 1 and 2). Because the administration of fibrinogen was necessary for rFVIIa to show an effect in the dilutional model, a dose response in samples containing fibrinogen was performed. ROTEM’s CT and Sonoclot’s ACT improved equally in all doses studied, even at the lowest dose. ROTEM’s angle ␣, MCF, and Sonoclot’s CR showed comparable results at half of the recommended dose compared with the recommended dose, but the procoagulant effect was lost at a quarter of the recom-
Table 1. Hematocrit and Standard Coagulation Variables Before and After Hemodilution
HCT (%) PT (s) aPTT (s) Platelets (103/mm3) Fibrinogen (g/L)
Baseline
Hemodilution
42 ⫾ 3 10 ⫾ 1 42 ⫾ 5 178 ⫾ 62 2.31 ⫾ 0.47
19 ⫾ 2 74 ⫾ 20 ⬎180 29 ⫾ 14 0.15 ⫾ 0.21
Abbreviation: HCT, hematocrit.
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Fig 1. Effects of rFVIIa and/or fibrinogen substitution on ROTEM and Sonoclot variables. The 2 phases of coagulation, initiation of coagulation (A) and clot formation and strength and stability (B) are analyzed by the ROTEM and Sonoclot analyzer. #p < 0.05: effect of modified hemodilution; §p < 0.05: effect of therapeutic doses of rFVIIa; °p < 0.05: effect of fibrinogen administration.
mended dose. Again, the new ROTEM variables did follow the trend of the CT, angle ␣, and MA (Table 2). The overall ROTEM test variability was 14% ⫾ 14% for CT, 9% ⫾ 11% for angle ␣, 10% ⫾ 12% for MCF, 13% ⫾ 14% for t-MaxVel, 9% ⫾ 13% for MaxVel, and 10% ⫾ 16% for AUC. For the Sonoclot Analyzer test, variability was 9% ⫾ 18% for ACT and 10% ⫾ 18% for CR. DISCUSSION
The present study investigated the effects of administration of rFVIIa and fibrinogen in an in vitro hemodilution model. The ROTEM and Sonoclot analyzer were able to monitor the procoagulant effects of rFVIIa and fibrinogen administration with diluted tissue factor–activated tests, tif-TEM, and MicroPT.
Interestingly, rFVIIa required high concentrations of fibrinogen in order to improve the severe coagulopathy. In the initial period of fluid resuscitation of patients with massive hemorrhage, large amounts of crystalloids, colloids, and universal 0 type RBCs are typically infused. Testing and preparing of blood coagulation products (eg, fresh frozen plasma, cryoprecipitate, and platelets) is time-consuming. Therefore, a severe dilutional coagulopathy may develop in the early period of massive transfusion because these coagulation products may not be readily available. The dilutional model aimed at reproducing an extreme dilutional coagulopathy but keeping minimal hemoglobin and platelet levels (Table 1). In this model of severe hemodilution, rFVIIa only improved the initiation phase of coagulation (PT, CT, and ACT). By contrast,
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Fig 2. The effects of recombinant factor VIIa (rFVIIa) and fibrinogen on additional ROTEM variables. #p < 0.05: effect of modified hemodilution; §p < 0.05: effect of therapeutic doses of rFVIIa; °p < 0.05: effect of fibrinogen administration.
isolated fibrinogen administration improved not only the initiation of coagulation but also formation and strength of the developing clot (␣-angle, MCF, and CR). Combined application of rFVIIa and fibrinogen further improved the coagulation status of the sample significantly. There is a growing body of evidence suggesting that aggressive fibrinogen substitution may significantly reverse dilutional coagulopathy, thereby reducing blood loss after severe injury.15-18 The substitution of fibrinogen in the authors’ dilutional model up to 2 g/L significantly improved the coagulation status of the blood samples. Fibrinogen is the substrate to form a clot, thereby explaining its key role in coagulation. Furthermore, combining fibrinogen and prothrombin complex concentrate (factor II, VII, IX, and X) administration has recently been shown to further improve dilutional coagulopathy resulting in normalization of coagulation parameters measured.27 rFVIIa treatment is currently approved for patients with congenital or acquired hemophilia with antibodies to factor VIII or IX (United States and Europe), factor VII deficiency,
and Glanzmanns thrombasthenia (Europe). However, rVIIa is increasingly used in off-label indications to control severe bleeding.11 Because rFVIIa is a very potent prohemostatic agent, there is concern that rFVIIa may cause thromboembolic adverse events resulting in serious morbidity and mortality.28,29 Therefore, the risks and benefits have to be carefully outweighed before each single administration. In cardiac surgery, for example, there is little evidence to suggest a prophylactic use of rFVIIa. However, in patients experiencing refractory postoperative hemorrhage, the use of rFVIIa seems promising and relatively safe, although definitive evidence from randomized controlled trials is lacking.30,31 Doses of rFVIIa ranging from 20 to 200 g/kg have been given with varying success, and 90 to 120 g/kg of rFVIIa is generally considered the recommended initial dose.3,4,32 The present results in severe hemodilution suggest that half of the recommended dose (⬃50 g/kg, final concentration of 0.7 g/mL) has a similar effect as compared with the full dose. Further decreasing the administered dose, however, resulted in a loss of the procoagulant effect of rFVIIa.
Table 2. rFVIIa Dose Response for ROTEM and Sonoclot Variables in Hemodiluted Blood Samples After Fibrinogen Substitution rVIIa
CTROTEM (s) ACTSonoclot (s) CFTROTEM (s) Angle ␣ROTEM (°) MCFROTEM (mm) CRSonoclot t-MaxVelROTEM (s) MaxVelROTEM (cm/s) AUCROTEM (mm2)
Dilution ⫹ Fibrinogen
⫹0.35 g/mL
⫹0.7 g/mL
⫹1.4 g/mL
563 ⫾ 102 375 ⫾ 66 434 ⫾ 141 41 ⫾ 10 24 ⫾ 4 6⫾1 628 ⫾ 112 5⫾1 2,652 ⫾ 461
404 ⫾ 82* 230 ⫾ 34* 444 ⫾ 139* 41 ⫾ 11 25 ⫾ 5 6⫾2 455 ⫾ 114* 5⫾1 2,732 ⫾ 540
396 ⫾ 50* 224 ⫾ 43* 446 ⫾ 121* 46 ⫾ 8*† 27 ⫾ 4*† 7 ⫾ 1*† 475 ⫾ 102*† 6 ⫾ 3*† 2,786 ⫾ 492
385 ⫾ 60* 215 ⫾ 26* 451 ⫾ 104* 47 ⫾ 7*† 27 ⫾ 4*† 7 ⫾ 1*† 436 ⫾ 62*† 6 ⫾ 3*† 2,917 ⫾ 447*
*p ⬍ 0.05: effect of rFVIIa (doses of 1.4 g/mL, 0.7 g/mL, and 0.35 g/mL compared with hemodiluted blood samples after fibrinogen substitution). †p ⬍ 0.05: effect of rFVIIa (doses of 1.4 g/mL and 0.7 g/mL compared with 0.35 g/mL).
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The present data are in accordance with previously published reports showing that isolated rFVIIa administration has failed to correct coagulopathy in an in vitro model of hemodilution.33 Furthermore, rFVIIa treatment has shown minimal effects on blood loss after major hemorrhage in animals with severe dilutional coagulopathy.34,35 The concept of rFVIIa is to activate coagulation at sites of tissue factor exposure. The resulting thrombin burst then leads to the formation of a fibrin clot, provided sufficient fibrinogen levels and platelets are present. In order to get the maximum effect of rFVIIa, consensus guidelines recommend first that the bleeding source should be controlled as best as possible and second that patients be optimized before the administration of rFVIIa targeting a hematocrit ⬎24%, fibrinogen ⬎0.5 to 1 g/L, platelets ⬎50 to 100,000 ⫻ 109/L, and pH ⱖ7.2.3,4,32 In the dilutional model, however, rFVIIa improved the coagulation status significantly even with lower platelets (32,000 ⫻ 109/L) if prior fibrinogen substitution was performed. ROTEM and the Sonoclot analyzer are both viscoelastic POC coagulation analyzers. They measure the entire coagulation process starting with fibrin formation and continue through to clot retraction and lysis at the bedside with minimal time delays. Furthermore, physiologic clot development is depicted as a result of whole-blood analysis of the coagulation status. ROTEM measures the shear elasticity of the blood sample. The rotation of the pin begins to be impaired after fibrin-platelet bonding has linked the cup and pin together. The strength of these fibrin-platelet bonds affects the magnitude of the pin motion. Thus, the output is directly related to the strength of the formed clot. The Sonoclot analyzer, on the other hand, uses a different approach. A plastic probe is immersed and oscillates vertically in the sample. The output is sensitive to viscosity and monitors viscosity changes that occur during the initiation of coagulation and clot development. Viscoelastic POC analyzers have been used to evaluate the effects of hemostatic agents, such as rFVIIa.6-8 In theses studies, thromboelastography/thromboelastometry seems to be a promising method for the characterization of phenotypic variance among patients as well as in detection of the individual response to rFVIIa before and after rFVIIa administration. The presence of high amounts of tissue factor may directly activate the coagulation cascade (bypassing agent), and the effects of rFVIIa may no longer be monitored. Therefore, activation with
minute amounts of tissue factor has been recommended to visualize the particular signature in different coagulopathies and particularly to show the rFVIIa response.11 Recently, modified parameters of the thromboelastography/ thromboelastometry have been introduced based on the first derivative of the original tracing and have been shown to correlate closely with thrombin formation.11,23 These parameters, t-MaxVel, MaxVel, and total thrombus generation (AUC), are supposed to be more sensitive to rFVIIa treatment than standard thromboelastography/thromboelastometry parameters.26 However, these modified parameters did not better perform in monitoring rFVIIa administration in the present study compared with ROTEM’s conventional ␣-angle and MCF as well as Sonoclot’s CR. The interpretation of the data presented has to be within the limitations of an in vitro investigation with cautious extensions of the findings into clinical application only. In vitro coagulation studies may not necessarily reflect in vivo conditions because the effects of tissue damage, endothelial injury, and physiologic reactions to correct coagulation are missing in vitro. Furthermore, the study was performed with citrated blood samples of healthy male volunteers only. Additionally, the authors chose to study severe hemodilution with albumin 5% to have minimal effects on coagulation other than dilutional. It is likely that in vitro hemodilution with other colloids or crystalloids will show different results. Nevertheless, the present study provides some mechanistic insights into how rFVIIa is dependent on a sufficient concentration of fibrinogen and investigates for the first time the 2 POC coagulation analyzers ROTEM and Sonoclot in this indication. In summary, the administration of rFVIIa alone resulted in the present in vitro model of severe hemodilution in a shortened initiation phase of coagulation as detected by ROTEM and Sonoclot. Isolated fibrinogen administration to physiologic concentrations improved both the initiation of coagulation as well as clot formation and strength. Combined fibrinogen and rFVIIa administration further improved both effects significantly. These data suggest that fibrinogen is a key component in the coagulation process and that adequate levels of fibrinogen should be present before considering the administration of rFVIIa. However, further studies in vivo are required to confirm these findings.
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does not alter mortality and outcome. Clin Lab Haematol 28:309-312, 2006 6. Sorensen B, Ingerslev J: Thromboelastography and recombinant factor VIIa-hemophilia and beyond. Semin Hematol 41:140-144, 2004 7. Sorensen B, Ingerslev J: Whole blood clot formation phenotypes in hemophilia A and rare coagulation disorders. Patterns of response to recombinant factor VIIa. J Thromb Haemost 2:102-110, 2004 8. Kawaguchi C, Takahashi Y, Hanesaka Y, et al: The in vitro analysis of the coagulation mechanism of activated factor VII using thromboelastogram. Thromb Haemost 88:768-772, 2002 9. Pusateri AE, Park MS: Mechanistic implications for the use and monitoring of recombinant activated factor VII in trauma. Crit Care 9:S15-S24, 2005 (suppl) 10. Engstrom M, Reinstrup P, Schott U: An in vitro evaluation of standard rotational thromboelastography in monitoring of effects of
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recombinant factor VIIa on coagulopathy induced by hydroxyethyl starch. BMC Blood Disord 5:3, 2005 11. Sorensen B, Johansen P, Christiansen K, et al: Whole blood coagulation thromboelastographic profiles employing minimal tissue factor activation. J Thromb Haemost 1:551-558, 2003 12. Rossaint R, Cerny V, Coats TJ, et al: Key issues in advanced bleeding care in trauma. Shock 26:322-331, 2006 13. Hiippala ST, Myllyla GJ, Vahtera EM: Hemostatic factors and replacement of major blood loss with plasma-poor red cell concentrates. Anesth Analg 81:360-365, 1995 14. Singbartl K, Innerhofer P, Radvan J, et al: Hemostasis and hemodilution: A quantitative mathematical guide for clinical practice. Anesth Analg 96:929-935, 2003 15. Fenger-Eriksen C, Anker-Moller E, Heslop J, et al: Thromboelastographic whole blood clot formation after ex vivo addition of plasma substitutes: Improvements of the induced coagulopathy with fibrinogen concentrate. Br J Anaesth 94:324-329, 2005 16. Fries D, Innerhofer P, Reif C, et al: The effect of fibrinogen substitution on reversal of dilutional coagulopathy: An in vitro model. Anesth Analg 102:347-351, 2006 17. De LC, Calatzis A, Welsch U, et al: Fibrinogen concentrate reverses dilutional coagulopathy induced in vitro by saline but not by hydroxyethyl starch 6%. Anesth Analg 102:1194-1200, 2006 18. Fries D, Krismer A, Klingler A, et al: Effect of fibrinogen on reversal of dilutional coagulopathy: A porcine model. Br J Anaesth 95:172-177, 2005 19. Egli GA, Zollinger A, Seifert B, et al: Effect of progressive haemodilution with hydroxyethyl starch, gelatin and albumin on blood coagulation. Br J Anaesth 78:684-689, 1997 20. Niemi TT, Suojaranta-Ylinen RT, Kukkonen SI, et al: Gelatin and hydroxyethyl starch, but not albumin, impair hemostasis after cardiac surgery. Anesth Analg 102:998-1006, 2006 21. Luddington RJ: Thromboelastography/thromboelastometry. Clin Lab Haematol 27:81-90, 2005 22. Hett DA, Walker D, Pilkington SN, et al: Sonoclot analysis. Br J Anaesth 75:771-776, 1995 23. Rivard GE, Brummel-Ziedins KE, Mann KG, et al: Evaluation of the profile of thrombin generation during the process of whole blood
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clotting as assessed by thromboelastography. J Thromb Haemost 3:2039-2043, 2005 24. Nielsen VG: A comparison of the thromboelastograph and the ROTEM. Blood Coagul Fibrinolysis 18:247-252, 2007 25. Ganter MT, Hofer CK: Coagulation monitoring: current techniques and clinical use of viscoelastic point-of-care coagulation devices. Anesth Analg (in press) 26. Sorensen B, Ingerslev J: Tailoring haemostatic treatment to patient requirements—An update on monitoring haemostatic response using thromboelastography. Haemophilia 11:1-6, 2005 (suppl) 27. Fries D, Haas T, Klingler A, et al: Efficacy of fibrinogen and prothrombin complex concentrate used to reverse dilutional coagulopathy—A porcine model. Br J Anaesth 97:460-467, 2006 28. O’Connell KA, Wood JJ, Wise RP, et al: Thromboembolic adverse events after use of recombinant human coagulation factor VIIa. JAMA 295:293-298, 2006 29. Lichtman AD, Carullo V, Minhaj M, et al: Case 6 —2007: Massive intraoperative thrombosis and death after recombinant activated factor VII administration. J Cardiothorac Vasc Anesth 21:897902, 2007 30. Warren O, Mandal K, Hadjianastassiou V, et al: Recombinant activated factor VII in cardiac surgery: A systematic review. Ann Thorac Surg 83:707-714, 2007 31. Karkouti K, Beattie WS, Crowther MA, et al: The role of recombinant factor VIIa in on-pump cardiac surgery: Proceedings of the Canadian Consensus Conference. Can J Anaesth 54:573-582, 2007 32. Martinowitz U, Michaelson M: Guidelines for the use of recombinant activated factor VII (rFVIIa) in uncontrolled bleeding: A report by the Israeli Multidisciplinary rFVIIa Task Force. J Thromb Haemost 3:640-648, 2005 33. Sorensen B, Fenger-Eriksen C, Ingerslev J: Recombinant factor VIIa fails to correct coagulopathy induced by haemodilution with colloid. Br J Anaesth 94:862-863, 2005 34. Schreiber MA, Holcomb JB, Hedner U, et al: The effect of recombinant factor VIIa on coagulopathic pigs with grade V liver injuries. J Trauma 53:252-257, 2002 35. Sondeen JL, Pusateri AE, Hedner U, et al: Recombinant factor VIIa increases the pressure at which rebleeding occurs in porcine uncontrolled aortic hemorrhage model. Shock 22:163-168, 2004
Measurements and Main Results: The administration of therapeutic doses of rFVIIa to hemodiluted samples shortened the initiation phase of coagulation only. Isolated fibrinogen administration to physiologic levels improved both the initiation of coagulation as well as clot formation and strength. Combined fibrinogen and rFVIIa administration further improved both effects. Conclusions: ROTEM and Sonoclot were able to monitor the effects of rFVIIa and fibrinogen administration with 1:1,000 diluted tissue factor–activated tests. The efficacy of rFVIIa was largely dependent on the presence of high levels of fibrinogen in reversing this severe dilutional coagulopathy. © 2008 Elsevier Inc. All rights reserved.
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and the Sonoclot analyzer; Sienco Inc, Arvada, CO). The authors’ hypothesis was that rFVIIa may only reverse severe dilutional coagulopathy in the presence of sufficient fibrinogen levels.
ECOMBINANT ACTIVATED FACTOR VII (rFVIIa) increasingly is being given on a compassionate basis to control severe bleeding1 and has been shown to result in a significant reduction in red blood cell transfusion in severe blunt trauma.2 Although consensus guidelines for use of rFVIIa have been published recently,3,4 a paucity of data from randomized controlled trials limit the strength and scope of these recommendations. No specific test is currently available to indicate the need for rFVIIa or to monitor its efficacy. Therefore, the administration of rFVIIa in patients with massive hemorrhage still depends largely on clinical judgment.5 Viscoelastic techniques like thromboelastography/ thromboelastometry or Sonoclot analysis appear to be highly desirable and have shown some promising results.6-8 Coagulation is assessed in whole blood allowing coagulation factors to interact with red cells and platelets. rFVIIa increases thrombin formation by tissue factor– dependent and –independent activation of factor X on the surface of platelets.9 To study the effects of rFVIIa, blood samples need to be activated with minute amounts of tissue factor for best sensitivity.10,11 The presence of high amounts of tissue factor may directly activate the coagulation cascade (bypassing agent), and effects of rFVIIa may no longer be monitored.11 The modern practice of coagulation management is based on rapid diagnosis of the patient’s coagulation status, specific component therapy, and monitoring of the procoagulant treatment.12 Measuring clotting factors during progressive hemodilution showed that fibrinogen is the first factor to become critically low.13,14 Fibrinogen is a key coagulation factor (substrate to form a clot), and isolated fibrinogen substitution in severe models of dilutional coagulopathy resulted in a significantly improved clot strength and reduced blood loss.15-18 The aim of this in vitro study was to determine the efficacy of rFVIIa in a model of severe dilutional coagulopathy by 2 different viscoelastic point-of-care (POC) coagulation analyzers (ROTEM system; Pentapharm GmbH, Munich, Germany;
KEY WORDS: recombinant activated factor VII, fibrinogen concentrate, hemodilution, dilutional coagulopathy, thromboelastography, thromboelastometry, ROTEM, Sonoclot analyzer
METHODS With institutional approval, blood was withdrawn from 10 healthy volunteers. Exclusion criteria were hereditary or acquired coagulation disorders including pharmacologically induced coagulopathies (ie, treatment with any anticoagulants or antiplatelet drugs 14 days before blood withdrawal). Fifty milliliters of venous blood were sampled after application of minimum stasis from the antecubital fossa via a 21-G needle. The blood was instilled into citrated tubes (sodium citrate, 0.109 mol/L; BD Vacutainer, Becton Dickinson), and the initial tube was discarded before collection of the test tubes to avoid tissue factor contamination. An extra tube (EDTA; BD Vacutainer, Becton Dickinson, Franklin Lakes, NJ) was obtained for whole blood count and platelet measurement.
From the *Institute of Anesthesiology, University Hospital Zurich, Zurich, Switzerland; †Institute of Anesthesiology and Intensive Care Medicine, Triemli City Hospital, Zurich, Switzerland; and ‡Department of Anesthesiology, University of Colorado Health Sciences Center, Denver, CO. M.T. Ganter and S. Schmuck contributed equally to this work. Supported by Pentapharm GmbH (Munich, Germany), Sienco Inc (Arvada, CO), and Novo Nordisk (Cophenhagen, Denmark). An educational grant for this study was provided by ZLB Behring (Berne, Switzerland). None of the authors is related to or has financial interests in the manufacturers of products studied. Presented in part at the annual meeting of the American Society of Anesthesiologists, Chicago, IL, October 15-17, 2006. Address reprint requests to Christoph K. Hofer, MD, Institute of Anesthesiology and Intensive Care Medicine, Triemli City Hospital Zurich, Birmensdorferstr 497, 8063 Zurich, Switzerland. E-mail: [email protected] © 2008 Elsevier Inc. All rights reserved. 1053-0770/08/2205-0005$34.00/0 doi:10.1053/j.jvca.2008.01.017
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In order to mimic a scenario of maximum dilution of clotting factors but maintaining a minimally required hemoglobin concentration and platelet count, the authors processed the samples to obtain platelet-rich plasma (PRP, centrifugation at 80g for 8 minutes). PRP was carefully collected, and the remaining sample was recentrifuged (400g for 3 minutes) to further concentrate the red blood cells (RBCs). The supernatant (remaining plasma and buffy coat) was discarded, and the RBC was washed twice with 0.9% normal saline. Then, PRP was diluted 1:20 with albumin 5% (ZLB Behring, Berne, Switzerland; sodium citrate, 0.109 mol/L was added to the albumin solution before the dilution of PRP), and washed RBCs were added to obtain a final targeted hematocrit of 20%. Albumin 5% was chosen in this hemodilution model because it has been shown previously to have the least adverse effect on hemostasis compared with other colloids.19,20 The reconstituted blood samples were treated with a therapeutic dose of rFVIIa (Novo Nordisk, Copenhagen, Denmark; final concentration 1.4 g/mL) corresponding to a clinical dose of 100 g/kg bodyweight. Furthermore, diluted blood samples were treated with fibrinogen (Calbiochem, San Diego, CA; final targeted concentration 2 g/L) alone or combined with rFVIIa. Because the maximum effect of rFVIIa was seen in blood samples treated with fibrinogen, a dose response of rFVIIa was then performed in these blood samples. Whole-blood coagulation analyses were performed with the rotation thromboelastometry ROTEM (Pentapharm GmbH) and the Sonoclot Coagulation and Platelet Function Analyzer (Sienco Inc). Both technologies have been described in detail elsewhere.21,22 Briefly, the measurements are based on the detection of viscoelastic changes of a blood sample after activation with different coagulation activators (1:1,000 diluted tissue factor was used for this study). ROTEM measures and graphically displays the time until initial fibrin formation (coagulation time [CT], denoted as clot initiation), the kinetics of fibrin formation, clot development (␣-angle, denoted as clot propagation), and the ultimate clot strength and stability (maximum clot firmness [MCF]).16,23-25 To study thrombus generation, modified ROTEM parameters (based on the original tracing) have been introduced recently including maximum velocity of clot formation (maximum rate of thrombus generation [MaxVel]), time to reach MaxVel (time to maximum thrombus generation [t-MaxVel]), and total thrombus generation (area under the curve [AUC]).11,23 These parameters are supposed to be more sensitive to rFVIIa than standard ROTEM parameters.26 The Sonoclot analyzer provides information on the entire hemostasis process both in a qualitative graph, known as Sonoclot signature, and as quantitative results including the activated coagulation time (ACT), the clot rate (CR), and the platelet function. The ACT is the time from the activation of the sample until the beginning of a fibrin formation. Besides providing information on the initiation phase of coagulation, the Sonoclot analyzer also measures the kinetics of fibrin formation and clot development, expressed as CR (ie, the maximum slope of the Sonoclot signature during initial fibrin polymerization and clot development). Furthermore, the Sonoclot analyzer analyzes the timing and quality of the clot retraction and calculates the function of the platelets accordingly.25 All analyses were performed at 37°C in duplicate using 1:1,000 diluted tissue factor–activated tests provided by the manufacturer (for ROTEM: tif-TEM; Pentapharm GmbH, Munich, Germany; and for Sonoclot: microPT; Sienco Inc, Arvada, CO). Recalcification of blood samples was done by adding 20 L of 0.25 mol/L of CaCl2 to the test cuvettes containing 20 L of coagulation activator. Subsequently, 330 L of blood specimen were dispensed with a pipette, mixed, and analyzed. Routine coagulation tests included platelet count, prothrombin time (PT), activated partial thromboplastin time, and fibrinogen concentration determined by Clauss method. StatView for Windows version 5.01 (SAS Institute Inc, Cary, NC) and SPSS for Windows Release 12.0.2 (SPSS Inc, Chicago, IL) were
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used to perform the statistical analyses. Analysis of variance with post hoc Bonferroni-Dunn correction was performed to compare the different conditions of the blood samples (p value adjusted to 5 [effect of rFVIIa and fibrinogen on hemodiluted blood samples] and 4 comparisons [dose response of rFVIIa], respectively). Test variability was calculated as the percent difference between duplicate measurements in relation to the mean of duplicate measurements. Results are given as mean ⫾ standard deviation; p ⬍ 0.05 was considered significant. RESULTS
Venous blood was obtained from 10 male donors (age, 35.5 ⫾ 7.5 years). They were nonsmokers, had no history of abnormal bleeding, and presented without a coagulation disorder or anemia (Table 1). Diluting blood samples according to the authors’ model resulted in a final hematocrit of 19% on average and significantly impaired standard coagulation values (Table 1). ROTEM and Sonoclot variables reflected the severe hemodilution; ROTEM’s CT and t-MaxVel significantly increased, whereas all other variables (angle ␣, MCF, MaxVel, and AUC) significantly decreased. The same effect was observed for the Sonoclot variables ACT and CR (Figs 1 and 2). The administration of therapeutic doses of rFVIIa to hemodiluted samples significantly shortened PT (⫺31 ⫾ 11 seconds), ROTEM’s CT (⫺180 ⫾ 90 seconds), and Sonoclot’s ACT (⫺88 ⫾ 180 seconds). However, no effects on ROTEM’s angle ␣, MCF, and Sonoclot’s CR were observed (Figs 1 and 2). Single administration of fibrinogen to diluted samples resulted in a final concentration of fibrinogen of 2.0 ⫾ 0.3 g/L as determined by the Clauss method. Compared with hemodiluted blood samples, fibrinogen substitution decreased PT significantly by ⫺12 ⫾ 7 seconds. Furthermore, all ROTEM and Sonoclot variables improved significantly (Figs 1 and 2). There was a reduction of CT, t-MaxVel, and ACT values combined with an increase of angle ␣, MCF, MaxVel, AUC, and CR values. The combined application of rFVIIa and fibrinogen further reduced PT significantly (⫺15 ⫾ 9 seconds). ROTEM’s CT and t-MaxVel significantly decreased. Angle ␣, MCF, MaxVel, and AUC significantly increased. A similar effect was observed for the Sonoclot variables ACT and CR (Figs 1 and 2). Because the administration of fibrinogen was necessary for rFVIIa to show an effect in the dilutional model, a dose response in samples containing fibrinogen was performed. ROTEM’s CT and Sonoclot’s ACT improved equally in all doses studied, even at the lowest dose. ROTEM’s angle ␣, MCF, and Sonoclot’s CR showed comparable results at half of the recommended dose compared with the recommended dose, but the procoagulant effect was lost at a quarter of the recom-
Table 1. Hematocrit and Standard Coagulation Variables Before and After Hemodilution
HCT (%) PT (s) aPTT (s) Platelets (103/mm3) Fibrinogen (g/L)
Baseline
Hemodilution
42 ⫾ 3 10 ⫾ 1 42 ⫾ 5 178 ⫾ 62 2.31 ⫾ 0.47
19 ⫾ 2 74 ⫾ 20 ⬎180 29 ⫾ 14 0.15 ⫾ 0.21
Abbreviation: HCT, hematocrit.
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Fig 1. Effects of rFVIIa and/or fibrinogen substitution on ROTEM and Sonoclot variables. The 2 phases of coagulation, initiation of coagulation (A) and clot formation and strength and stability (B) are analyzed by the ROTEM and Sonoclot analyzer. #p < 0.05: effect of modified hemodilution; §p < 0.05: effect of therapeutic doses of rFVIIa; °p < 0.05: effect of fibrinogen administration.
mended dose. Again, the new ROTEM variables did follow the trend of the CT, angle ␣, and MA (Table 2). The overall ROTEM test variability was 14% ⫾ 14% for CT, 9% ⫾ 11% for angle ␣, 10% ⫾ 12% for MCF, 13% ⫾ 14% for t-MaxVel, 9% ⫾ 13% for MaxVel, and 10% ⫾ 16% for AUC. For the Sonoclot Analyzer test, variability was 9% ⫾ 18% for ACT and 10% ⫾ 18% for CR. DISCUSSION
The present study investigated the effects of administration of rFVIIa and fibrinogen in an in vitro hemodilution model. The ROTEM and Sonoclot analyzer were able to monitor the procoagulant effects of rFVIIa and fibrinogen administration with diluted tissue factor–activated tests, tif-TEM, and MicroPT.
Interestingly, rFVIIa required high concentrations of fibrinogen in order to improve the severe coagulopathy. In the initial period of fluid resuscitation of patients with massive hemorrhage, large amounts of crystalloids, colloids, and universal 0 type RBCs are typically infused. Testing and preparing of blood coagulation products (eg, fresh frozen plasma, cryoprecipitate, and platelets) is time-consuming. Therefore, a severe dilutional coagulopathy may develop in the early period of massive transfusion because these coagulation products may not be readily available. The dilutional model aimed at reproducing an extreme dilutional coagulopathy but keeping minimal hemoglobin and platelet levels (Table 1). In this model of severe hemodilution, rFVIIa only improved the initiation phase of coagulation (PT, CT, and ACT). By contrast,
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Fig 2. The effects of recombinant factor VIIa (rFVIIa) and fibrinogen on additional ROTEM variables. #p < 0.05: effect of modified hemodilution; §p < 0.05: effect of therapeutic doses of rFVIIa; °p < 0.05: effect of fibrinogen administration.
isolated fibrinogen administration improved not only the initiation of coagulation but also formation and strength of the developing clot (␣-angle, MCF, and CR). Combined application of rFVIIa and fibrinogen further improved the coagulation status of the sample significantly. There is a growing body of evidence suggesting that aggressive fibrinogen substitution may significantly reverse dilutional coagulopathy, thereby reducing blood loss after severe injury.15-18 The substitution of fibrinogen in the authors’ dilutional model up to 2 g/L significantly improved the coagulation status of the blood samples. Fibrinogen is the substrate to form a clot, thereby explaining its key role in coagulation. Furthermore, combining fibrinogen and prothrombin complex concentrate (factor II, VII, IX, and X) administration has recently been shown to further improve dilutional coagulopathy resulting in normalization of coagulation parameters measured.27 rFVIIa treatment is currently approved for patients with congenital or acquired hemophilia with antibodies to factor VIII or IX (United States and Europe), factor VII deficiency,
and Glanzmanns thrombasthenia (Europe). However, rVIIa is increasingly used in off-label indications to control severe bleeding.11 Because rFVIIa is a very potent prohemostatic agent, there is concern that rFVIIa may cause thromboembolic adverse events resulting in serious morbidity and mortality.28,29 Therefore, the risks and benefits have to be carefully outweighed before each single administration. In cardiac surgery, for example, there is little evidence to suggest a prophylactic use of rFVIIa. However, in patients experiencing refractory postoperative hemorrhage, the use of rFVIIa seems promising and relatively safe, although definitive evidence from randomized controlled trials is lacking.30,31 Doses of rFVIIa ranging from 20 to 200 g/kg have been given with varying success, and 90 to 120 g/kg of rFVIIa is generally considered the recommended initial dose.3,4,32 The present results in severe hemodilution suggest that half of the recommended dose (⬃50 g/kg, final concentration of 0.7 g/mL) has a similar effect as compared with the full dose. Further decreasing the administered dose, however, resulted in a loss of the procoagulant effect of rFVIIa.
Table 2. rFVIIa Dose Response for ROTEM and Sonoclot Variables in Hemodiluted Blood Samples After Fibrinogen Substitution rVIIa
CTROTEM (s) ACTSonoclot (s) CFTROTEM (s) Angle ␣ROTEM (°) MCFROTEM (mm) CRSonoclot t-MaxVelROTEM (s) MaxVelROTEM (cm/s) AUCROTEM (mm2)
Dilution ⫹ Fibrinogen
⫹0.35 g/mL
⫹0.7 g/mL
⫹1.4 g/mL
563 ⫾ 102 375 ⫾ 66 434 ⫾ 141 41 ⫾ 10 24 ⫾ 4 6⫾1 628 ⫾ 112 5⫾1 2,652 ⫾ 461
404 ⫾ 82* 230 ⫾ 34* 444 ⫾ 139* 41 ⫾ 11 25 ⫾ 5 6⫾2 455 ⫾ 114* 5⫾1 2,732 ⫾ 540
396 ⫾ 50* 224 ⫾ 43* 446 ⫾ 121* 46 ⫾ 8*† 27 ⫾ 4*† 7 ⫾ 1*† 475 ⫾ 102*† 6 ⫾ 3*† 2,786 ⫾ 492
385 ⫾ 60* 215 ⫾ 26* 451 ⫾ 104* 47 ⫾ 7*† 27 ⫾ 4*† 7 ⫾ 1*† 436 ⫾ 62*† 6 ⫾ 3*† 2,917 ⫾ 447*
*p ⬍ 0.05: effect of rFVIIa (doses of 1.4 g/mL, 0.7 g/mL, and 0.35 g/mL compared with hemodiluted blood samples after fibrinogen substitution). †p ⬍ 0.05: effect of rFVIIa (doses of 1.4 g/mL and 0.7 g/mL compared with 0.35 g/mL).
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The present data are in accordance with previously published reports showing that isolated rFVIIa administration has failed to correct coagulopathy in an in vitro model of hemodilution.33 Furthermore, rFVIIa treatment has shown minimal effects on blood loss after major hemorrhage in animals with severe dilutional coagulopathy.34,35 The concept of rFVIIa is to activate coagulation at sites of tissue factor exposure. The resulting thrombin burst then leads to the formation of a fibrin clot, provided sufficient fibrinogen levels and platelets are present. In order to get the maximum effect of rFVIIa, consensus guidelines recommend first that the bleeding source should be controlled as best as possible and second that patients be optimized before the administration of rFVIIa targeting a hematocrit ⬎24%, fibrinogen ⬎0.5 to 1 g/L, platelets ⬎50 to 100,000 ⫻ 109/L, and pH ⱖ7.2.3,4,32 In the dilutional model, however, rFVIIa improved the coagulation status significantly even with lower platelets (32,000 ⫻ 109/L) if prior fibrinogen substitution was performed. ROTEM and the Sonoclot analyzer are both viscoelastic POC coagulation analyzers. They measure the entire coagulation process starting with fibrin formation and continue through to clot retraction and lysis at the bedside with minimal time delays. Furthermore, physiologic clot development is depicted as a result of whole-blood analysis of the coagulation status. ROTEM measures the shear elasticity of the blood sample. The rotation of the pin begins to be impaired after fibrin-platelet bonding has linked the cup and pin together. The strength of these fibrin-platelet bonds affects the magnitude of the pin motion. Thus, the output is directly related to the strength of the formed clot. The Sonoclot analyzer, on the other hand, uses a different approach. A plastic probe is immersed and oscillates vertically in the sample. The output is sensitive to viscosity and monitors viscosity changes that occur during the initiation of coagulation and clot development. Viscoelastic POC analyzers have been used to evaluate the effects of hemostatic agents, such as rFVIIa.6-8 In theses studies, thromboelastography/thromboelastometry seems to be a promising method for the characterization of phenotypic variance among patients as well as in detection of the individual response to rFVIIa before and after rFVIIa administration. The presence of high amounts of tissue factor may directly activate the coagulation cascade (bypassing agent), and the effects of rFVIIa may no longer be monitored. Therefore, activation with
minute amounts of tissue factor has been recommended to visualize the particular signature in different coagulopathies and particularly to show the rFVIIa response.11 Recently, modified parameters of the thromboelastography/ thromboelastometry have been introduced based on the first derivative of the original tracing and have been shown to correlate closely with thrombin formation.11,23 These parameters, t-MaxVel, MaxVel, and total thrombus generation (AUC), are supposed to be more sensitive to rFVIIa treatment than standard thromboelastography/thromboelastometry parameters.26 However, these modified parameters did not better perform in monitoring rFVIIa administration in the present study compared with ROTEM’s conventional ␣-angle and MCF as well as Sonoclot’s CR. The interpretation of the data presented has to be within the limitations of an in vitro investigation with cautious extensions of the findings into clinical application only. In vitro coagulation studies may not necessarily reflect in vivo conditions because the effects of tissue damage, endothelial injury, and physiologic reactions to correct coagulation are missing in vitro. Furthermore, the study was performed with citrated blood samples of healthy male volunteers only. Additionally, the authors chose to study severe hemodilution with albumin 5% to have minimal effects on coagulation other than dilutional. It is likely that in vitro hemodilution with other colloids or crystalloids will show different results. Nevertheless, the present study provides some mechanistic insights into how rFVIIa is dependent on a sufficient concentration of fibrinogen and investigates for the first time the 2 POC coagulation analyzers ROTEM and Sonoclot in this indication. In summary, the administration of rFVIIa alone resulted in the present in vitro model of severe hemodilution in a shortened initiation phase of coagulation as detected by ROTEM and Sonoclot. Isolated fibrinogen administration to physiologic concentrations improved both the initiation of coagulation as well as clot formation and strength. Combined fibrinogen and rFVIIa administration further improved both effects significantly. These data suggest that fibrinogen is a key component in the coagulation process and that adequate levels of fibrinogen should be present before considering the administration of rFVIIa. However, further studies in vivo are required to confirm these findings.
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