Development of a prediction model for bacteremia in hospitalized adults with cellulitis to aid in the efficient use of blood cultures: a retrospective cohort study

Cellulitis is a common infectious disease which accounted for 10.1 % of infectious disease–related hospitalizations in US from 1998 to 2006 [1]. The infection can cause significant local tissue damage, and can spread systemically via the lymphatic system and bloodstream. The most common pathogens isolated from patients with non-purulent and purulent cellulitis are β-hemolytic streptococci and Staphylococcus aureus, respectively [2].

Guidelines for treating specific infectious diseases often emphasize the need to determine the microbial etiology of the invading pathogen(s) to plan the most effective antimicrobial therapy. However, in cases of cellulitis, diagnosis and management largely depend on the morphological features of the lesion and the clinical setting; the causal pathogen is less important [3]. The role of blood culture in the management of cellulitis remains especially controversial. This relates to the fact that the incidence of bacteremia in cellulitis is relatively low (2.0–18.5 %) [2, 4‐9], and contamination rates are relatively high (3.6–4.1 %), which devalues the clinical significance of blood culture [4, 8]. Additionally, several studies suggest that blood culture is not cost-effective as a routine test, and has only a marginal effect on treatment efficacy [4, 8, 10, 11]. As a result, the 2014 Infectious Diseases Society of America (IDSA) guidelines for the management of skin and soft tissue infections state that blood cultures are recommended only for patients with deleterious conditions, such as malignancy, sepsis, immersion injury, animal bites, neutropenia, and severe cell-mediated immunodeficiency [3]. However, evidence to support these recommendations is limited.

Although there are many reported risk factors for bacteremia in cellulitis cases, including age >45 years, length of illness <2 days, temperature >38.5 °C on admission, a white blood cell count (WBC) >13,300/mm³ on admission, lymphedema, liver cirrhosis, and chronic kidney disease [4, 6, 9], they have not been subjected to multivariable analysis to more accurately identify cellulitis patients at risk of bacteremia, or risk stratification to quantify the probability of bacteremia in cellulitis patients. Therefore, when confronted with cellulitis, clinicians are often unable to discriminate which patients will benefit from blood culture examination immediately upon admission. This lack of quantified risk stratification and clear evidence-based guidance for cellulitis patients means that the majority of clinicians routinely order blood culture, even when there is a low risk of bacteremia [2, 4, 9]. This can be a waste of both time and medical resources, which is an increasingly important issue in the era of rising healthcare costs [12]. To identify the cellulitis patients who might benefit most from blood cultures, clinicians need an informative diagnostic scoring system to quantify a patient’s risk of bacteremia. With such a tool, the number of routine blood cultures performed in low risk groups might be significantly reduced. However, to the best of our knowledge, such a diagnostic prediction model to estimate the probability of true bacteremia in cellulitis has not yet been developed.

The aim of this study was to develop a diagnostic scoring system, referred to as the Bacteremia Score of Cellulitis, based on demographic data and clinical manifestations, to better predict cases of bacteremia in hospitalized adults. This system will provide a more evidence-based approach to order blood cultures, and could be implemented as part of clinical practice guidance for cellulitis.

The participant flow diagram is outlined in Fig. 1. During the 1-year study period, 968 patients matching the ICD-9-CM criteria were hospitalized. Of these, 617 (63.7 %) were excluded following chart review. Of the 351 patients enrolled in this study, 33 (9.4 %) were positive blood culture group. There were a total of 691 blood samples (on average two cultures/patient). Contaminants, as defined in Methods, were isolated from a further 17 patients (4.8 %).

This analysis was used to develop an initial diagnostic prediction model that might help primary physicians in the decision-making process surrounding initial diagnosis of bacteremia in cases of cellulitis. Although the rounded score performed well in predicting bacteremia in our study population (AUC = 0.865; 95 % CI, 0.804–0.926), it still needs further validation with independent samples before it can be used in clinical care.

Our findings showed that the weighted combination of four independent predictors (age ≥65 years, involvement of non-lower extremities, liver cirrhosis, and SIRS) can help discriminate between patients with and without true bacteremia in hospitalized adults with cellulitis. This Bacteremia Score of Cellulitis employs clinical and demographic variables to stratify cellulitis patients, and thereby identify those at higher risk of true bacteremia. The medium and high risk groups were more likely to benefit from blood culture than the overall population in this study (14.7 % and 41.2 % vs. 9.4 %, respectively). Conversely, the study patients who had a rounded Bacteremia Score of Cellulitis of ≤1.5 were at much lower risk of true bacteremia than the overall population (1.0 % vs. 9.4 %) (Fig. 4). The Bacteremia Score of Cellulitis will thus be useful for stratifying hospitalized adults with cellulitis according to their bacteremia risk, which in turn will help clinicians optimize decision making on when to order blood cultures on admission.

However, without more cost-effective decision analyses, the choice of a so-called rational cut-off value to determine whether to order a blood culture seems somewhat arbitrary. When we used a cut-off value of 2.0, the majority (57.5 %) of patients were stratified into the low risk group. With a high negative predictive value (99.0 % in the present study), a cut-off value of 2 is a good negative screening threshold, thereby reducing the number of routine blood cultures in low risk groups. This could lead to a substantial reduction in the costs associated with blood cultures. However, the use of a cut-off value means that some patients with true bacteremia will not be identified. In the current study, two cases of true bacteremia in the low risk group would not be identified if a cut-off value of 2 was used. In one 54-year-old man without co-morbidities, the antimicrobial treatment was de-escalated from vancomycin to penicillin based on isolation of group B Streptococcus from blood culture. In the other, a 50-year-old man with history of allograft stem cell transplantation for acute myeloid leukemia, the antimicrobial treatment was switched from oxacillin to piperacillin according to isolation of Morganella morganii. The role of immunocompromised status (i.e., patients receiving immunosuppressive agents or chemotherapy, those with hematological malignancy, or those infected with human immunodeficiency virus) in this prediction model remains unknown because of the small number of immunocompromised patients in our study. However, even without further evidence, it is reasonable to assume that blood cultures would be beneficial for cellulitis patients with deleterious conditions such as malignancy, neutropenia, and severe cell-mediated immunodeficiency [3], even in cases with a rounded Bacteremia Score of Cellulitis ≤1.5.

The present study showed that cirrhosis was a predictor for true bacteremia in cellulitis cases. This may reflect the multiple immune system defects associated with cirrhosis, including reduced polymorphonuclear leukocyte activity, reduced Kupffer cell numbers, and increased bacterial translocation from the gut resulting from altered intestinal immunity and bacterial overgrowth [18]. This immune dysfunction may promote bacteremia caused by GNB, leading to hematogenous seeding to the skin and soft tissue at distant sites [18].

The present study identified involvement of non-lower extremities as an independent predictor of bacteremia in cellulitis, which has not been reported previously. In most cases, cellulitis is caused by a microbial breach of the cutaneous layer, particularly in patients with predisposing conditions [3]. Such infections are most common in the lower limbs [3]. For cellulitis localized outside the bilateral lower limbs, we hypothesize that the condition may be caused by hematogenous seeding of bacteria into the skin and soft tissue from a more distant site, rather than a local microbial breach. This may explain why the involvement of non-lower extremities is a predictor for bacteremia in cellulitis.

Consistent with previous studies [7], we found that β-hemolytic streptococci were the most common bacteria isolated from the 33 positive blood cultures (n = 16; 48.5 %). Moreover, non-group A β-hemolytic streptococci were isolated more frequently than group A β-hemolytic streptococci (39.4 % vs. 9.1 %). Group G Streptococcus was the most commonly isolated pathogen (24.2 %), which confirms the findings of other studies [9, 19]. However, a notable finding of the present study was that GNB were isolated in 24.2 % (8/33) of bacteremia cases. The 2014 IDSA guidelines do not recommend empirical antimicrobial therapy against GNB for the management of erysipelas and cellulitis except in severely compromised patients, in whom broad-spectrum antimicrobial agents such as vancomycin plus either piperacillin-tazobactam or imipenem/meropenem are recommended [3]. Because we only identified 33 cases of true bacteremia in the current study, further multicenter studies are needed to identify the risk factors for GNB bacteremia in cellulitis.

Our study design has several limitations. First, because it is retrospective in nature, clinical signs and co-morbidities were only derived from patient records. Second, although the prescription rate for antimicrobial agents prior to blood culture was not significantly different between the two groups (negative blood culture vs. positive blood culture: 1.89 % vs. 3.03 %, p = 0.66), it was difficult to accurately determine the true timing of prescription of antimicrobial agents relative to blood culture sampling from the computerized records. Further prospective studies are needed to control the confounding factor of pretreatment with antimicrobial agent. Third, the prediction model was developed for hospitalized patients in a tertiary teaching hospital in Taiwan over a 1-year period. Thus, the selection bias of a population with a higher degree of disease severity is inevitable, and our findings may not be generalizable to other hospital or outpatient settings in Taiwan or overseas. In addition, the study cohort seems to be limited for model training and testing as performed in our study. Therefore, external validation with an independent sample, either from a different time period at the same collection site or from a different collection site, is needed to validate our preliminary results and evaluate the generalizability of the model. Finally, this study was limited to adults. Because of differences in demography, disease co-morbidities, and microbiology, the results of the current study cannot be applied to children [20].

This study has provided a preliminary, diagnostic prediction model to estimate the probability of true bacteremia in cases of cellulitis. Based on the demographic and clinical characteristics of patients upon admission, the Bacteremia Score of Cellulitis may provide a simple prediction model to stratify cellulitis patients into low, medium, and high risk groups, and help clinicians optimize decision making upon admission. However, this prediction model has several limitations, as described above. A multicenter prospective study with a larger number of cellulitis patients, including more immunocompromised hosts and children, is needed to validate the Bacteremia Score of Cellulitis. This may lead to the development of an easy-to-use and validated diagnostic model to restrict the drawing of blood cultures in cellulitis cases to those with a high probability of true bacteremia.