Scavengers of hemoproteins as potential biomarkers for severe sepsis and septic shock

Background

Despite improvements in diagnosis, interventions and supportive care, mortality among sepsis patients is still high. Research of the past decade has attempted to identify biomarkers that can accurately discriminate sepsis from other diseases with comparable symptoms to improve diagnosis, but results have been lackluster. Recent studies have shown that hemoproteins and damage-associated molecular patterns (DAMPs) such as mitochondrial DNA (mtDNA) released as the result of hemolysis play an important role in the pathogenesis of sepsis. The aim of this study was to measure plasma levels of the indirect markers for hemoproteins hemopexin, haptoglobin and heme oxygenase-1 (HO-1) as well as the mitochondrial damage marker mtDNA in the plasma of a cohort of sepsis patients to determine the feasibility of their use as biomarkers in the diagnosis of sepsis.

Methods

Hemopexin, haptoglobin and HO-1 were measured in plasma by ELISA and mtDNA was measured by digital droplet PCR. Plasma levels of hemopexin, haptoglobin, HO-1 and mtDNA were measured in 32 patients with severe sepsis and 8 patients with septic shock at baseline and 4 days after admission to the ICU and in 20 healthy donors.

Results

Plasma levels of hemopexin were significantly lower and plasma levels of HO-1, haptoglobin and mtDNA were significantly higher in patients with severe sepsis and septic shock at baseline compared to healthy controls. Additionally, HO-1 levels were significantly higher in patients with septic shock compared to patients with severe sepsis. Finally, levels of HO-1 and mtDNA, but not of hemopexin, seemed to slowly revert back towards levels measured in healthy donors within 5 days after admission.

Conclusions

Our results indicate that plasma levels of the hemoprotein scavengers hemopexin, haptoglobin and HO-1 and the mitochondrial damage marker mtDNA might be useful as additional biomarkers for the early diagnosis of sepsis and disease severity.

Severe sepsis is a result of an uncontrolled immune response of the host to infection. In the area of timely diagnosis, rapid interventions and intensive supportive care, mortality rates for severe sepsis still reach 20 %.[1,2,3] Even in the first year after hospital discharge, mortality among sepsis survivors is high and the long-term quality of life of these patients is impaired.[4] Studies have shown that an early diagnosis and intervention in patients with severe sepsis increases survival rates.[5, 6] However, symptoms are often variable and non-specific, making early diagnosis of sepsis a major challenge.[7] Therefore, there is an absolute need to identify biomarkers that can discriminate the presence of sepsis from other diseases and predict severity at early stages of this process.[7].

Sepsis is characterized by extensive cell death of hematopoietic as well as parenchymal cells, as evidenced by the systemic release of damage-associated molecular patterns (DAMPs) such as cell-free DNA.[8,9,10] Cell death is accompanied by disintegration of mitochondrial membranes with subsequent release of DAMPs in the form of hemoproteins containing heme and iron from the respiratory chain.[11] Changes in red blood cell (RBC) energy metabolism to maintain redox balance, alteration of RBC membrane properties, complement activation, pathogens invading RBCs and endothelial cell activation with subsequent microvascular RBC destruction result in hemolysis and subsequent systemic release of cell-free hemoglobin, cell-free heme and iron during sepsis. Finally, death of skeletal muscle cells accompanying sepsis results in the systemic release of myoglobin containing heme and iron.[11, 12] Endogenous plasma- and cellular systems protect the organism from the negative effects of hemoproteins and iron.[11] Cell-free hemoglobin and cell-free heme are scavenged by the plasma proteins haptoglobin and hemopexin, respectively. Heme oxygenase-1 (HO-1), an enzyme that is inducible by free heme and iron, catalyzes the degradation of heme into iron, biliverdin and CO intracellularly.[11] Subsequently, iron is neutralized by ferritin, the upregulation of which is coupled to the induction of HO-1. Previous studies have highlighted the important role of free heme in the pathogenesis of sepsis[2], and have linked plasma levels of haptoglobin and hemopexin to severity and outcome of disease.[13, 14] Moreover, increased HO-1 mRNA expression and protein levels have been shown to exert protection in experimental animal models for sepsis.[15, 16] Finally, mitochondrial DNA (mtDNA) released from mitochondria upon cell death has been shown to elicit immune responses through activation of TLR9 and the NLRP3 inflammasome.[17] In line with this, several studies and clinical trials (reviewed in Harrington et al., (2017)) have found mtDNA levels to be elevated in patients with sepsis, pointing to a probably role of mtDNA in sepsis pathogenesis.[18] As such, we questioned whether indirect markers for hemoproteins such as their respective scavengers and mitochondrial damage markers such as mtDNA might be useful as biomarkers for the diagnosis of severe sepsis in clinical practice.

In this study, we measured plasma levels of haptoglobin, hemopexin, HO-1 and mtDNA in patients with severe sepsis and septic shock and healthy donors to identify potentially novel biomarkers for severe sepsis and septic shock.

Patients

This study was approved by the medical ethical committees of the involved institutions, and all patients and healthy volunteers or their legal representatives gave written informed consent before inclusion. Sepsis patients were initially recruited as part of a randomized, double-blind placebo controlled trial aiming to investigate the efficacy and safety of C1-Inhibitor administration for the treatment of severe sepsis and septic shock.[19] Whole blood and plasma samples were taken from these patients at admission (t = 0), and daily thereafter for 4 consecutive days (5 time-points in total).[19] Plasma samples from 20 healthy Dutch volunteers were also obtained. Plasma samples were stored at -80ºC until further analysis. For analyses of baseline (t = 0) measurements, all patient samples were included. For the measurements over time, only samples of patients treated with placebo and not C1-inhibitor were included in the analysis.

Laboratory analyses

Digital droplet PCR

DNA was isolated from plasma using the QIAamp DSP virus kit (Qiagen), following the protocol included in the kit. For vacuum steps, instead of using vacuum technology, an Eppendorf centrifuge was used to spin down samples. 200 µl plasma was used for isolation, and reagent volumes for isolation were adjusted accordingly. DNA samples were thawed and diluted 1 in 5 in DNase-free water. A ddPCR reaction mixture for the appropriate number of samples, a control DNA sample with known quantity (isolated from MNCs and diluted 1 in 10 in DNase-free water) and a no-template control (NTC) was prepared with 11 µl 2x ddPCR Mastermix (no dUTP) (Biorad), 1 µl 20x ddPCR™ Copy Number Assay: ND1, Human (FAM) (Biorad, unique assay ID dHsaCNS669425578) and 9 µl DNase-free water per sample. For each DNA sample, 2 µl of pre-diluted DNA was added to 42 µl of ddPCR reaction mix. Droplets were generated with a QX200 droplet generator (Biorad), following the accessory instruction manual. 40 µl of droplets from the top wells of the cartridge were transferred to a 96-well TwinTec PCR plate (semi-skirted, green, Eppendorf). After sealing the plate, the PCR was carried out in a T100 thermal cycler (Biorad), with the heated lid set to 105 ºC and a sample volume of 40 µl. One cycle of enzyme activation was performed (95 ºC for 10 min), followed by 40 cycles of amplification (95 ºC for 30 s, 60 ºC for 1 min) and finally one cycle of enzyme deactivation (98 ºC for 10 min). A ramp rate of 2 ºC/second was maintained for all steps. After PCR was complete, the PCR plate was placed in a QX200 droplet reader (Biorad) for counting of the droplets. Results were analyzed using Quantasoft software (Biorad), and absolute values of mtDNA (ND1) (copies/µl) were calculated for each DNA sample by correcting for the corresponding dilution values.

ELISA

Heme oxygenase-1, haptoglobin and hemopexin were measured in plasma by ELISA. HO-1 was measured using a commercially available human heme oxygenase-1 matched antibody pair kit (Abcam, ab215401). Haptoglobin was measured using a commercially available human haptoglobin DuoSet ELISA (R&D Systems, DY8465-05). Hemopexin was measured using in-house capture and (biotinylated) detection antibodies. All coating steps were performed in PBS, samples and standard curves were measured diluted in high performance ELISA-buffer (HPE) and biotinylated detection antibodies were diluted in HPE. Poly-HRP diluted 1:10.000 was used for detection.

Statistical analyses

Results are expressed as mean ± SD or median with interquartile range. Statistical analyses were carried out using Graphpad Prism 8 software. Differences between groups were analyzed using the nonparametric, two-tailed Mann-Whitney U test for unpaired samples and the nonparametric Wilcoxon matched-pairs signed rank test was used for paired samples. A p-value at or below 0.05 was considered statistically significant.

Measurement of plasma levels of hemoprotein scavengers and mitochondrial damage markers

We measured levels of indirect markers for hemoproteins such as hemopexin, haptoglobin and HO-1 and mtDNA in the plasma of 40 patients with a median age of 64 yrs (range 28–75 yrs) with sepsis (32 severe sepsis and 8 septic shock patients) and in the plasma of 20 healthy controls. Plasma levels of hemopexin were significantly lower in the patients with severe sepsis and septic shock at t = 0 compared to the healthy controls (P < 0.0001). This indicates that hemopexin is consumed upon complexation with cell-free heme, which is released from hemoproteins into the plasma in patients suffering from sepsis (Fig. 1 a). In contrast, plasma levels of HO-1, haptoglobin and mtDNA were significantly higher in the patients with severe sepsis and septic shock at t = 0 compared to the healthy controls (P < 0.0001 and P = 0.0025, respectively) (Fig. 1 a). HO-1 is an intracellular enzyme that is upregulated upon stress, and is normally not secreted. Mitochondrial DNA can be released from mitochondria and cells in case of cellular stress and from cells undergoing apoptosis or necrosis.[20].

Hemoprotein scavengers and mitochondrial damage markers in sepsis patients at baseline and healthy donors. a Plasma levels of hemopexin, HO-1, haptoglobin and mitochondrial DNA are shown in healthy donors (n = 20) and in sepsis patients at baseline (n = 40). b Baseline (t = 0) plasma levels of hemopexin, HO-1, haptoglobin and mitochondrial DNA are shown in patients with severe sepsis (n = 32) and patients with septic shock (n = 8). Data are presented as median ± interquartile range. Groups have been compared using Mann-Whitney Rank Sum Test; P < 0.05 was considered significant. **P < 0.01, ****P < 0.0001

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Plasma levels of HO-1 were significantly higher in patients with septic shock (n = 8) compared to patients with severe sepsis (n = 32) at t = 0 (P = 0.0054). No difference in plasma levels of hemopexin, haptoglobin and mtDNA was observed when comparing patients with severe sepsis and septic shock (Fig. 1b). Overall, our data suggest that plasma levels of hemopexin, HO-1, haptoglobin and mtDNA are altered in sepsis, and as such might be useful as biomarkers for the diagnosis of the disease.

Of the 40 patients included in our study, 20 patients were not subjected to an intervention treatment in the context of the study and only received conventional standard supportive care for sepsis (which consisted of antibiotics, intravenous fluid substitutions and vasopressor therapy).[19] To determine whether plasma levels of hemopexin, HO-1, haptoglobin and mtDNA changed over time with standard care, we also measured these plasma levels in patients at day 4 after diagnosis. Both HO-1 and mtDNA were significantly lower at day 4 compared to baseline (P = 0.0071 and P = 0.0016, respectively), whereas hemopexin and haptoglobin levels did not change significantly in the first 4 days after diagnosis (Fig. 2). Only a small number of septic shock patients could be included in this analysis, and no clear differences were seen when comparing patients with severe sepsis and with septic shock.

Hemoprotein scavengers and mitochondrial damage markers in sepsis patients over time. Plasma levels of hemopexin, HO-1, haptoglobin and mitochondrial DNA are shown in severe sepsis patients (black) and septic shock patients (red) at baseline (t = 0) (n = 19, n = 18 for haptoglobin and mtDNA) and at day 4 after admission (t = 4) (n = 19, n = 18 for haptoglobin and mtDNA). Groups have been compared using Wilcoxon Rank Sum test. P < 0.05 was considered significant. **P < 0.01

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In this study, we assessed the applicability of the scavengers of hemoproteins hemopexin, haptoglobin and HO-1 and the mitochondrial damage marker mtDNA as biomarkers for the diagnosis of sepsis.

In a cohort of 40 patients suffering from severe sepsis or septic shock, we found plasma levels of hemopexin to be significantly decreased while plasma levels of HO-1, haptoglobin and mtDNA were significantly increased. The decreased levels of hemopexin are in line with research from other groups, which showed that low concentrations of hemopexin in serum are associated with a worse outcome in patients with septic shock[2] and which found plasma levels of hemopexin to be significantly higher in survivors of sepsis compared to non-survivors.[13] Upon complexation with heme, hemopexin-heme complexes are endocytosed by macrophages and hepatocytes after binding to CD91, the primary receptor for hemopexin-heme complexes.[21] This mechanism is likely causing the decrease of hemopexin seen in our patient samples. Interestingly, we found haptoglobin levels to be significantly higher in sepsis patients compared to healthy donors, in stark contrast with hemopexin. This may be due to a difference in dynamics of the two proteins, with the early induction of haptoglobin possibly being much faster and stronger than the induction of hemopexin. These data suggest that hemopexin, HO-1, haptoglobin and mtDNA could be potential biomarkers to be used in the diagnosis of sepsis. To further determine whether these markers can distinguish sepsis from other diseases, plasma levels of these markers should be compared with other conditions that fit the criteria used to diagnose sepsis, such as acute pancreatitis or trauma.[22].

We further show that, although our sample sizes are limited, patients with septic shock seem to have higher plasma levels of HO-1 and mtDNA, and lower levels of hemopexin compared to patients with severe sepsis. Finally, we found that plasma levels of HO-1 and mtDNA, on average, decrease again after several days of standard care treatment. Our data suggest that treatment may influence these markers and indicate that these markers may also provide extra information on the severity of the disease.

In conclusion, we have shown that plasma levels of hemopexin, HO-1, haptoglobin and mtDNA are altered in patients with severe sepsis and septic shock and that they could potentially be valuable biomarkers to be used in the diagnosis of sepsis. However, further research using larger sample groups allowing for the determination of both sensitivity and specificity of these markers is needed to confirm this.

Data in the current study is available from the corresponding author upon reasonable request.

DAMP:

Damage-associated molecular pattern

mtDNA:

mitochondrial DNA

HO-1:

heme oxygenase-1

Not applicable.

This work was financially supported by the Landsteiner Foundation for Blood Transfusion Research, grant F1719 (M.V., I.B., C.V. and S.Z.).

Authors and Affiliations

1. Department of Hematopoiesis, Sanquin Research and Landsteiner Laboratory, Amsterdam, The Netherlands

   Myrddin W. Verheij & Carlijn Voermans

2. Department of Immunopathology, Sanquin Research and Landsteiner Laboratory, Amsterdam, The Netherlands

   Ingrid Bulder & Sacha S. Zeerleder

3. Department of Hematology and Central Hematology, Department of Internal Medicine, Kantonsspital Lucerne, Lucerne and University of Bern, Bern, Switzerland

   Walter A. Wuillemin

4. Department of Hematology and Central Hematology Laboratory, Inselspital, Bern and Bern University Hospital, University of Bern, Bern, Switzerland

   Sacha S. Zeerleder

5. Department of Biomedical Research, University of Bern, Bern, Switzerland

   Sacha S. Zeerleder

Contributions

All authors contributed to study conception and design. MWV and IB collected the data and performed the experiments. MWV performed data analysis and statistics. MWV wrote the first draft of the manuscript. The manuscript was critically reviewed and edited by SSZ and CV and all authors read and approved the final version.

Corresponding author

Correspondence to Sacha S. Zeerleder.

Ethics approval and consent to participate

This study was approved by the medical ethical committees of the involved institutions, and all patients and healthy volunteers or their legal representatives gave written informed consent before inclusion.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no competing interests.

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