Can presepsin uniformly respond to various pathogens? - an in vitro assay of new sepsis marker -

Presepsin (soluble CD14 subtype) is a novel biomarker of sepsis [1]. The plasma presepsin level rises as early as within 2 h of inflammation onset, which is even earlier than C-reactive protein (CRP), procalcitonin, or interleukin-6 (IL-6) [2‐4]. With a high specificity for bacterial infections, presepsin has proved useful in early diagnosis and is a prognostic marker of severe sepsis [3‐8]. In recent years, the clinical importance of this molecule has been intensively discussed in various categories of infection such as surgery [9], burn [10], neonatal sepsis [11], and febrile neutropenia [12, 13]. Moreover, recent meta-analyses showed its efficacy in the diagnosis of sepsis [14, 15].

CD14 is the receptor for lipopolysaccharide (LPS) / LPS – binding protein (LPS/LBP) complexes [16] and is released in the early phase of infection. As LPS represents a characteristic attribute of gram-negative bacteria, the diagnostic value of this molecule for gram-positive bacteria, which contain less LPS, is uncertain.

In this study, we conducted a simple in vitro assay to evaluate presepsin levels in response to various gram-negative and gram-positive bacterial strains. Although other factors might influence the presepsin altitude in real septic patient’s environment, we tried to clarify the interspecies differences in response to various pathogens with this in vitro assay.

Figure 1 shows the comparison of presepsin levels between the gram-positive and gram-negative bacteria. The presepsin level in the gram-negative bacteria 273 (median, IQR = 218–352) pg/mL was significantly higher than in the gram-positive bacteria 200 (143–275) pg/mL (p = 0.0002, Wilcoxon rank sum test). The presepsin values in control group was 84.3 (73.9–103) pg/mL.

Figure 2 shows the comparison of the presepsin released in the assay of each species. The strains were sorted in the descending order of median values of the amount of presepsin released. The median (IQR) of the presepsin levels in gram-negative bacteria were Enterobacter cloacae 330 (246–462) pg/mL, Klebsiella. pneumoniae 301 (229–378) pg/mL, Stenotrophomonas maltophilia 284.5 (202.25–396) pg/mL, Escherichia coli 251.5 (175–289.25) pg/mL, and Pseudomonas aeruginosa 197 (169–274) pg/mL.

The presepsin levels in the gram-positive bacteria were Staphylococcus aureus 282 (225–452) pg/mL, Bacillus cereus 197 (140–324) pg/mL, Streptococcus pyogenes 171 (150–213) pg/mL, and Corynebacterium striatum 136 (119–193) pg/mL.

The Steel-Dwass test revealed that the presepsin levels were significantly lower in C. striatum, in comparison to E. cloacae (p = 0.0003), K. pneumoniae (p = 0.0005), S. aureus (p = 0.0005), S. maltophilia (p = 0.018), and E. coli (p = 0.047), respectively.

The presepsin levels were also significantly lower in S. pyogenes in comparison to E. cloacae (p = 0.0003), K. pneumoniae (p = 0.0006), and S. aureus (p = 0.0007), respectively.

The presepsin levels in P. aeruginosa were significantly lower compared to E. cloacae (p = 0.013).

Presepsin is a subtype of the N-terminal fragment of soluble CD14 with a molecular weight of 13 kDa. CD14 is known as the pattern recognition receptor (PRR) for the LPS-LBP complexes expressed on the cell membrane of the phagocytes. During phagocytosis, the CD14 molecule is internalized with the bacteria and cleaved into presepsin after phagolysosomal processing, and released into the plasma [1, 4, 5, 17].

Previous studies had focused on the clinical aspects of this molecule, such as sensitivity, specificity or positive predictive value in the diagnosis of infectious diseases. For example, higher presepsin level is indicative of severe sepsis and is also associated with poor prognosis [3‐8, 14, 15]. In those studies, the species of the bacteria causing sepsis were not considered in detail.

Because presepsin derives from CD14, one of the major PRRs, the degree of its response is presumed to reflect the surface structure of the confronting pathogen. Since LPS is specific for gram-negative bacteria, we attempted to evaluate the response of this molecule towards gram-positive bacteria. This is important because the existence of an interspecies difference might affect the reliability of presepsin as an early marker of infectious diseases.

Thus, we designed an in vitro assay to evaluate the presepsin levels in response to various strains including five gram-negative and four gram-positive bacteria. The assay system mimics the situation in bacteremia, reflecting the immediate phagocyte-bacterial interaction with the help of other circulating blood cells, plasma proteins or the complement system. Generally, the host-microbe interaction is difficult to evaluate because there are cascades of complex intervening inflammatory responses. However, unlike other assays, our system involves minimal requirements of host-microbe immunity. Therefore, evaluations in a direct and in a real time manner can be achieved.

Our results suggested that presepsin production can be also evoked by gram-positive bacteria. However, presepsin levels in response to the gram-positive bacteria were lower than those of gram-negative bacteria, as expected because LPS is a characteristic attribute of gram-negative bacteria. This trend was prominent in C. striatum and S. pyogenes. But some gram-positive organisms like S. aureus evoked relatively high levels of presepsin and gram-negative bacteria like P. aeruginosa evoked lower levels. This could probably be due to the difference in the immunogenicity or phagocytosis evocativenesss (sensitivity) among the species. The association of CD14 ligands, other than LPS, might influence its production. Or, the low presepsin level in response to S. pyogenes might be partly explained by phagocytosis escaping mechanisms [18]. Further analyses of the membrane structures or other factors affecting the levels of presepsin release should be carried out to elucidate the reasons for such a response.

This study has a few limitations. First, the host immune profile was not analyzed in detail, except that the number of neutrophils and the baseline presepsin levels were confirmed to be equivalent. We cannot exclude the influence of other immunological factors, such as lymphocyte subsets, complement, or cytokines. Second, we only used clinical isolates. We selected typical non-neutropenic bacteremia cases as a source of the bacterial strains. The cases showed bacteremia in the absence of neutropenia, immunosuppressants, and mechanical obstructions, which indicated that they are virulent enough to cause bacteremia in the general population. We intended to reproduce bacteremia in vitro with real world strains; however, whether they can be considered representative strains is debatable. All the species were correctly identified by biochemical analysis and confirmed by MALDI-TOF-MS. Moreover, to avoid potential strain bias, we integrated the data of 3 strains for one species. Third, the presepsin levels observed in this study cannot be applied in clinical settings. The values discussed here are a relative comparison among the species and do not reflect the cut-off values of either sepsis or the septic shock diagnostic criteria.

Taking the strengths and limitations of this study into consideration, our result is still meaningful because our assay mimics the clinical situation of bacteremia in which bacteria encounters immune cells in the blood, and we can directly evaluate the total immune response. Our experiment also warrants the need to consider the interspecies difference when presepsin is used as a diagnostic tool in sepsis.

In conclusion, using a simple in vitro presepsin releasing assay, we found that presepsin production can also be evoked by gram-positive bacteria, though the levels were significantly lower in comparison to the gram-negative bacteria. We also found interspecies differences in the presepsin response levels, which might be important in the diagnosis of infectious diseases caused by certain gram-positive bacteria, such as S. pyogenes or C. striatum. To our knowledge, this is the first report using an in vitro presepsin assay, and focusing on the difference of its responsiveness as a PRR against various bacterial species. Our experiment warrants the need to consider the interspecies difference when presepsin is used as a diagnostic tool in sepsis caused by certain gram-positive bacteria, such as S. pyogenes or C. striatum.

The system is a co-culture assay using whole blood and the bacterial strains obtained from blood culture.