Abstract
Colonization of in-dwelling catheters by microbial biofilms is a major concern in patient health eventually leading to catheter-related blood stream infections. Biofilms are less susceptible to standard antibiotic therapies that are effective against planktonic bacteria. Standard procedure for the detection of microorganisms on the catheter tip is culture. However, viable but non-culturable cells (VBNCs) may be missed. The aim of this study was to evaluate the use of fluorescence in situ hybridization (FISH) as an indicator to visualize and quantify the effect of the antibiotics daptomycin and vancomycin on biofilms in situ. We established an in vitro catheter biofilm model of Staphylococcus epidermidis biofilms on polyurethane catheters. Biofilm activity was measured by FISH and correlated to colony forming units (CFU) data. Digital image analysis was used for quantification of total biofilm mass and the area of the FISH positive biofilm cells. FISH showed a pronounced effect of both antibiotics on the biofilms, with daptomycin having a significantly stronger effect in terms of both reduction of biofilm mass and number of FISH-positive cells. This supports the anti-biofilm capacity of daptomycin. Interestingly, neither antibiotic was able to eradicate all of the FISH-positive cells. In summary, FISH succeeded in visualization, quantification, and localization of antibiotic activity on biofilms. This technique adds a new tool to the arsenal of test systems for anti-biofilm compounds. FISH is a valuable complementary technique to CFU since it can be highly standardized and provides information on biofilm architecture and quantity and localization of survivor cells.
Highlights
In-dwelling medical devices such as central-venous catheters can become colonized by biofilms, leading to severe bacteraemia and sepsis
The S. epidermidis polysaccharide intercellular adhesin (PIA) 8400 strain chosen for the present study showed variation in the amount of biofilm obtained, in spite of the same stringent experimental conditions being maintained
The present study demonstrates, for the first time, the use of fluorescence in situ hybridization (FISH) for visualization, quantification, and localization of the rRNA containing cells within a catheter-related biofilm following antibiotic treatment
Summary
In-dwelling medical devices such as central-venous catheters can become colonized by biofilms, leading to severe bacteraemia and sepsis. Catheter-related blood stream infections have been shown to increase the financial burden for intensive care unit patients and the health care system in addition to causing higher patient mortality [2]. Long-term use of central venous catheters is associated with a risk of bloodstream infection and sepsis (2.7 cases per 1000 catheter-days) [3]. Vancomycin is the standard antibiotic agent for empirical therapy in cases of catheterrelated blood stream infections due to methicillin-resistant Staphylococcus spp.; for vancomycin minimal inhibitory concentrations (MICs) >2 μg/mL alternative treatment with daptomycin is recommended [4]. Emergence of resistance to vancomycin in blood stream infection cases of methicillin-resistant coagulase negative staphylococci caused by higher MICs has previously been reported [5, 6]
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