Nebulised amphotericin B to eradicate Candida colonisation from the respiratory tract in critically ill patients receiving selective digestive decontamination: a cohort study

This study was performed in a 32-bed mixed ICU of the University Medical Center Utrecht in the Netherlands between April 2008 and February 2012. The Ethics Committee of the University Medical Center Utrecht approved this study and waived the need for informed consent. We analysed all mechanically ventilated adults who had been admitted to the ICU for >72 hours. Microbiological screening for the presence of Candida was prospectively carried out on admission and twice weekly thereafter according to a standardised protocol that was part of a SDD/Selective Oropharyngeal Decontamination (SOD) trial [12]. In brief, samples were inoculated on malt extract agar plates, and Candida load was semi-quantitatively determined (that is classified as <10, 10 to 100, and >100 colony-forming units). Colonisation was defined as the presence of Candida species in two or more consecutive bronchoalveolar lavage or sputum samples obtained on different days in the ICU, and the colonisation start date as the first positive sample. Decolonisation was defined as the absence of Candida in two consecutive samples on different days, or as the absence of Candida in the last available sample. We excluded episodes during which patients had received systemic antifungal treatment, as well as episodes during which NAB was initiated within the first two days after colonisation start date (before results of microbiological surveillance cultures had become available), because the reason for use of amphotericin B in these cases was likely to be different.

All patients received either SDD (from April 2008 to August 2009 and from June 2011 to February 2012) or SOD (from September 2009 to May 2011). During SDD (but not during SOD) NAB, four times 5 mg daily, was recommended in case of Candida colonisation of the LRT [12]. To this end, 50 mg of conventional amphotericin B for intravenous use was dissolved in 10 mL water for injection. For each nebulisation session 2 mL of water for injection was added to 1 mL (= 5 mg amphotericin B) of the prepared solution and aerosolised with a jet nebuliser system (Covidien, Mansfield, MA, USA). Air or oxygen under high pressure with a flow rate of 5 to 8 L per minute was used to generate aerosols with a mass median aerodynamic diameter of <5 micrometer. Each session lasted until all medication was inhaled (about 15 to 30 minutes). The nebuliser was attached to the ventilator circuit with a T-piece adaptor positioned between the endotracheal tube and the humidification filter. The nebulisation protocol did not recommend specific ventilator settings. In our clinical practice, however, patients remained on a pressure-controlled ventilator with unchanged positive end-expiratory pressure (PEEP) and inspiratory pressure settings. Depending on the mechanical ventilator type nebulisation was continuously administered during both inspiration and expiration in half of the NAB treatments, whereas in the remaining cases nebulisation was only during inspiration. Allocation of a ventilator depended on availability and was independent of patient characteristics. The humidification filter in the mechanical ventilation circuit was changed after each nebulisation session to avoid obstruction.

Because the delay in the initiation of NAB treatment (relative to the start of colonisation) may vary between patients, it is important to correct for time-varying bias, which occurs when the exposure variable is categorised to its final status rather than considering the timing of the change in status [13, 14]. Furthermore, patients who spontaneously decolonise early have less opportunity to receive NAB. These cases contribute better outcomes to the non-exposed group and therefore may lead to an underestimation of the treatment effect. To deal with these issues, we used time-varying Cox proportional hazards regression with adjustment for age, Sequential Organ Failure Assessment (SOFA) score, Candida load at baseline, and concurrent use of corticosteroids.

In order to graphically represent the results of our time-varying analysis and correctly estimate the median time to decolonisation relative to the start of NAB [15], we used the multistate model shown in Figure 1[16].

As a secondary study outcome, we compared the incidence rates of VAP occurring after the onset of the Candida colonisation episode in both groups. For the period 2008 to 2010, we retrospectively assessed the medical records for the occurrence of VAP, according to established CDC criteria [17]. For the period 2011 to 2012, we prospectively recorded the incidences of VAP as part of an ongoing cohort study that is aimed at finding early diagnostic and prognostic markers of sepsis [18]. Furthermore, we compared ICU mortality and remaining length of stay in ICU following the onset of Candida colonisation in patients receiving NAB compared to patients not receiving NAB.

To assess possible effect modification by the timing of treatment, we performed a secondary analysis on the overall treatment effect by comparing patients who had received NAB treatment early (within five days) versus late (after five days) following the colonisation start date. Because of a reduced number of decolonisation events in this subgroup analysis of early and late NAB starters, we tested possible confounders by adding each of them separately to a univariable Cox regression model containing only NAB as an explanatory variable and examining its effect on the beta coefficient of the NAB variable on decolonisation. Covariables that caused substantial confounding (that is a change in effect estimate greater than 10%) were included in the final multivariable models. In addition, to assess possible indication bias we performed a per-protocol analysis of patients treated according to the SDD and SOD arms of the trial. Data were analysed with SAS 9.2 (SAS Institute, Inc., Cary, NC, USA) and R 2.15.1 software (package mstate).

There were 27/31 (87%) and 24/28 (86%) decolonisation events in early and late NAB starters, respectively, resulting in an adjusted HR of 2.0 (95% CI 1.3 to 3.1), and 2.0 (95% CI 1.3 to 3.2), respectively. During the SOD period, in which NAB treatment was not recommended in the protocol, NAB was applied in 6 of 166 (4%) cases, whereas during the SDD period 114 of 167 (68%) cases did not receive NAB while being colonised. However, after exclusion of episodes during SDD in which NAB was not started as well as episodes during SOD in which NAB was administrated (per-protocol analysis), the effect estimates remained similar (crude HR 2.1; 95% CI 1.4 to 3.0, adjusted HR 2.2; 95% CI 1.5 to 3.3).