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Plasma protein C levels in immunocompromised septic patients are significantly lower than immunocompetent septic patients: a prospective cohort study
Journal of Hematology & Oncology volume 2, Article number: 43 (2009)
Activated Protein C [APC] improves outcome in immunocompetent patients with severe sepsis particularly in those who are perceived to have high mortality risk. Before embarking on a trial of APC administration in immunocompromised septic patients, a preliminary study on plasma levels of protein C in this cohort is essential.
To assess serum Protein C concentrations in immunocompromised patients as compared to immunocompetent patients during sepsis, severe sepsis, septic shock and recovery.
Prospective cohort study in a tertiary hospital. Patients satisfying inclusion criteria were enrolled after informed consent. Clinical variables were noted with sample collection when patients met criteria for sepsis, severe sepsis, septic shock and recovery. Protein C levels were measured using monoclonal antibody based fluorescence immunoassay.
Thirty one patients participated in this study (22 immunocompromised, 9 immunocompetent). Protein C levels were found to be significantly lower in the immunocompromised group compared to the immunocompetent group, particularly observed in severe sepsis [2.27 (95% CI: 1.63-2.9) vs 4.19 (95% CI: 2.87-5.52) mcg/ml] (p = 0.01) and sepsis [2.59 (95% CI: 1.98-3.21) vs 3.64 (95% CI: 2.83-4.45) mcg/ml] (p = 0.03). SOFA scores were similar in both the groups across sepsis, severe sepsis and septic shock categories. Protein C levels improved significantly in recovery (p = 0.001) irrespective of immune status.
Protein C levels were significantly lower in immunocompromised patients when compared to immunocompetent patients in severe sepsis and sepsis categories. Our study suggests a plausible role for APC in severely septic immunocompromised patients which need further elucidation.
The role of Protein C pathway in regulating thrombosis, fibrinolysis and inflammatory cascade in a septic patient is well established. Both baseline serum protein C and early reduction in protein C concentrations have been found to be independent predictors of outcome in severe sepsis [1, 2]. This in combination with blunted generation of activated Protein C (APC) act in concert with reduced expression of thrombomodulin to contribute to a procoagulant state during sepsis [3, 4]. The resulting intravascular deposition of fibrin and microvascular thrombosis contributes to the organ dysfunction and mortality in sepsis . A phase III randomised controlled trial of activated protein C (APC) supplementation in severe sepsis (PROWESS), based on understanding of the pathophysiology, demonstrated a mortality benefit of APC therapy in severe sepsis that was statistically significant in the subgroup with protein C deficiency (p = 0.009) compared to those without protein C deficiency (p = 0.06) . These findings were supported by the ENHANCE trial , although not by the ADDRESS trial . Of note, in all these major trials, patients with immunocompromised states were excluded. One of the main reasons for exclusion of immunocompromised patients was their perceived high risk of bleeding. However, the advent of newer non-anticoagulant recombinant activated protein C molecule has allayed some concerns about the risk of bleeding which is a major drawback of APC as an effective anti-inflammatory drug [9, 10]. Anecdotal evidence suggests that there may be a potential benefit of adding APC to standard therapy in septic shock after hematopoietic stem cell transplantation . Preliminary data (Mesters et al) indicated that plasma protein C concentration diminished rapidly in the neutropenic patients who developed septic shock . Thus the question still remains unresolved whether APC may have a role in the management of neutropenic sepsis. More fundamentally, it is not clear whether protein C and APC concentrations are reduced in immunocompromised sepsis. This study was therefore designed to assess and compare protein C levels in immunocompromised patients to immunocompetent patients during sepsis, severe sepsis, septic shock and recovery.
Research design and the methods
This was a single centre prospective cohort study involving immunocompromised and immunocompetent patients in the haematology ward and the intensive care unit of Princess Alexandra Hospital, Brisbane. The study was approved by the Princess Alexandra Hospital human research ethics committee and informed consent was obtained either from patients or their next of kin. All patients admitted with a diagnosis of sepsis or those who developed sepsis during their admission were eligible. Three groups of patients were enrolled for the study: Immunocompetent patients with sepsis, immunocompromised patients with sepsis and immunocompromised patients without sepsis.
The diagnosis of SIRS, sepsis, severe sepsis and septic shock were based on standard criteria . Patients were identified as recovered for the purpose of study when they no longer satisfied the sepsis criteria for at least 48 hours.
Patients were classified as immunocompromised if they were diagnosed with neutropenia (absolute count < 0.5 × 109/L); myeloproliferative or lymphoproliferative condition; hyposplenism (based on history and imaging) or undergoing chemotherapy.
The exclusion criteria were:
Presence of hepatic failure (as protein C is secreted in hepatic cells)
History of spontaneous venous thrombosis and/or pulmonary embolism
Patients on Warfarin (Protein C is a vitamin K dependent protein)
Disseminated Intravascular Coagulation (DIC)
Patients already on activated protein C infusion
Failure to obtain consent
Patients were excluded from the study if they had DIC on basis of the modified overt diagnostic criteria of ISTH (International society of thrombosis and hemostasis) subcommittee on DIC.  In absence of any specific DIC criteria particularly for patients with hematopoietic malignancies and those on chemotherapy , we modified platelet count criteria for myelosuppressed patients to score 1 if reduction in platelet count by > 30% in last 24 hours not accompanied by similar fall in leucocyte count and score 2 if reduction in platelet count > 50% platelet in last 24 hours not accompanied by similar fall in leucocyte count.
The care of the patients was as per standard practice. No patient received APC infusion during the study.
Protein C test methodology
Blood for protein C assay was collected in citrated tubes, double centrifuged before separation of plasma which was then aliquoted; snap frozen, labelled and stored at -75°C for assay. Fluorescence Immunoassay (Triage Protein C Meter, Biosite†) was used for rapid, quantitative determination of protein C in thawed aliquoted samples. The mean protein C concentration in healthy men and women, when tested using the protein C meter, is reported to be 4.23 μg/ml (median- 4.70 μg/ml) . The coefficient of variation of the assay is reported to be 2-4% . To ensure the accuracy, the supplied quality control device was run prior to each run of patient's samples. The test performance was also monitored using external protein C controls. Five samples (7% of total samples) were randomly tested twice and their results confirmed the validity of this commercial assay.
Data collection and Blood sampling
The demographics, APACHE II  and SOFA scores  were collected on all patients. Post recruitment, patient's daily observation charts were closely followed up to assess if they satisfy criteria for sepsis, severe sepsis, septic shock or recovery. If patient's clinical condition fits in any of the abovementioned categories, then serum aliquots (for protein C assay) were prepared from their morning blood samples, if collected that day within last 6 hours, or else protein C test was requested to be done not later than by next morning. The blood samples were thus collected within 18 hours of clinical and biochemical observations that were noted for the purpose of calculating APACHE II score and SOFA score on all occasions. None of the patient had repeated sampling/measurements for any individual septic categories.
All statistical calculations were performed using the StatsDirect statistical software package. All continuous variables were analysed using basic descriptive statistics and univariate analysis was performed to obtain mean, standard deviation and/or confidence limits. The variables between two independent groups (e.g. immunocompromised and immunocompetent) were compared using unpaired t-test and the data was expressed as mean difference with 95% confidence interval (CI). A p < 0.05 was accepted as statistically significant. When the blood samples and other variables in the immunocompromised group obtained during different septic categories were compared against each other, one-way ANOVA for multiple comparison using Tukey-Kramer method (as unequal group sizes) was used.
Thirty eight patients were found to be eligible over a period of four months. Two patients were from non-English background and were excluded. Five patients refused consent. Thirty one patients participated in the study (22 Immunocompromised and 9 Immunocompetent).
Immunocompetent patients with sepsis (n = 9)
Immunocompromised patients with sepsis (n = 16)
Immunocompromised patients without sepsis (n = 6)
Table 1 shows the demographic data and the aetiologies of sepsis in all three groups. The groups were well matched in terms of age and the length of hospital stay. The causes for low immunity in the immunocompromised group were neutropenia (16/22), lymphoproliferative condition (4/22), hyposplenism (1/22) and minimally myelosuppressive chemotherapy (1/22). Five patients included in the neutropenia group were on myelosuppressive chemotherapy.
Breakdown of Septic episodes
Among the immunocompromised septic patients (n = 16), 7 patients developed sepsis, 11 patients developed severe sepsis and 2 progressed to develop septic shock. The corresponding figures for the immunocompetent septic group (n = 9 patients) were 8, 6 and 3 respectively. None of the patient was represented more than once in any of the individual septic category.
There were two deaths among study patients, one of which was in the immunocompromised severe sepsis category and other one was in the immunocompromised septic shock category.
Protein C concentration
Table 2 provides comparative data in the immunocompromised cohort measured during non-sepsis, sepsis, severe sepsis, septic shock and recovery. There was a statistically significant reduction in protein C concentrations in sepsis- 2.59 (95% CI: 1.98- 3.21) μg/ml [p = 0.03], severe sepsis- 2.27 (95% CI: 1.63- 2.9) μg/ml [p = 0.001] and septic shock - 1.23 μg/ml, when compared to values during recovery - 3.82 (95% CI: 3.23- 4.40) μg/ml. Moreover, there was no statistically significant difference between the protein C concentrations during recovery and non-sepsis - 3.96 (95% CI: 2.51- 5.41) μg/ml. Protein C levels, APACHE II scores and SOFA scores were similar across non-sepsis and recovery categories. Although, fibrinogen levels were elevated in sepsis, severe sepsis and septic shock, these did not reach statistical significance.
Comparison of immunocompromised sepsis vs immunocompetent sepsis
Serum protein C concentrations were found to be significantly lower in the immunocompromised group compared to the immunocompetent group, particularly observed in severe sepsis [2.27 (95% CI: 1.63-2.9) vs 4.19 (95% CI: 2.87-5.52) μg/ml] (p = 0.01) and sepsis [2.59 (95% CI: 1.98-3.21) vs 3.64 (95% CI: 2.83-4.45) μg/ml] (p = 0.03). The results are summarised in Table 3.
SOFA scores were similar in both the groups across sepsis, severe sepsis and septic shock categories. Of note, the statistically significant difference in APACHE II scores between the immunocompromised and the immunocompetent groups should be looked at in light of the fact that all immunocompromised patients gained 5 extra points on chronic health adjustment (on account of being immunosuppressed) while calculating APACHE II scores and thus it does not imply any significant difference in the level of sickness among the two groups.
The principal finding of this study was that the plasma protein C concentrations in the immunocompromised septic patients were lower than those seen in the immunocompetent septic patients and the protein C levels improved with recovery. To our knowledge, this study represents the first clinical trial investigating protein C levels in immunocompromised patients as compared to immunocompetent patients across different septic categories.
Mechanism of Protein C reduction in Sepsis
Protein C is an important component of the natural anticoagulant pathway. Under resting physiological conditions, protein C is continuously activated to maintain an anticoagulant milieu . Severe sepsis is known to cause generalized endothelial dysfunction resulting in a pro-coagulant state in the microvasculature [21, 22]. The activated coagulation cascade results in thrombin formation which then binds to thrombomodulin (TM). TM bound thrombin cause proteolysis of protein C and convert it to activated protein C (APC) which then down-regulates thrombin formation in negative feedback loop . This activation of protein C is augmented by 20 fold in the presence of endothelial protein C receptor (EPCR)  which is known to have increased plasma concentrations in septic patients . This interaction is a critical step in the host defence against sepsis since inhibition of protein C binding to EPCR (in baboon model) is shown to convert the response to sublethal concentrations of E.coli into a lethal response . Protein C is thus consumed during development of severe sepsis thereby contributing further to the development of microvascular thrombosis and disseminated intravascular coagulation. Moreover, the cytokine response in sepsis may also result in decreased expression levels of TM and EPCR on endothelium and thus decreased activation of protein C . These mechanisms may explain the reduction in plasma protein C concentrations in severe sepsis observed in our study.
However, our data indicates that plasma protein C levels are even lower in immunocompromised septic patients compared to the immunocompetent septic patients. There are various plausible mechanisms. A link between the protein C anticoagulant pathway and neutrophil functions is suggested by the observation that the soluble EPCR binds to activated neutrophils via Proteinase-3 and this binding is supported by β2 integrin involved in neutrophil signalling and cell-cell adhesion events . It is possible that these molecular interactions are significantly affected by haematological malignancies, neutropenia or endothelial dysfunction induced by cytotoxic drugs thereby further impairing the protein C system in our immunocompromised septic patients. Most of our patients in the immunocompromised cohort had received chemotherapy at some stage for their underlying haematological condition. Chemotherapy has been shown to induce endothelial dysfunction that was observed in young adult survivors treated for acute lymphoblastic leukaemia in childhood [29, 30] Malignancies and chemotherapy induced endothelial dysfunction might have predisposed our immunocompromised septic patients to have higher incidence of non-overt DIC resulting in increased consumption of protein C. It is also possible that protein C synthesis failed to keep up during the critical illness particularly when patients were on chemotherapy. Chemotherapy for breast cancer is known to decrease protein C concentrations . Doxorubicin has been shown to induce dose and time dependent decrease in cell surface EPCR levels and increase in cell surface thrombomodulin in human umbilical vein endothelial cells (HUVEC) with a net effect of impaired capacity of HUVECs to convert protein C to activated protein C . Since, activation of protein C system largely depends on TM and EPCR, it is important to study TM expression and EPCR expression in immunocompromised patients during non-sepsis state and in face of septic challenge in future studies. Other mechanisms that should be investigated are protein C consumption primarily due to DIC or reduced synthesis due to liver dysfunction. We excluded patients with overt DIC in this study and there were no significant differences between the two groups with respect to prothrombin time and bilirubin concentrations during any of the septic categories (Table 3).
Possible Clinical significance of these results
The significance of protein C arises from published literature on activated protein C. Whilst we did not measure APC in this study, it is well recognised that circulating levels of APC strongly correlate (r = 0.75, p < 0.0001) with levels of protein C antigen in both healthy men and individuals with protein C deficiency suggesting that the circulating protein C concentration is the limiting factor in the rate of activation of protein C . Therefore, protein C levels may reliably reflect APC levels in vivo.
This was a single centre study with small sample size. APC and other coagulation factors were not measured along with protein C. Moreover, the possible mechanisms of reduction in protein C such as soluble EPCR -neutrophils interaction in the immunocompromised patients, non-overt DIC scores and TM concentrations were not investigated and lastly, the relationship between protein C concentrations and outcome could not be examined owing to the small sample size.
This preliminary study reveals significantly lower protein C levels in the immunocompromised patients during sepsis and severe sepsis as compared to the immunocompetent patients. There was a significant improvement in protein C levels with recovery in both groups of patients. Further studies are required to confirm the findings of our study in a larger setting, and investigate relationship between protein C concentrations and outcome in immunocompromised septic patients. Our pilot study might provide the platform for a future clinical trial designed to study benefits of activated protein C therapy in the immunocompromised septic patients.
Plasma protein C concentrations in immunocompromised patients are lower than immunocompetent patients, particularly observed in sepsis and severe sepsis.
Protein C levels improved significantly with recovery irrespective of immune status.
The study suggests a plausible role for APC in severely septic immunocompromised patients which need further elucidation in a randomized controlled clinical trial.
Shorr AF, Bernard GR, Dhainaut JF, Russell JR, Macais WL, Nelson DR, Sundin DP: Protein C concentrations in severe sepsis: an early directional change in plasma levels predicts outcome. Crit Care. 2006, 10 (3): R 92-10.1186/cc4946. ISSN: 1466-609X
Fisher CJ, Yan SB: Protein C levels as a prognostic indicator of outcome in sepsis and related diseases. Crit Care Med. 2000, 28 (9 Suppl): S49-56. 10.1097/00003246-200009001-00011.
Liaw PC, Esmon CT, Kahnamoui K, Schmidt S, Kahnamoui S, Ferrell G, Beaudin S, Julian JA, Weitz JI, Crowther M, Loeb M, Cook D: Patients with severe sepsis vary markedly in their ability to generate activated Protein C. Blood. 2004, 104 (13): 3958-64. 10.1182/blood-2004-03-1203.
Conway EM, Rosenberg RD: Tumor necrosis factor suppresses transcription of the thrombomodulin gene in endothelial cells. Mol Cell Biol. 1988, 8 (12): 5588-92.
Fourrier F, Chopin C, Goudemand J, Hendrycx S, Caron C, Rime A, Marey A, Lestavel P: Septic shock, multiple organ failure, and disseminated intravascular coagulation. Compared patterns of antithrombin III, protein C and protein S deficiencies. Chest. 1992, 101 (3): 816-23. 10.1378/chest.101.3.816.
Bernard GR, Vincent JL, Laterre PF, LaRosa SP, Dhainaut JF, Lopez-Rodriguez A, Steingrub JS, Garber GE, Helterbrand JD, Ely EW, Fisher CJ, Recombinant Human Protein C Worldwide Evaluation in Severe Sepsis (PROWESS) study group: Efficacy and safety of recombinant human activated protein C for severe sepsis. N Engl J Med. 2001, 344 (10): 699-709. 10.1056/NEJM200103083441001.
Vincent JL, Bernard GR, Beale R, Doig C, Putensen C, Dhainaut JF, Artigas A, Fumagalli R, Macias W, Wright T, Wong K, Sundin DP, Turlo MA, Janes J: Drotrecogin alfa (activated) treatment in severe sepsis from the global open-label trial ENHANCE: further evidence for survival and safety and implications for early treatment. Crit Care Med. 2005, 33 (10): 2266-77. 10.1097/01.CCM.0000181729.46010.83.
Abraham E, Laterre PF, Garg R, Levy H, Talwar D, Trzaskoma BL, Francois B, Guy JS, Bruckmann M, Rea-Neto A, Rossaint R, Perrotin D, Sablotzki A, Arkins N, Utterback BG, Macias WL: Drotrecogin alfa (activated) for adults with severe sepsis and low risk of death. N Engl J Med. 2005, 353 (13): 1332-41. 10.1056/NEJMoa050935.
Weiler H, Ruf W: Activated protein C in sepsis: the promise of nonanticoagulant activated Protein C. Curr Opin Hematol. 2008, 15 (5): 487-93. 10.1097/MOH.0b013e32830abdf4.
Bae JS, Yang L, Manithody C, Rizaie AR: Engineering a disulfide bond to stabilize the calcium-binding loop of activated Protein C eliminates its anticoagulant but not its protective signaling properties. J Biol Chem. 2007, 282 (12): 9251-9. 10.1074/jbc.M610547200.
Pastores SM, Papadopoulos E, Brink van den M, Alicea M, Halpern NA: Septic shock and multiple organ failure after hematopoietic stem cell transplantation: treatment with recombinant human activated protein C. Bone Marrow Transplant. 2002, 30 (2): 131-4. 10.1038/sj.bmt.1703618.
Mesters RM, Helterbrand J, Utterback BG, Yan SB, Chao YB, Fernandez JA, Griffin JH, Hartman DL: Prognostic value of protein C concentrations in neutropenic patients at high risk of severe septic complications. Crit Care Med. 2000, 28 (7): 2209-16. 10.1097/00003246-200007000-00005.
Levy MM, Fink MP, Marshall JC, Abraham E, Angus D, Cook D, Cohen J, Opal SM, Vincent JL, Ramsay G: 2001 SCCM/ESICM/ACCP/ATS/SIS International Sepsis Definitions Conference. Crit Care Med. 2003, 31 (4): 1250-6. 10.1097/01.CCM.0000050454.01978.3B.
Taylor FB, Toh CH, Hoots WK, Wada H, Levi M: Towards definition, clinical and laboratory criteria, and a scoring system for disseminated intravascular coagulation. Thromb Haemost. 2001, 86: 1327-30.
Gando S, Iba T, Eguchi Y, Ohtomo Y, Okamoto K, Koseki K, Mayumi T, Murata A, Ikeda T, Ishikura H, Ueyama M, Ogura H, Kushimoto S, Saitoh D, Endo S, Shimazaki S, Japanese Association for Acute Medicine Disseminated Intravascular Coagulation (JAAM DIC) Study Group: A multicenter, prospective validation of disseminated intravascular coagulation diagnostic criteria for critically ill patients: Comparing current criteria. Crit Care Med. 2006, 34: 625-31.
Triage Protein C test Manual # 98500, © 2007 Biosite Incorporated.
Miletich JP, Broze GJ: Human plasma protein Z antigen: range in normal subjects and effect of warfarin therapy. Blood. 1987, 69 (6): 1580-6.
Knaus WA, Draper EA, Wagner DP, Zimmerman JE: APACHE II: a severity of disease classification system. Crit Care Med. 1985, 13 (10): 818-29. 10.1097/00003246-198510000-00009.
Vincent JL, Moreno R, Takala J, Willatts S, De Mendonca A, Bruining H, Reinhart CK, Suter PM, Thijs LG: The SOFA (Sepsis-related Organ Failure assessment) score to describe organ dysfunction/failure. On behalf of the working group on Sepsis-related Problems of the European Society of Intensive Care Medicine. Intensive Care Med. 1996, 22 (7): 707-10. 10.1007/BF01709751.
Dutt T, Toh CH: The Yin-Yang of thrombin and activated protein C. Br J Haematol. 2008, 140 (5): 505-15. 10.1111/j.1365-2141.2007.06977.x.
Aird WC: The role of the endothelium in severe sepsis and multiple organ dysfunction syndrome. Blood. 2003, 101 (10): 3765-77. 10.1182/blood-2002-06-1887.
Drake TA, Cheng J, Chang A, Taylor FB: Expression of tissue factor, thrombomodulin and E-selectin in baboons with lethal Escherichia coli sepsis. Am J Pathol. 1993, 142 (5): 1458-70.
Esmon CT: The Protein C pathway. Chest. 2003, 124 (3 Suppl): 26S-32S. 10.1378/chest.124.3_suppl.26S.
Fukudome K, Ye X, Tsuneyoshi N, Tokunaga O, Sugawara K, Mizokami H, Kimoto M: Activation mechanism of anticoagulant Protein C in large blood vessels involving the endothelial cell Protein C receptor. J Exp Med. 1998, 187 (7): 1029-35. 10.1084/jem.187.7.1029.
Kurosawa S, Stearns-Kurosawa DJ, Carson CW, D'Angelo A, Della Valle P, Esmon CT: Plasma levels of endothelial cell protein C receptor are elevated in patients with sepsis and systemic lupus erythematosus: lack of correlation with thrombomodulin suggests involvement of different pathologic processes. Blood. 1998, 91 (2): 725-7.
Taylor FB, Stearns-Kurosawa DJ, Kurosawa S, Ferrell G, Chang AC, Laszik Z, Kosanke S, Peer G, Esmon CT: The endothelial cell protein C receptor aids in host defense against Escherichia coli sepsis. Blood. 2000, 95 (5): 1680-6.
Dahlback B, Villoutreix BO: Regulation of blood coagulation by the protein C anticoagulant pathway: novel insights into structure-function relationships and molecular recognition. Arterioscler Thromb Vasc Biol. 2005, 25 (7): 1311-20. 10.1161/01.ATV.0000168421.13467.82.
Kurosawa S, Esmon CT, Stearns-Kurosawa DJ: The soluble Endothelial Protein C receptor binds to activated neutrophils: involvement of Proteinase-3 and CD 11b/18. J Immunol. 2000, 165 (8): 4697-703.
Chow AY, Chin C, Dahl G, Rosenthal DN: Anthracyclines cause endothelial injury in pediatric cancer patients: a pilot study. J Clin Oncol. 2006, 24 (6): 925-8. 10.1200/JCO.2005.03.5956.
Dengel DR, Ness KK, Glasser SP, Williamson EB, Baker KS, Gurney JG: Endothelial function in young adult survivors of childhood acute lymphoblastic leukemia. J Paediatr Hematol Oncol. 2008, 30 (1): 20-5. 10.1097/MPH.0b013e318159a593.
Rogers JS, Murgo AJ, Fontana JA, Raich PC: Chemotherapy for breast cancer decreases plasma Protein C and Protein S. J Clin Oncol. 1988, 6 (2): 276-81.
Woodley-Cook J, Shin LY, Swystun L, Caruso S, Beaudin S, Liaw PC: Effects of the chemotherapeutic agent doxorubicin on the Protein C anticoagulant pathway. Mol Cancer Ther. 2006, 5 (12): 3303-11. 10.1158/1535-7163.MCT-06-0154.
España F, Zuazu I, Vicente V, Estelles A, Marco P, Aznar J: Quantification of Circulating Activated Protein C in human plasma by immunoassays- Enzyme levels are proportional to total Protein C levels. Thromb Hemost. 1996, 75 (1): 56-61.
The funding for this study was awarded by ANZCA research grant committee.
† Triage Protein C Meter and the test kits were kindly provided by Biosite on our request.
The authors declare that they have no competing interests.
RP, BV and PK were responsible for study design and data management. RP recruited patients, carried out Protein C assays and recorded all clinical data. RP and BV did statistical analysis and drafted the manuscript. BV, PK, RB, LN and DG were responsible for patient management. GD was responsible for managing protein C meter, preparing and preserving aliquots. RP, BV and PK did the data interpretation. BV, PK, RB and LN participated together with RP in editing the manuscript. All authors read and approved the final manuscript.
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Panwar, R., Venkatesh, B., Kruger, P. et al. Plasma protein C levels in immunocompromised septic patients are significantly lower than immunocompetent septic patients: a prospective cohort study. J Hematol Oncol 2, 43 (2009) doi:10.1186/1756-8722-2-43
- Severe Sepsis
- Disseminate Intravascular Coagulation
- Immunocompetent Patient
- Sofa Score
- Overt Disseminate Intravascular Coagulation