Microbiological analysis of endotracheal aspirate and endotracheal tube cultures in mechanically ventilated patients

Inclusion criteria: Patients treated with MV at the ICU of Jiading District Central Hospital Affiliated Shanghai University of Medicine & Health Sciences. All intubations were preformed according to “American Journal of respiratory and critical care medicine” [15]. Exclusion criteria: (1) Refusal by the patients’ guardian; (2) Patients showing inconsistency in the results of Gram staining and microbiological culture; (3) Other factors (Patients with no ETAs, ETTs contamination during extubation or transportation, etc.).

Diagnostic criteria for lower respiratory tract infections: (1) Patients with body temperature more than 38 °C, (2) leukocytosis, (3) microbiological culture showed a positive result, (4) lung density in physical examination in association with the presence or changes in radiographic infiltration [16, 17].

General information (gender, age) and past medical history (hypertension, diabetes, etc.) of patients were collected, and the Acute Physiology and Chronic Health Evaluation II (APACHE-II) score was calculated on the day of admission. The length of hospital stay of each patient were tracked until leaving the ICU or death.

ETTs were obtained immediately after extubation. Roughly 1 cm of the distal end of the ETTs was cut for microbiological culture analysis. ETAs was extracted by a steriled suction tube, which inserted into the lower respiratory tract through a catheter.

Blood agar plates, MacConkey plates, and chocolate agar plates were provided by Shanghai Yihua Biotechnology Co., Ltd. (Shanghai, China). The VITEK 2 compact automatic bacterial identification and drug susceptibility analysis systems (bioMérieux, Marcy-l’Étoile, France) was used. Staphylococcus aureus (ATCC29213) and Pseudomonas aeruginosa (ATCC27853) were purchased from the Shanghai Clinical Laboratory Center as the quality control strains.

Microbiological culture analysis of ETAs and ETTs collected was preformed according to the CSLI method [18]. Briefly, part of the ETAs and ETTs collected was subjected to Gram staining, and the rest of the samples were immediately incubated onto a blood agar plate, a MacConkey plate, and a chocolate agar plate. All plates were incubated at 35 °C with 5% CO₂ for 18–24 h before interpretation. Pure cultures and dominant pathogens were identified by the VITEK2 systems. The result of microbiological culture was included only when the dominant strains were consistent with the Gram staining result.

All statistical analyses were performed in the R environment [19]. Data were summarized as mean ± standard deviation (SD) or percentage. For the data of duration of ventilation days, the median was used, indicated as M (Q1~Q3). One-way analysis of variance and chi-square test were used for statistical analysis. Spear-man correlation analysis, coincidence rate, kappa coefficient and PCA were performed to analyze the results of microbiological culture from the two kinds of samples.

There were 332 patients admitted to the ICU of Jiading District Central Hospital Affiliated Shanghai University of Medicine & Health Sciences from September 1st, 2017 to August 31st, 2018, of which 144 were treated with MV. 81 of them matched the criteria and were included in this study. The reasons of hospitalization were summarized as followed: severe pneumonia (n = 24), severe cerebrovascular disease (n = 19), multiple injuries (n = 15), acute exacerbation of chronic obstructive pulmonary disease (n = 9), cerebral trauma (n = 9), and others (n = 5; Fig. 1). The mean age of patients was 62.1 ± 19.7 years, in which 63 patients were males (77.8%) and 18 patients were females (22.2%; Table 1). ETTs was extubated when: (i) Patients recovered (n = 49, 60.5%); (ii) change of ETTs (n = 3, 3.7%); and (iii) patients succumbed to mortality (n = 29, 35.8%).

Within 81 ETTs, 61 of them (75.3%) grew one (50) or two (11) major populations of pathogenic bacteria, while the other 20 samples grew single major population of normal respiratory track flora. i.e. A total number of 92 major populations of cells were observed, in which 72 of them were pathogenic bacteria and 20 were normal respiratory track flora. Bacterial identification results showed that the main pathogens observed were A. baumannii (39.1%, 36/92), P. aeruginosa (12.0%, 11/92), S. aureus (9.8%, 9/92), and K. pneumoniae (7.6%, 7/92) respectively (Fig. 2a).

For ETAs analysis, 57 specimens (70.4%) grew pathogenic bacteria as major cell population, while 24 of them grew normal respiratory track flora as major population of cell. Totally 89 populations of cells were observed, of which 63 were pathogenic bacteria and 26 were normal respiratory track flora. The main pathogenic bacteria stains were A. baumannii (34.8%, 31/89), P. aeruginosa (13.5%, 12/89), S. aureus (7.9%, 7/89), and K. pneumoniae (7.9%, 7/89; Fig. 2b).

Spear-man correlation analysis showed that in general the results of microbiological culture from ETAs were positively correlated with those from ETTs (Spear-man γ = 0.757, P < 0.01). In addition, P. aeruginosa, normal respiratory flora, S. aureus, K. pneumoniae, and A. baumannii showed positively correlation between two kinds of specimens (Spear-man γ = 0.951, 0.757, 0.730, 0.687, 0.676, all P < 0.01). Lower respiratory tract infection rate was positively correlated with age (Spear-man γ = 0.561, P < 0.01). The presence of normal respiratory flora is negatively correlated with the growth of pathogens in either ETTs (Spear-man γ = − 1, P < 0.01) or ETAs (Spear-man γ = − 0.970, P < 0.01) samples (Table 2) as expected. Meanwhile, we analyzed factors including diabetes mellitus, hypertension, duration of ventilation days, APACHE-II and the cause of hospital admission with the results of microbiological culture from the two samples types (Additional file 1: Table S1, S2), the results showed low correlation between those factors and the type and diversity of bacterial species found within either type of the two samples.

The comparison between culture data of ETAs and ETTs showed that the total microbial coincidence rate was 96.7%. The coincidence rate of K. pneumoniae, P. aeruginosa, and A. baumannii were 100, 90.9, and 86.1%, respectively (Table 3).

Kappa analysis showed that microbial data of ETAs and ETTs were highly conserved in general (κ = 0.751); The κ values of P. aeruginosa, S. aureus, K. pneumoniae, and A. baumannii were 0.949, 0.723, 0.687, and 0.670, respectively (all P < 0.001).

PCA was performed and the result was as shown in Fig. 3. Each pathogen and the overall culture results showed a high degree of similarity.