Regulatory Mechanisms
in biosystems
Regulatory Mechanisms
in
Biosystems
ISSN 2519-8521 (Print) ISSN 2520-2588 (Online) Regul. Mech. Biosyst., 8(1), 98-103 doi: 10.15421/021717
Ultrastructural changes in biofilm forms of staphylococci cultivated in a mixed culture with lactobacilli
G. Lavryk, O. Korniychuk, M. Tymkiv
Danylo Halytskyi Lviv National Medical University, Lviv, Ukraine
Article info
Received 19.01.2017 Received in revised form
17.02.2017 Accepted 20.02.2017
Danylo Halytskyi Lviv National Medical University, Pekarska Str., 69, Lviv, 79000, Ukraine E-mail: [email protected]
Lavryk, G., Korniychuk, O., & Tymkiv, M. (2017). Ultrastructural changes in biofilm forms of staphylococci cultivated in a mixed culture with lactobaciUi. Regulatory Mechanisms in Biosystems, 8(1), 98-103. doi: 10.15421/021717
The capacity of opportunistic bacteria for biofilm formation plays an important role in the development of chronic inflammatory processes, which are difficult to treat. To improve antimicrobial therapy methods, the influence of lactobacilli on the ultrastructure of biofilm-forming clinical strains of staphylococci when co-cultured was investigated. 5 biofilm-forming clinical strains of S. aureus from the skin of acne vulgaris patients (n = 24) were isolated. Using transmission electron microscopy (TEM) the morphological changes of S. aureus cells in the mixed culture with standard strains of Lactobacillus plantarum 8P-A3 and clinical strains of L. fermentum (n = 4) were studied. It was found that in 48 hours after the inoculation on the medium of samples of mixed cultures of L. plantarum 8P-A3 and S. aureus growth of staphylococci was not revealed. Only in some cases of mixed cultures of L. fermentum and biofilm-forming staphylococci was growth of S. aureus obtained. In electron diffraction patterns of control samples of 24-hour staphylococcal monocultures and 48-hour lactobacilli monocultures, natural development of the population at the cellular level was observed. Destructive changes under the influence of lactobacilli (probiotic and clinical strains) were detected in all ultrathin sections of the cells of biofilm-forming and planktonic staphylococci. Significant destructive changes in the cell wall of the staphylococci were observed: thickening, obtaining of irregular form, detachment of the cytoplasmic membrane, the complete destruction of the peptidoglycan layer and the emergence of "shadow cells". On all electron diffraction patterns fibrillar-threadlike structures of DNA could not be observed, but in some cases mesosome-like formations were poorly contrasted. It was established that the surface S-layer of lactobacilli was expressed on a significantly larger scale in the mixed culture with staphylococci. In mixed culture of clinical strains of lactobacilli with biofilm form of S. aureus, staphylococcal cells could be found in a dormant state. Thanks to an experimental model of biofilm in a mixed culture, the development of destructive changes of staphylococci under the influence of the lactobacilli both on the morphological and at the population levels has been assessed. The results obtained can be used in improving the schemes of complex antimicrobial therapy of pyoinflammatory processes with the use of biological preparations, which are composed of lactobacilli, including those in the form of local application.
Keywords: biofilm; Lactobacillus; Staphylococcus aureus; transmission electron microscopy
renko, 2010). Biofilm microbiota, being in a symbiotic relationship with the macroorganism, create a powerful biological barrier, which prevents colonization of the epithelium by pathogenic microorganisms and ensures the preservation of its own microflora in natural human biotopes (Shyrobokov et al., 2009; He et al., 2011). It was found that human commensal microorganisms, being a part of the skin microbiocenoses, intestines, mucous, form complex interspecific communities (Hall-Stoodley and Stoodley, 2009; Harriott and No-verr, 2009). These formations are social systems characterized by certain co-operation and functional specialization, controlled by the QS-system (quorum sensing). Global regulation ensures the formation of biofilm, as well as increased bacterial adhesion, the beginning of the synthesis of the factors associated with the antagonistic activity for representatives of indigenous microflora and the manifestation of the pathogenicity for opportunistic microflora (MacFarlane, 2008; Bondarenko, 2011).
Lactobacilli are essential symbionts and members of various human body ecosystems. Anti-staphylococcal activity of lactobacilli strains is carried out by the production of nonspecific antimicrobial metabolites, such as organic acids including lactic, acetic, propionic and butyric, hydrogen peroxide, lysozyme and bacteriocin-like inhi-
Introduction
Staphylococci, as ubiquitous opportunistic microorganisms, colonize the skin of the mucous membranes of many human body ecosystems (nasopharynx and oropharynx, gastrointestinal tract, vagina) (Wertheim et al., 2005). The carriage of staphylococci in the human population is over 20% (Kluytmans et al., 1997; Dall'Antonia et al., 2005). Staphylococcus aureus biofilm formation is a serious problem in nosocomial infections, and especially in the development of resistance to the majority of existing antibiotics. It should be stated that the ability to colonize and form biofilms on medical implants, catheters, endotracheal tubes, leads to the emergence of serious catheter-ventilator-associated infectious complications, sepsis (Reid, 1999; Weinstein and Darouiche, 2001; Ghannoum and O'Toole, 2004; Pal et al., 2007; Eftekhar and Mirmohamadi, 2009; Revdiwala et al., 2012, Nair et al., 2014). Furthermore, 60-65% of infections of the respiratory and urinary tract, osteomyelitis, endocarditis, cystic fibrosis, perio-dontitis, sores, etc. are caused by biofilm forms of bacteria (Hall-Stoodley and Stoodley, 2009; Wang et al., 2010). S. aureus is a major cause of development of persistent, chronic pyoinflammatory infections (Otto, 2008; Hall-Stoodley and Stoodley, 2009; Gostev and Sido-
biting substances (BLIS), biosurfactants (glycolipids, rhamnolipids, lipopeptides, polysaccharide-protein complexes, phospholipids, fatty acids and neutral lipids) (Dworkin et al., 2006; Varma et al., 2010, 2011; Dobson et al., 2012).
The efficacy of probiotic preparations containing lactobacilli is largely due to the activity of various antimicrobial agents, including biosurfactants (Velraeds et al., 1996), which introduce a powerful intervention into biofilm communities by changing the surface properties of bacterial cells, reduce their adhesion (Ahimou et al., 2000) and hinder the development of biofilms and intercellular interaction (Rasmussen and Givskov, 2006; Valle et al., 2006).
Consequently, the metabolites of lactobacilli are able to inhibit biofilm formation and cause ultrastructural changes in S. aureus and S. epidermidis cells, which leads to their death (Varma et al., 2011).
The aim of this study is to investigate the influence of lacto-bacilli on the ultrastructure of biofilm-forming clinical strains of staphylococci when co-cultured.
Materials and methods
For the investigation, 5 biofilm-forming clinical strains, isolated from the skin of acne vulgaris patients (n = 24), were selected. Primary selection of the strains was carried out on the basis of changes in their culture properties, including expressed increase in colony viscosity. Thus the proportion of biofilm-forming forms was 20.8%. The strains of Lactobacillus fermentum (n = 4) were isolated from the mucosa of the upper respiratory tract of healthy patients. Isolation and identification of staphylococci were performed using standard nutrient medium in the laboratory of the microbiology department of Danylo Halytskyi Lviv National Medical University according to the conventional techniques (Birger, 1982; Vos et al., 2009).
Staphylococcal biofilm formation was performed at the bottom of plastic cups (0 50 mm) using nutrient broth ("Farmactiv", Ukraine), biofilm of lactobacilli - using MRS-broth (de Man, Rogosa, Sharpe, India). 4 ml of broth and 10 ^l of culture with turbidity 1,5 x 109 CFU/ml (corresponding to 5 McFarland units according to the standard) were added to each cup, in such a way that the suspension was uniformly distributed on the bottom of the cups. The cups with the staphylococci inoculations were placed in an incubator for 24 hours and the plates
Table
The dynamics of microorganisms growth after inoculation from biofilm
with the lactobacilli inoculations placed in an incubator for 48 hours, both at a temperature of 37 °C. After this exposure, the residual medium was collected from the cups in order not to destroy the existing biofilm and was washed with distilled water three times.
Similarly mixed cultures of Staphylococcus and Lactobacilli in MRS-broth were formed within 48 hours at 37 °C. For this 4 ml of the mentioned medium and 5 ^l of lactobacilli and the staphylococcal suspension with density 1,5 x 109 CFU/ml were added to the plastic cups. As a control, a live culture of Lactobacillus plantarum 8P-A3, which is included in the composition of a probiotic preparation "Lactobacterin", which was obtained by cultivation in micro-aerophilic conditions first in thioglycollate medium and then on MRS-agar, was used. The standard film-forming strain of S. aureus ATCC 25923 and not the film-forming strain of S. aureus ATCC 12228, were used to determine a benchmark.
To determine the number of viable cells both the staphylococci and lactobacilli in mixed cultures of biofilms, inoculations of 10 ^l on the solid medium immediately after the inoculation and at 12, 24, 48 hours were produced. In the case of a high density of the received culture it was diluted before the inoculation, which made it possible to set the number of germinated colonies.
Preparation of samples for transmission electron microscopy (TEM) was performed by classical methods (Weekly, 1975; Goldstein et al., 1984). They were viewed in the transmission electron microscope PEM-100-01 at a voltage of 75 kV at magnifications from x1,000 to x30,000.
Statistical analysis of experimental data was performed using Excel for PC. The significance of the difference between the two rates was assessed by Student's test. The difference was considered significant at P < 0.05.
Results and discussions
Comparison of capacities for isolation from mixed cultures in a nutrient medium and in conditions of the biofilm structure modeling was conducted. Controlling inoculation on the solid medium immediately after the inoculation in all samples of mixed cultures has demonstrated the presence of staphylococci in an amount, close to the inoculated dose from (4.5 ± 0.02) to (4.8 ± 0.04) x 108 CFU/ml (Table).
The number of microorganisms, CFU/ml
Bacterial strains associants
inoculated
the growth after inoculation from structured biofilm
dose U 11 12 h 24 h 48 h
L. plantarum 8P-A3 and 109 0* (1.1 ± 0.09) x 104 3 x 107 (0.9 ± 0.08) x 1012*
S. aureus ATCC 25923 (1:1) (4.7x ± 0.02) x 108 (1.2 ± 0.01) x 106 (1.35 ± 0.09) x 102 0*
L. plantarum 8P-A3 and 109 0* (1.3 ± 0.08) x 104 108 (1.0 ± 0.1) x 1012
S. aureus ATCC 12228 (1:1) (4.8x ± 0.02) x 108 (2.0 ± 0.02) x 106 75 ± 0.56 0*
L. fermentum, N = 4 109 0* (1.5 ± 0.08) x 104 1.5 x 108 0.85 ± 0.09) x 1012*
S. aureus (biofilm-forming form), N = 5 (1:1) (4.6x ± 0.02) x 108 (8.7 ± 0.07) x 106 (1.35 ± 0.09) x 102 (1.8 ± 0.2) x 102*
L. fermentum, N = 4 109 0* 3 x 104 1.5 x 107 (1.0 ± 0.08) x 1012*
S. aureus ATCC 12228 (1:1) (4.5x ± 0.02) x 108 (1.2 ± 0.04) x 106 (2.0 ± 0.10) x 103 0*
Note: statistically significant difference compared to control strains * - P < 0.05.
Growth of lactobacilli was absent. In isolation of cultures from structured biofilm samples association L. plantarum 8P-A3 as with the standard biofilm-forming strain of Staphylococcus and non-biofilm form strain after 12 hours, the number of lactobacilli was 1.1 ± 0.09 x 104 and 1.3 ± 0.08 x 104 CFU/ml, respectively, with an increase in the number of staphylococci to (1.2 ± 0.015) and (2.0 ± 0.03) x 106 CFU/ml. After 24 hours, the number of viable staphylococci rapidly decreased to (2.3 ± 0.02) and (2.0 ± 0.04) x 103 CFU/ml, and lactobacilli - increased to 107-8 CFU/ml.
The trend in the nature of isolation from biofilm structures of clinical isolates L. fermentum and S. aureus association was similar but more active isolation of both associant species was registered after 12 hours. After 24 hours the number of isolated L. fermentum was somewhat reduced in comparison with the activity of probiotic
lactobacilli. Inhibition of Staphylococcus growth to (1.35 ± 0.09) x 102 (biofilm form) was also observed and this inhibition was even more pronounced with the non-biofilm forming standard strain of staphy-lococci - 75 ± 0.56 CFU/ml. In 48 hours after the inoculation on the medium lactobacilli, were isolated from all samples, and reached the quantitative level 1012. Isolation of staphylococcus was discontinued, except for L. fermentum and S. aureus (biofilm form, the number (1.8 ± 0.2) x 102) and the growth of individual colonies of clinical isolates of staphylococci in the modeling of biofilm was registered (P < 0.05). Thus, clinical strains of lactobacilli adapted to the conditions of the organism are actively reproduced in vitro, being sufficiently effective antagonists under the conditions of biofilm. However, quantitatively, lactic acid lactobacilli promote more rapid death of staphylococci in a mixed culture. The studies also show higher
potential of preservation of the viability of biofilm form bacteria in the bi-species biofilm. To assess the nature ofthe cell damage in the staphylococci in the mixed culture with the lactobacilli, the ulrastructue of these species of bacteria was studied in biofilm modeling conditions. In analyzing electron diffraction patterns in control samples of 24-hour
film-forming monocultures and planktonic Staphylococcus and 48-hour lactobacilli, natural development of the population at the cellular level was observed (Fig. 1o-c). Cells were visualized at different stages of morphogenesis: separation with forming cytoplasmic wall, at rest, as well as with complete and partial autolysis (Fig. 16).
Fig. 1. Microphotography (TEM) of staphylococci and lactobacilli monocultures: (a) planktonic form of S. aureus ATCC 12228, (b) biofilm form of S. aureus ATCC 25923 at different stages of cell development, (c) clinical strain of L. fermentum
In most cells, a characteristic ultrastructural organization was observed: thick peptidoglycan layer, cytoplasmic membrane, nucleoid located diffusely in the form of light fibrillar-threadlike DNA structures, mesosomes (vesicular and lamellar membrane structures) in the place of septum formation. With almost all ultrathin sections of lactobacilli cells, the surface S-layer is visible. Only in the mixed culture of lactobacilli with staphylococci is it expressed on a significantly larger scale (Fig. 2c).
Comparing the electron diffraction patterns of 48-hour staphy-lococcal monocultures and cultures mixed with lactobacilli in the composition of biofilms, significant destructive changes in the ultrastructure of staphylococcal cells were observed (Fig. 2). Destabili-zation of the cell wall was manifested in its thickening, in the irregular form acquired by the cocci, detachment of the cytoplasmic membrane from the cell wall (Fig. 2f) and in the complete destruction of the peptidoglycan layer (Fig. 2a, e). Cell wall ruptures with the outflow of cell content were also recorded (Fig. 2b, e), which leads to a complete loss of colloid and corresponding protoplasmic structures and appearance of "shadow-cells" (Fig. 2d). Due to the high electron density of the cytoplasm in the nucleoid zone, it was impossible to oberve characteristic pronounced fibrillar-threadlike structures of DNA, in some electron diffraction patterns mesosome-like formations were poorly contrasted. Such destructive changes were detected in all the ultrathin sections of cells of biofilm-forming and planktonic staphylococci induced by probiotic (Fig. 2g, h) as well as clinical lactobacilli (Fig. 2a-e).
It is known that bacterial cells, growing in adverse conditions of a natural or artificial environment, such as the depletion of nutrients, oxygen, inadequate pH, etc. can be transformed into uncultivated (VBNC - viable but non-culturable) forms with a slow metabolism, but preserving their viability. The uncultivated state is characterized by a number of molecular, structural and functional characteristics of the biofilm (Lleo et al., 2007; Stewart and Franklin, 2008; Oliver, 2010; Trevors, 2011).
VBNC forms are in transient dormancy condition and are orientated towards adaptation to stress and are associated with significant dwarfism of cells, as well as the inability to grow on nutrient media. Nevertheless, uncultivated cells that retain a certain degree of metabolic activity can be restored in cultivated states with the help of appropriate stimulation (Oliver, 2010; Trevors, 2011; Zandri et al, 2012).
Our studies have shown that in the case of a combination of a biofilm form of S. aureus and clinical strains of lactobacilli dormant
staphylococci cells are found in the field of view (Fig. 2a). Difficulties in the treatment of many bacterial infections are associated with formation of biofilm by microorganisms in the patient, which plays an important role in clinical medicine (Chebotar et al., 2010; Qu et al., 2010). One way to improve the effectiveness of antimicrobial therapy of diseases caused by staphylococci, is the use of tools that contribute to the disintegration of the biofilm to the transition of the pathogen in planktonic form. Microorganisms-antagonists in composition of eubiotic preparations, particularly, lacto-bacilli may be used for this (Samot and Badet, 2013; Lee and Kim, 2014; Nair et al., 2014).
Different Lactobacillus species are part of the natural human body biosystems and participate in the formation of multispecies biofilms which contain two or more members within the association. It has been proved that L. reuteri, on the basis of which a large number of probiotics are created, can prevent reproduction of pathogenic bacteria and restore the natural biofilm of the urogenital tract in women (Whitchurch et al., 2002; Younes et al., 2012).
The bacterial cell wall and its associated proteins mediate the interaction between the environment and the cytoplasm of micro-bial cells. It acts as a structural barrier against the action of toxic chemicals, protects the cell from changing environmental conditions and plays an important role in infection and pathogenicity (Dmitriev et al., 2004). Changes in cell wall thickness take place under the influence of various factors. In particular, its thickening has been fixed among strains of antibiotic-resistant S. aureus in the presence of antibiotics (Cui et al., 2000; Cui et al., 2003; Kim et al., 2012). Increase in the thickness of the cell wall and its changes in biochemical composition have also been obtained under the influence of cold stress (Onyango et al., 2012). The phenomenon of "shadow cells" with the release of cellular material outside is described in the study of the damaging effect of silver on Pseudomonas aeruginosa using TEM. The results obtained are confirmed by the scanning electron microscopy (SEM): the complete loss of cell membranes with disintegration of intracellular material was recorded in the processed cells (Dosunmu et al., 2015). Similar investigations on the study of the silver ions mechanism of action were carried out on cultures of S. aureus and Escherichia coli. In gram-positive and gram-negative bacteria cell wall damage, the release of cell content, complete or partial separation of the cyto-plasmic membrane from the cell wall, and decrease in electron density in the cytoplasm were identified (Jung et al., 2008). The interaction between the silver and the components of bacterial membrane
causes structural changes and damage to membranes and intracellular metabolic activity, which may be the cause or the consequence of cell lysis (McDonnell et al., 1999; Sondi and Salopek-Sondi, 2004; Pal et al., 2007). Antiadhesive, antimicrobial and antibiofilm influence of biosurfactants produced by strains of L. jensenii and L. rhamnosus, in respect to a number of bacteria with clinical multidrug resistance (Acinetobacter baumannii, Escherichia coli and Staphylococcus
aureus (MRSA)), which can form biofilms on wounds, medical implants and industrial surfaces was revealed.Confirmation of TEM has shown cell wall damage and the appearance of shadow-cells (Sambanthamoorthy et al., 2014).
Comparing our results with those of other researchers, it may be suggested that such reaction of the cell wall may be common to bacterial cells under the influence of different stress factors.
Fig 2. Microphotography (TEM) of mixed cultures of staphylococci and lactobacilli: (a) L. fermentum and S. aureus ATCC 12228, (b) L. fermentum - excess of S-layer, (c, d, e, f L. fermentum and biofilm form of S. aureus (ultrastructural changes in staphylococcal cells are marked with arrows), (g) L. plantarum 8P-A3 and biofilm-forming form of S. aureus. L. plantarum 8P-A3 and S. aureus ATCC 12228
In one recent study (Khaleghi and Kermanshahi, 2012), the authors showed that environmental conditions affect the protein of the S-layer and the slpA gene expression. During the electron-microscopic examination of Lactobacillus acidophilus ATCC 4356, the excess of the S-layer was found at both ends of the bacterial cell at a temperature of 45 °C. This allows one to suggest that the S-layer protein is predominantly expressed in conditions which are not optimal for bacterial growth. The S-layer probably acts as a protective shell in L. acidophilus ATCC 4356. In addition, the results of some studies indicate the involvement of lactobacilli S-layer proteins in providing hydrophobicity, autoaggregation and adhesion of these bacteria to a variety of surfaces (Van der Mei et al., 2003; Vadillo-Rodriguez et al., 2004; Khaleghi and Kermanshahi, 2012; Hynonen and Palva, 2013).
In our studies, when comparing the S-layer of lactobacilli in mono- and mixed cultures, its increase was seen only in the second case - in the mixed culture of lactobacilli with staphylococci. These results confirm the hypothesis that the observed changes are the indicators of the reaction general to the bacteria manifested by morphological modifications in the conditions of interaction with the "unfriendly" assiociants.
Conclusions
In terms of bi-species biofilm modeling, survival of assiociants of both species increases. The probiotic strain of lactobacilli reveals a more pronounced antagonistic effect on the staphylococci cultures in comparison with the activity of clinical isolates, while maintaining a minimum viability of probiotic forms of Staphylococcus. At the population level, the ratio of morphological types of S. aureus cells with an increase in the amount of involutional and lysed cells changed. Significant ultrastructural changes took place at the morphological level of staphylococcal cells. In mixed cultures of clinical strains of lactobacilli and biofilm-forming staphylococci, the latter moved into a state of rest, fixed by TEM, and during inoculation they retained their capacity for cultivation in vitro, which indicates the high competitiveness of staphylococci. Thanks to an experimental model of biofilm in a mixed culture, the present study has allowed us to establish the nature of the antagonistic action of lactobacilli on S. aureus and to evaluate the development of destructive changes in the dynamics. The results obtained can be used in improving the schemes of complex antimicrobial therapy of pyoinflammatory processes with the use of biological preparations, which are composed of lactobacilli, including those in the form of local application.
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