TY - JOUR
AU - Visscher, Christian
AB - Introduction Campylobacteriosis is one of the world's most important diarrhoeal diseases in humans [1]. It was estimated that in 2010, Campylobacter was responsible for 166 million diarrhoeal illnesses and 31,700 Guillain–Barré syndrome cases worldwide [2]. In Europe, in the overwhelming majority of cases Campylobacter-associated diarrhoeal diseases is caused by the consumption of contaminated poultry meat [3]. One approach to eliminating C. jejuni in the food chain is to prevent the colonisation of broiler chickens [4]. The extent of contamination shows a positive correlation between the counts of Campylobacter in the caecal content and the number of bacteria on the carcass and the pectoral muscle [5]. In in vitro studies, lauric acid was one of the most effective acids for inhibition (<0.5 mM for C. jejuni ssp. jejuni CCM 6214T) in the growth of C. jejuni [6]. Also, short chain fatty acids have been tested in vitro, butyrate being the most successful one [7]. The addition of butyrate as a coated formulation in an in vivo experiment failed to reduce caecal colonisation [7] as did diets supplemented with 1% (wt/wt) noncoated caproic, caprylic, or capric acid sodium salt [8]. Substituting 1% soybean-oil with 1% LodestarTM C8-10 (Loders Croklaan, Wormerveer, the Netherlands; 56% C10, 30% C8, 10% C12, <3% C6, and <3%) showed an effect on the number of C. jejuni bacteria required to colonise 50% of inoculated broilers. This was estimated to be 200 times higher in broilers fed with supplemented feed than in control broilers [9]. Studies regarding the effect of lauric acid rich fats in vivo are rare. Palm kernel oil and coconut oil belong to the group of lauric acid rich oils [10]. In the physical refining of palm kernel oil, palm kernel fatty acid distillates are obtained as a by-product and contain more than 38% lauric acid [11, 12]. Under common rearing conditions of broilers, C. jejuni is rarely found in birds less than three weeks of age [13]. In older bird, the relationship between birds`age and C. jejuni prevalence shows no uniform results. On the one side, Campylobacter counts were 0.5 and 0.7 log10 units higher on carcasses of 42-d-old birds as compared to counts on carcasses of broilers 49 and 56 d of age, respectively [14]. On the other side, there are research groups who showed that the prevalence increases with the age of the birds in the form of a quick, usually unnoticed spread throughout the flock [15]. In conventional poultry farming, economically effective production systems are established, using modern breeds for fattening with high feed intake and body weight gains [16]. It is known from meta-analytically collected data that increased growth has a significant correlation with reduced immune function [17]. For example, there was a large (standard difference in means ≈-0.8) and a significant (P<0.001) negative effect of selection for body mass on immune function [17]. In organic poultry farming, however, other breeds are used. These slow-growing breeds are described as having a lower mortality rate [18] and a more robust immune system [19]. Therefore, it is surprising at first glance that Campylobacter prevalence in organic poultry farming is very high [20], sometimes significantly higher than in conventional farming [21]. Campylobacter spp. were isolated from 100% of organic broiler flocks, from 36.7% of conventional broiler flocks and from 49.2% of extensive indoor broiler flocks [21]. There are hardly any statements about C. jejuni prevalence in laying hens. In one study, Campylobacter could be detected at a high prevalence in caeca (53.3%) [22]. Therefore, it is not clear whether the differences in C. jejuni prevalence between production methods (conventional or organic) and direction of use (poultry intended for meat or egg production) can be explained by a different risk of infection from the environment, differences in feeding, the age of birds or by different genetics. Therefore, to our knowledge, there are no in vivo studies describing the fate of lauric acid from palm kernel fat in the gastrointestinal tract of broiler chickens. Furthermore, in a second approach, the course and intensity of an experimental C. jejuni challenge under the influence of a lauric acid rich palm kernel fatty acid distillate in poultry of different age at challenge and breeds was studied. The objective of this experimental C. jejuni infection approach was to investigate, (I) the fundamental effect of lauric acid supplementation in poultry of different breeds and directions of use, (II) the effect of age at time of experimental infections, (III) or rather the effect of breeds for different directions of use on C. jejuni spreading in small groups of birds. Materials and methods Animal experiments were performed in accordance with the German rules and regulations and approved by the Ethics Committee of Lower Saxony for Care and Use of Laboratory Animals LAVES (Niedersaechsisches Landesamt fuer Verbraucherschutz und Lebensmittelsicherheit; reference: 33.19-42502-05-15A500). Animals and housing The birds used in the experiment were supplied as day-old chicks directly from the hatcheries. The chicks of the genetics CobbSasso 175 (CS175; only genetic for experiment 1), Ross 308 (R308), and Hubbard JA 757 (Hb757) were obtained from BWE-Brueterei Weser Ems, Visbek, Germany. Male chicks of the Lohmann Brown-Classic (LBC-A42, LBC-A98; male; two age groups) and Lohmann Dual (LD) breeds were supplied by Lohmann Tierzucht GmbH, Cuxhaven, Germany. The experiments were divided into two parts: In the first part (Experiment 1), chickens of the genetics CS175 were used for analysing the concentrations of lauric acid in different parts of the gastrointestinal tract at dissection. The birds were given either a conventional complete diet or a lauric acid rich diet. In total, 32 chickens were kept in two different groups after the pre-experimental period of two weeks up to the end of day 42 of life. The experiment was conducted once. In the second part (Experiment 2), identical diets (without/with lauric acid supplement) were offered in birds of different breeds. For this second experiment chicks of the genetics R308, Hb757, LBC and LD were used. Therefore, effects on the spread of an experimentally induced C. jejuni infection were analysed depending on diet (without/with lauric acid supplement), age of the chickens (LBC-A42, LBC-A98) and on genetics (R308, Hb757, LBC, LD) during infection. For Experiment 2 (Table 1), four different breeds (R308, Hb757, LD, LBC) were reared under the same conditions in three independent repetitions (r = 3). Each breed consisted of 30 broilers which were randomly assigned to two subpopulations (15 birds, respectively). Only male birds from laying hybrids (LD and LBC) were used for the experiments. Birds of the LBC breed were also integrated into the experimental phase at different ages (LBC-A42, LBC-A98). Five birds per repetition, kept in a separate pen in the same room were used as sentinels. Therefore, the trials were based on a total of 465 chickens, conducted in three repetitions with 155 birds each. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 1. Experimental design showing distribution of birds based on breed, age and diet. https://doi.org/10.1371/journal.pone.0204483.t001 In the pre-experimental period (Fig 1), all birds were reared in identical floor pens littered with wood shavings. The pens were each equipped with an infrared lamp in order to reach a temperature at the outset of about 34–36°C. The temperature was lowered by about 1°C every two days, reaching a minimum temperature of about 20°C. The photoperiod beginning from d 4 was 16 h of light and 8 h of darkness during the whole trial. Download: PPT PowerPoint slide PNG larger image TIFF original image Fig 1. Schedule of the trial (Experiment 2) with actions, analyses and parameters in chickens of different breeds (R308 = Ross 308; Hb757 = Hubbard JA 757; LD = Lohmann Dual; LBC-A42 = Lohmann-Brown-Classic, dissection after 42 days; LBC-A98 = Lohmann-Brown-Classic, dissection after 98 days). https://doi.org/10.1371/journal.pone.0204483.g001 After the fourteen-day rearing phase, all chickens in groups R308, Hb757, LD and LBC-A42 were transferred from the rearing to the infection unit of the animal house (security level 2). The experimental period started about four weeks before dissection (d-28). Birds in group LBC-A98 had been purchased seven (trial 1) or eight (trials 2+3) weeks prior to the start of the experimental period at a greater age. Therefore, these birds were transferred after an extended rearing phase to the infection unit at an age of about 63 or 70 days. At this time, birds of all genetic breeds and ages were randomly subdivided into ten subgroups for each repetition. Groups received either a control (CON) or the experimental lauric acid rich diet (LA; Table 2). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 2. Ingredient composition of the different experimental diets during the different fattening phases. https://doi.org/10.1371/journal.pone.0204483.t002 During the experimental period (d-28–d0) the birds were kept on solid floor pens in groups of 15 birds (“subgroup”) up to the end of the experimental period. A maximum stocking density of 30 kg per square metre applied to all groups. Due to the use of different breeds, metabolic body mass was applied as the standard dimension. A stocking density of 30 kg per square metre corresponds to a metabolic body mass of 23.3 kg0.75 per square metre. Due to the expected final body weight of the different breeds at the time of the dissection, the size of the boxes was then established. The base area of the feeding trough and the water lines, 0.17 square metres, was added to the calculated box size. As a result, the subgroups of different breeds had boxes with varying degrees of floor space available (R308: 1.53 m2, Hb757: 1.21 m2, LD: 1.04 m2, LBC-A42: 0.59 m2, LBC-A98: 1.17 m2 [Experiment 1] and 1.25 m2 [Experiment 2]). Movable partition walls made of stainless steel at a height of 60 cm made it possible to adapt the floor space to the desired stocking density. The boxes were separated from each other by 80 cm high completely closed plastic walls on the other three sides. The boxes were 106 cm wide but varied in depth. Between adjacent boxes there was also a distance of 106 cm. Boxes were littered with wood shavings (1 kg/m2). Feeding regime and diet The diets used in the study were produced and delivered by a feed company producing compound diets (Best 3 Gefluegelernährung GmbH, Twistringen, Germany). The rearing phase was divided into a one-week starter phase with a conventional pelleted starter diet (starter) and a subsequent seven-day phase with a commercially available pelleted grower diet (grower). All diets were offered ad libitum. During the first three days additional feed was available (about 300 g/d) on so-called Chickpaper to get the birds accustomed to the diet. The different diets for the experimental period were designed in accordance with the recommendations for the energy and nutrient supply of the laying hens and fowls (broilers) of the Committee for Needs Standards of the Society for Nutritional Physiology [23]. The energy and nutrient content were comparable to the commercially available standard fattening diet (Table 3). The basic finisher feed for diets CON and LA was a common pellet diet which had been reduced by 2% in its fat content. In the CON groups, the diet was supplemented by 5% of a commercial standard fat (C 12 < 6%). In the LA groups, 5% fat enriched with palm kernel fatty acids including high levels of lauric acid (C 12 = 42–53%) was added as already described [24]. From the results of preliminary tests on the suitability of palm kernel fatty acids or combination of palm kernel fatty acids and capric acid and capric acid (data not shown), the use of a palm kernel product was preferred. The application amount was also determined in preliminary tests. Two different concentrations (2% and 5%) were tested. There was no negative effect on performance at the higher concentration. The higher concentration would also be the economically acceptable upper limit. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 3. Energy content and nutrient composition of the experimental diets during the different fattening phases. https://doi.org/10.1371/journal.pone.0204483.t003 Circular feeding troughs were used (Crown Poultry Feeders, Nelson, New Zealand). In the rearing phase water was offered ad libitum in double-cylinder plastic bell drinkers. Later, drinking lines equipped with Top Nipples with a drinking cup were used (Big Dutchman International GmbH, Vechta-Calveslage, Germany). The water was treated with chlorine containing product (Virbac Clean Pipe, VIRBAC Tierarzneimittel GmbH, Bad Oldesloe, Germany) at a concentration of 0.3 mg free chlorine/L to kill any C. jejuni in the drinking water. Feed and chyme analysis Diets were analysed by standard procedures in accordance with the official methods of the VDLUFA [25]. The analyses were always performed in duplicate. The dry matter content (DM) was determined by drying to the weight constancy at 103°C. The raw ash was analysed by means of incineration in the muffle furnace at 600°C for six hours. The total nitrogen content was determined by elemental analyser (Elementar, Hanau, Germany), which operates according to the principle of a catalytic tube combustion (DUMAS combustion method). Molecular nitrogen formed by reduction from nitric oxide was detected by a thermal conductivity detector. The nitrogen content was calculated with the device software. Therefore, the crude protein content of the sample was determined by multiplying with a constant factor of 6.25. The crude fat content was determined after acid digestion in the soxhlet apparatus. The content of crude fibre was determined after washing in dilute acids and alkalis. Starch determination was carried out polarimetrically (Polatronic E, Schmidt und Haensch GmbH & Co., Berlin, Germany). The sugar content was analysed in accordance with Luff-Schoorl method by titration with sodium thiosulphate. The mineral content was determined in accordance with the official methods [25] by atomic absorption spectrometry (Unicam Solaar 116, Thermo, Dreieich, Germany). Amino acids were determined by ion-exchange chromatography (AA analyser LC 3000, Biotronic, Maintal, Germany) and results evaluated in accordance with established methods [26]. Determining levels of medium and long chain fatty acids in the diet and intestinal content samples was carried out using established methods [27]. Exactly 200 mg of analytical material was placed in a glass tube. A methanol-hexane-tridecanoic-acid mixture was utilised as standard. Subsequently, acetyl chloride was added and the sample was heated, followed by the addition of potassium chloride solution. The measurement was carried out by gaschromatography (GC TRACE 1300, Thermo Scientific, Dreieich, Germany; SP-2560 Column, Supelco, Bellefonte, USA; carrier gas: nitrogen) after centrifugation with the superior hexane phase. Experimental design and sampling Performance parameters. In Experiment 1, the individual body weight (BW) of birds was determined (PCE TB 30, PCE Instruments, Meschede, Germany) at the beginning and at the end of the feeding phase (d-28, d0) and the average daily feed intake (ADFI) on a subgroup basis to determine average daily weight gains (ADWG) and the feed conversion ratio (FCR). In Experiment 2, the BW of the chickens was recorded individually at the start, at the time of experimental challenge and at the end of the experimental period (d-28, d-21 and d0). The ADFI was recorded at the level of the subgroup. Each subgroup had a 30 L polypropylene feed bucket into which the diet for the corresponding subgroup for the whole experimental period was stored. The feeding troughs were filled daily from these buckets. At the end of the trial, residuals in the troughs and buckets were weighed at a subgroup level (Systemwaage PCE TB 30, PCE Instruments, Meschede, Germany). The fresh drinking water for the storage tanks of the specific subgroups was weighed before filling the tanks daily. Sampling–Experiment 1. The lauric acid content in the contents of the crop, the gizzard, anterior small intestine (ASI; end of muscular stomach to diverticulum vitellinum), posterior small intestine (PSI; diverticulum vitellinum to caeca) and caeca were determined exactly 42 days (d0) after hatch (Analysis described in the section "Feed and chime analysis"). Experimental challenge and sampling–Experiment 2. Prior to the described experimental challenge, Campylobacter exclusion diagnosis had been performed in two stages. First, three days before the experimental challenge five chickens per subgroup (n = 150/450) had been tested by means of a cloacal swab (Cary Blair smear test system, Suesse Labortechnik GmbH & Co. KG, Gudensberg, Germany) regarding a possible excretion of C. jejuni. If these birds had been positive, the experiment would not have been carried out. This was a termination criterion for the approved animal experiment. It takes about three days to confirm the Campylobacter-free status. Therefore, the first C. jejuni analysis had to be carried out three days before starting the experimental challenge. To justify the continuation of the experiments, all birds (n = 450/450) were again sampled prior to the experimental challenge (on the same day). If a bird had been positive at this stage, the experiment could have been stopped three days after the experimental challenge, when results of sampling would have been confirmed. This procedure has to taken place to ensure absolutely comparable starting conditions, i.e. Campylobacter-free status as a result of the second pre-sampling. The experimental challenge with C. jejuni took place at d 21 in all subgroups. In each subgroup, three out of 15 broilers in a box were administered orally with a C. jejuni inoculum. When using pathogens with a low infection dose and a high tendency to spread and simultaneously keeping the birds in small groups, it is legally obliged to reduce the number of primary-infected birds to the lowest necessary level. This is preferable because the process of application of the pathogen can be seen as a burden. Therefore, only three out of 15 chickens were experimentally infected. In the case of natural infection in a flock it can also be assumed that the entry of the pathogen takes place at one location. Therefore, additionally the spread within the groups in case of partial infection is a particularly interesting parameter to test the efficiency of a dietetic concept as a model for the situation in practice. A direct comparison of the dietary concepts with respect to the quantitative excretion of Campylobacter was carried out exclusively by determining the number of Campylobacter in the excreta of primarily infected birds. A field strain of C. jejuni was used for the experimental challenge [28]. This isolate was identified as C. jejuni both culturally and mass-spectrometrically (MALDI-TOF MS) in a commercial laboratory (AniCon Labor GmbH, Hoeltinghausen, Germany). The advantage of this procedure is that only previously cultivated bacteria can be used for identification using MALDI-TOF. In our case, this means that we have also reliably identified the "infectious agent". Only one strain of Campylobacter was used for inoculation. This was done because muscle samples from the experiments should still be used for further questions [24]. Muscle samples from the experiment were spiked with a Campylobacter coli strain (Campylobacter coli strain DSM 4689). Lauric acid was present in higher concentrations in the muscle samples of birds offered the lauric acid supplement. In these in vitro experiments reduction of viable Campylobacter coli's was tested on the meat surface. In order to simplify the diagnosis of exclusion (possible contamination of the sample material with Campylobacter jejuni), only one pathogen was used in our inoculation model. The conserved strain for experimental inoculation was recultivated on solid selective culture media (mCCD agar; Oxoid Germany GmbH, Wesel, Germany). After incubation at 41.5°C in a microaerobic atmosphere for 43.5 hours, the challenge strain was used in its stationary growth phase (24 h to 48 h) for preparing the challenge inoculum. An isotonic 0.9% sodium chloride solution was used as the basis for the infection bouillon. A defined density of C. jejuni was adjusted (0.5 McFarland units corresponding to about 1 × 107 CFU C. jejuni per mL) using a densitometer (DEN 1B, biosan SIA, Riga, Latvia). To obtain a challenge dose of about 10,000 CFU/1 mL of challenge inoculum, the inoculum was further diluted with sodium chloride. Three parallel batches were prepared. For the experimental challenge, three out of 15 birds were randomly selected. Infection bouillon was administered orally by means of a button cannula (single-button cannula, sterile, 1.0×100 mm, Meiser Medical GmbH, Neuenstein, Germany). Each of the three identically prepared challenge inocula was used for only one bird per subgroup. In the experimental period, qualitative detection of C. jejuni took place on the day of experimental challenge (d-21), at further sampling points (d-19, d-17, d-14, d-7) and on the day of dissection (d0) in all birds (Fig 1). Quantitative detection of C. jejuni was done three times in seeder birds (three birds per subgroup) at d-19, d-10 and d-4. For excreta collection, the corresponding chickens were individually placed in purified, disinfected 10 L plastic buckets (ᴓ 26.5 cm) to collect fresh excreta. At dissection, samples of ceacal content were taken to analyse the counts of C. jejuni in this material. In sentinel birds (five birds per repetitions, housed in a separate box in the security level 2-flock) regular spotchecks were carried out on the excretion of C. jejuni. Dissection. Following the experimental period (d-28–d0), all chickens were dissected. Anaesthesia and killing of birds were carried out in accordance with EC 1099/2009. Anaesthesia was done by head stroke, after that the birds were bled. The contents of the different sections were removed under sterile conditions and placed in a screw cup (screw cup 100 mL, PP, Sarstedt AG & Co., Nuembrecht, Germany) for further analysis. Bacteriological analyses The qualitative bacteriological examination was based on the DIN EN ISO 10272–1:2006, taken from the official collection of analysis methods in accordance with § 64 LFBG. First, pre-enrichment was performed in a liquid selective nutrient medium (Bolton Boullion). For this purpose, 500 mL of a basic nutrient medium (Bolton Brothbase, VWR International GmbH, Darmstadt, Germany) were first heated to 50°C in a water bath (GFL Gesellschaft fuer Labortechnik GmbH, Burgwedel, Germany). Lyophilised additives (Modified Bolton Broth Selective Supplement, Oxoid Deutschland GmbH, Wesel, Germany) were resuspended in a mixture of 2.5 mL ethanol and 2.5 mL autoclaved water. Afterwards, the additives were first transferred to the base nutrient medium, 25 mL lysed horse blood (Oxoid Deutschland GmbH, Wesel, Germany) subsequently being added. The sample matrix to be examined was incubated in a one-to-nine ratio (sample:bolton-boullion) in sterile 5 mL tubes mounted with a vent cap (Sarstedt AG & Co., Nuembrecht, Germany). Incubation lasting 4 h at 37°C was followed by 44 h±4 h at 41.5°C in a microaerobic atmosphere (oxygen content of 5%±2%, carbon dioxide content of 10%±3%) in a CO2 incubator with O2 control (CB 160, BINDER GmbH, Tuttlingen, Germany). After enrichment, the samples were streaked onto two solid selective culture media (mCCD agar and Karmali agar; Oxoid Germany GmbH, Wesel, Germany) by sterile 10 μL inoculation loops. The incubation of the inoculated selective culture was carried out again for 44 h±4 h at 41.5°C in a microaerophilic atmosphere. Individual colonies were analysed to confirm the presence of Campylobacter. This was done by phase contrast microscopy (Distelkamp-Electronic, Kaiserslautern, Germany) and biochemical methods (apiCampy, bioMérieux SA, Marcy- l`Etoile, France). For quantitative bacteriological examination a 10-fold dilution series (0.5 g sample material in 4.5 mL of sterile Phosphate Buffered Saline—PBS) was made with PBS (Phosphate Buffered Saline, Oxoid Germany GmbH, Wesel, Germany). In duplicate, 100 μL of each dilution was plated onto mCCD agar (Oxoid Germany GmbH, Wesel, Germany). After incubation in a microaerophilic atmosphere for 44 h±4 h at 41.5° C, the colonies were counted and an average value from the two duplicate experiments was taken for calculating the CFU/g intestinal content. A diagnosis of exclusion concerning Salmonella spp. was performed as previously described [29]. Detection concerning coccidia was done weekly by an already described method [30]. Statistical analyses The statistical analyses were performed using the Statistical Analysis System for Windows, version 9.3, (SAS Institute Inc., Cary, North Carolina, USA). The group comparison for lauric acid concentrations in the gut contents was performed by a one-way analysis of variance (ANOVA) for independent samples on level of the different intestinal sections. Differences in concentration between the different sections of the gastrointestinal tract at group level were examined by means of one-way analyses of variance for repeated measures. The performance data were analysed by means of analyses of variance for independent samples with regard to the influence factors “diet” at the level of the genetic breed x diet, “age” and “genetic breed”. The Ryan-Einot-Gabriel-Welsch multiple Range-Test was used for the multiple pairwise means comparisons. The distributions of the residuals from the linear models belonging to the analyses of variance were close to the normal one. The qualitative target values concerning C. jejuni prevalence were assessed with Pearson’s Chi-square-Test for homogeneity and for low frequencies with Fisher’s exact test. For the statistical evaluation of counts of C. jejuni in excreta and caecal content samples, the data were logarithmised. The possible influence of the diet or of genetic breed on C. jejuni counts in the excreta of seeder birds was first determined by means of a one-way analysis of variance (ANOVA) for independent samples for the three different measurement times. Subsequently, the influence of time was determined by means of an analysis of variance for repeated measures. The counts of C. jejuni in the caecal content were analysed with respect to the factors “diet”, “age” and “genetic breed” by one-way analysis of variance (ANOVA) for independent samples. All statements of statistical significance are based upon p-values smaller than 0.05. This approach holds the comparisonwise error rate. Animals and housing The birds used in the experiment were supplied as day-old chicks directly from the hatcheries. The chicks of the genetics CobbSasso 175 (CS175; only genetic for experiment 1), Ross 308 (R308), and Hubbard JA 757 (Hb757) were obtained from BWE-Brueterei Weser Ems, Visbek, Germany. Male chicks of the Lohmann Brown-Classic (LBC-A42, LBC-A98; male; two age groups) and Lohmann Dual (LD) breeds were supplied by Lohmann Tierzucht GmbH, Cuxhaven, Germany. The experiments were divided into two parts: In the first part (Experiment 1), chickens of the genetics CS175 were used for analysing the concentrations of lauric acid in different parts of the gastrointestinal tract at dissection. The birds were given either a conventional complete diet or a lauric acid rich diet. In total, 32 chickens were kept in two different groups after the pre-experimental period of two weeks up to the end of day 42 of life. The experiment was conducted once. In the second part (Experiment 2), identical diets (without/with lauric acid supplement) were offered in birds of different breeds. For this second experiment chicks of the genetics R308, Hb757, LBC and LD were used. Therefore, effects on the spread of an experimentally induced C. jejuni infection were analysed depending on diet (without/with lauric acid supplement), age of the chickens (LBC-A42, LBC-A98) and on genetics (R308, Hb757, LBC, LD) during infection. For Experiment 2 (Table 1), four different breeds (R308, Hb757, LD, LBC) were reared under the same conditions in three independent repetitions (r = 3). Each breed consisted of 30 broilers which were randomly assigned to two subpopulations (15 birds, respectively). Only male birds from laying hybrids (LD and LBC) were used for the experiments. Birds of the LBC breed were also integrated into the experimental phase at different ages (LBC-A42, LBC-A98). Five birds per repetition, kept in a separate pen in the same room were used as sentinels. Therefore, the trials were based on a total of 465 chickens, conducted in three repetitions with 155 birds each. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 1. Experimental design showing distribution of birds based on breed, age and diet. https://doi.org/10.1371/journal.pone.0204483.t001 In the pre-experimental period (Fig 1), all birds were reared in identical floor pens littered with wood shavings. The pens were each equipped with an infrared lamp in order to reach a temperature at the outset of about 34–36°C. The temperature was lowered by about 1°C every two days, reaching a minimum temperature of about 20°C. The photoperiod beginning from d 4 was 16 h of light and 8 h of darkness during the whole trial. Download: PPT PowerPoint slide PNG larger image TIFF original image Fig 1. Schedule of the trial (Experiment 2) with actions, analyses and parameters in chickens of different breeds (R308 = Ross 308; Hb757 = Hubbard JA 757; LD = Lohmann Dual; LBC-A42 = Lohmann-Brown-Classic, dissection after 42 days; LBC-A98 = Lohmann-Brown-Classic, dissection after 98 days). https://doi.org/10.1371/journal.pone.0204483.g001 After the fourteen-day rearing phase, all chickens in groups R308, Hb757, LD and LBC-A42 were transferred from the rearing to the infection unit of the animal house (security level 2). The experimental period started about four weeks before dissection (d-28). Birds in group LBC-A98 had been purchased seven (trial 1) or eight (trials 2+3) weeks prior to the start of the experimental period at a greater age. Therefore, these birds were transferred after an extended rearing phase to the infection unit at an age of about 63 or 70 days. At this time, birds of all genetic breeds and ages were randomly subdivided into ten subgroups for each repetition. Groups received either a control (CON) or the experimental lauric acid rich diet (LA; Table 2). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 2. Ingredient composition of the different experimental diets during the different fattening phases. https://doi.org/10.1371/journal.pone.0204483.t002 During the experimental period (d-28–d0) the birds were kept on solid floor pens in groups of 15 birds (“subgroup”) up to the end of the experimental period. A maximum stocking density of 30 kg per square metre applied to all groups. Due to the use of different breeds, metabolic body mass was applied as the standard dimension. A stocking density of 30 kg per square metre corresponds to a metabolic body mass of 23.3 kg0.75 per square metre. Due to the expected final body weight of the different breeds at the time of the dissection, the size of the boxes was then established. The base area of the feeding trough and the water lines, 0.17 square metres, was added to the calculated box size. As a result, the subgroups of different breeds had boxes with varying degrees of floor space available (R308: 1.53 m2, Hb757: 1.21 m2, LD: 1.04 m2, LBC-A42: 0.59 m2, LBC-A98: 1.17 m2 [Experiment 1] and 1.25 m2 [Experiment 2]). Movable partition walls made of stainless steel at a height of 60 cm made it possible to adapt the floor space to the desired stocking density. The boxes were separated from each other by 80 cm high completely closed plastic walls on the other three sides. The boxes were 106 cm wide but varied in depth. Between adjacent boxes there was also a distance of 106 cm. Boxes were littered with wood shavings (1 kg/m2). Feeding regime and diet The diets used in the study were produced and delivered by a feed company producing compound diets (Best 3 Gefluegelernährung GmbH, Twistringen, Germany). The rearing phase was divided into a one-week starter phase with a conventional pelleted starter diet (starter) and a subsequent seven-day phase with a commercially available pelleted grower diet (grower). All diets were offered ad libitum. During the first three days additional feed was available (about 300 g/d) on so-called Chickpaper to get the birds accustomed to the diet. The different diets for the experimental period were designed in accordance with the recommendations for the energy and nutrient supply of the laying hens and fowls (broilers) of the Committee for Needs Standards of the Society for Nutritional Physiology [23]. The energy and nutrient content were comparable to the commercially available standard fattening diet (Table 3). The basic finisher feed for diets CON and LA was a common pellet diet which had been reduced by 2% in its fat content. In the CON groups, the diet was supplemented by 5% of a commercial standard fat (C 12 < 6%). In the LA groups, 5% fat enriched with palm kernel fatty acids including high levels of lauric acid (C 12 = 42–53%) was added as already described [24]. From the results of preliminary tests on the suitability of palm kernel fatty acids or combination of palm kernel fatty acids and capric acid and capric acid (data not shown), the use of a palm kernel product was preferred. The application amount was also determined in preliminary tests. Two different concentrations (2% and 5%) were tested. There was no negative effect on performance at the higher concentration. The higher concentration would also be the economically acceptable upper limit. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 3. Energy content and nutrient composition of the experimental diets during the different fattening phases. https://doi.org/10.1371/journal.pone.0204483.t003 Circular feeding troughs were used (Crown Poultry Feeders, Nelson, New Zealand). In the rearing phase water was offered ad libitum in double-cylinder plastic bell drinkers. Later, drinking lines equipped with Top Nipples with a drinking cup were used (Big Dutchman International GmbH, Vechta-Calveslage, Germany). The water was treated with chlorine containing product (Virbac Clean Pipe, VIRBAC Tierarzneimittel GmbH, Bad Oldesloe, Germany) at a concentration of 0.3 mg free chlorine/L to kill any C. jejuni in the drinking water. Feed and chyme analysis Diets were analysed by standard procedures in accordance with the official methods of the VDLUFA [25]. The analyses were always performed in duplicate. The dry matter content (DM) was determined by drying to the weight constancy at 103°C. The raw ash was analysed by means of incineration in the muffle furnace at 600°C for six hours. The total nitrogen content was determined by elemental analyser (Elementar, Hanau, Germany), which operates according to the principle of a catalytic tube combustion (DUMAS combustion method). Molecular nitrogen formed by reduction from nitric oxide was detected by a thermal conductivity detector. The nitrogen content was calculated with the device software. Therefore, the crude protein content of the sample was determined by multiplying with a constant factor of 6.25. The crude fat content was determined after acid digestion in the soxhlet apparatus. The content of crude fibre was determined after washing in dilute acids and alkalis. Starch determination was carried out polarimetrically (Polatronic E, Schmidt und Haensch GmbH & Co., Berlin, Germany). The sugar content was analysed in accordance with Luff-Schoorl method by titration with sodium thiosulphate. The mineral content was determined in accordance with the official methods [25] by atomic absorption spectrometry (Unicam Solaar 116, Thermo, Dreieich, Germany). Amino acids were determined by ion-exchange chromatography (AA analyser LC 3000, Biotronic, Maintal, Germany) and results evaluated in accordance with established methods [26]. Determining levels of medium and long chain fatty acids in the diet and intestinal content samples was carried out using established methods [27]. Exactly 200 mg of analytical material was placed in a glass tube. A methanol-hexane-tridecanoic-acid mixture was utilised as standard. Subsequently, acetyl chloride was added and the sample was heated, followed by the addition of potassium chloride solution. The measurement was carried out by gaschromatography (GC TRACE 1300, Thermo Scientific, Dreieich, Germany; SP-2560 Column, Supelco, Bellefonte, USA; carrier gas: nitrogen) after centrifugation with the superior hexane phase. Experimental design and sampling Performance parameters. In Experiment 1, the individual body weight (BW) of birds was determined (PCE TB 30, PCE Instruments, Meschede, Germany) at the beginning and at the end of the feeding phase (d-28, d0) and the average daily feed intake (ADFI) on a subgroup basis to determine average daily weight gains (ADWG) and the feed conversion ratio (FCR). In Experiment 2, the BW of the chickens was recorded individually at the start, at the time of experimental challenge and at the end of the experimental period (d-28, d-21 and d0). The ADFI was recorded at the level of the subgroup. Each subgroup had a 30 L polypropylene feed bucket into which the diet for the corresponding subgroup for the whole experimental period was stored. The feeding troughs were filled daily from these buckets. At the end of the trial, residuals in the troughs and buckets were weighed at a subgroup level (Systemwaage PCE TB 30, PCE Instruments, Meschede, Germany). The fresh drinking water for the storage tanks of the specific subgroups was weighed before filling the tanks daily. Sampling–Experiment 1. The lauric acid content in the contents of the crop, the gizzard, anterior small intestine (ASI; end of muscular stomach to diverticulum vitellinum), posterior small intestine (PSI; diverticulum vitellinum to caeca) and caeca were determined exactly 42 days (d0) after hatch (Analysis described in the section "Feed and chime analysis"). Experimental challenge and sampling–Experiment 2. Prior to the described experimental challenge, Campylobacter exclusion diagnosis had been performed in two stages. First, three days before the experimental challenge five chickens per subgroup (n = 150/450) had been tested by means of a cloacal swab (Cary Blair smear test system, Suesse Labortechnik GmbH & Co. KG, Gudensberg, Germany) regarding a possible excretion of C. jejuni. If these birds had been positive, the experiment would not have been carried out. This was a termination criterion for the approved animal experiment. It takes about three days to confirm the Campylobacter-free status. Therefore, the first C. jejuni analysis had to be carried out three days before starting the experimental challenge. To justify the continuation of the experiments, all birds (n = 450/450) were again sampled prior to the experimental challenge (on the same day). If a bird had been positive at this stage, the experiment could have been stopped three days after the experimental challenge, when results of sampling would have been confirmed. This procedure has to taken place to ensure absolutely comparable starting conditions, i.e. Campylobacter-free status as a result of the second pre-sampling. The experimental challenge with C. jejuni took place at d 21 in all subgroups. In each subgroup, three out of 15 broilers in a box were administered orally with a C. jejuni inoculum. When using pathogens with a low infection dose and a high tendency to spread and simultaneously keeping the birds in small groups, it is legally obliged to reduce the number of primary-infected birds to the lowest necessary level. This is preferable because the process of application of the pathogen can be seen as a burden. Therefore, only three out of 15 chickens were experimentally infected. In the case of natural infection in a flock it can also be assumed that the entry of the pathogen takes place at one location. Therefore, additionally the spread within the groups in case of partial infection is a particularly interesting parameter to test the efficiency of a dietetic concept as a model for the situation in practice. A direct comparison of the dietary concepts with respect to the quantitative excretion of Campylobacter was carried out exclusively by determining the number of Campylobacter in the excreta of primarily infected birds. A field strain of C. jejuni was used for the experimental challenge [28]. This isolate was identified as C. jejuni both culturally and mass-spectrometrically (MALDI-TOF MS) in a commercial laboratory (AniCon Labor GmbH, Hoeltinghausen, Germany). The advantage of this procedure is that only previously cultivated bacteria can be used for identification using MALDI-TOF. In our case, this means that we have also reliably identified the "infectious agent". Only one strain of Campylobacter was used for inoculation. This was done because muscle samples from the experiments should still be used for further questions [24]. Muscle samples from the experiment were spiked with a Campylobacter coli strain (Campylobacter coli strain DSM 4689). Lauric acid was present in higher concentrations in the muscle samples of birds offered the lauric acid supplement. In these in vitro experiments reduction of viable Campylobacter coli's was tested on the meat surface. In order to simplify the diagnosis of exclusion (possible contamination of the sample material with Campylobacter jejuni), only one pathogen was used in our inoculation model. The conserved strain for experimental inoculation was recultivated on solid selective culture media (mCCD agar; Oxoid Germany GmbH, Wesel, Germany). After incubation at 41.5°C in a microaerobic atmosphere for 43.5 hours, the challenge strain was used in its stationary growth phase (24 h to 48 h) for preparing the challenge inoculum. An isotonic 0.9% sodium chloride solution was used as the basis for the infection bouillon. A defined density of C. jejuni was adjusted (0.5 McFarland units corresponding to about 1 × 107 CFU C. jejuni per mL) using a densitometer (DEN 1B, biosan SIA, Riga, Latvia). To obtain a challenge dose of about 10,000 CFU/1 mL of challenge inoculum, the inoculum was further diluted with sodium chloride. Three parallel batches were prepared. For the experimental challenge, three out of 15 birds were randomly selected. Infection bouillon was administered orally by means of a button cannula (single-button cannula, sterile, 1.0×100 mm, Meiser Medical GmbH, Neuenstein, Germany). Each of the three identically prepared challenge inocula was used for only one bird per subgroup. In the experimental period, qualitative detection of C. jejuni took place on the day of experimental challenge (d-21), at further sampling points (d-19, d-17, d-14, d-7) and on the day of dissection (d0) in all birds (Fig 1). Quantitative detection of C. jejuni was done three times in seeder birds (three birds per subgroup) at d-19, d-10 and d-4. For excreta collection, the corresponding chickens were individually placed in purified, disinfected 10 L plastic buckets (ᴓ 26.5 cm) to collect fresh excreta. At dissection, samples of ceacal content were taken to analyse the counts of C. jejuni in this material. In sentinel birds (five birds per repetitions, housed in a separate box in the security level 2-flock) regular spotchecks were carried out on the excretion of C. jejuni. Dissection. Following the experimental period (d-28–d0), all chickens were dissected. Anaesthesia and killing of birds were carried out in accordance with EC 1099/2009. Anaesthesia was done by head stroke, after that the birds were bled. The contents of the different sections were removed under sterile conditions and placed in a screw cup (screw cup 100 mL, PP, Sarstedt AG & Co., Nuembrecht, Germany) for further analysis. Performance parameters. In Experiment 1, the individual body weight (BW) of birds was determined (PCE TB 30, PCE Instruments, Meschede, Germany) at the beginning and at the end of the feeding phase (d-28, d0) and the average daily feed intake (ADFI) on a subgroup basis to determine average daily weight gains (ADWG) and the feed conversion ratio (FCR). In Experiment 2, the BW of the chickens was recorded individually at the start, at the time of experimental challenge and at the end of the experimental period (d-28, d-21 and d0). The ADFI was recorded at the level of the subgroup. Each subgroup had a 30 L polypropylene feed bucket into which the diet for the corresponding subgroup for the whole experimental period was stored. The feeding troughs were filled daily from these buckets. At the end of the trial, residuals in the troughs and buckets were weighed at a subgroup level (Systemwaage PCE TB 30, PCE Instruments, Meschede, Germany). The fresh drinking water for the storage tanks of the specific subgroups was weighed before filling the tanks daily. Sampling–Experiment 1. The lauric acid content in the contents of the crop, the gizzard, anterior small intestine (ASI; end of muscular stomach to diverticulum vitellinum), posterior small intestine (PSI; diverticulum vitellinum to caeca) and caeca were determined exactly 42 days (d0) after hatch (Analysis described in the section "Feed and chime analysis"). Experimental challenge and sampling–Experiment 2. Prior to the described experimental challenge, Campylobacter exclusion diagnosis had been performed in two stages. First, three days before the experimental challenge five chickens per subgroup (n = 150/450) had been tested by means of a cloacal swab (Cary Blair smear test system, Suesse Labortechnik GmbH & Co. KG, Gudensberg, Germany) regarding a possible excretion of C. jejuni. If these birds had been positive, the experiment would not have been carried out. This was a termination criterion for the approved animal experiment. It takes about three days to confirm the Campylobacter-free status. Therefore, the first C. jejuni analysis had to be carried out three days before starting the experimental challenge. To justify the continuation of the experiments, all birds (n = 450/450) were again sampled prior to the experimental challenge (on the same day). If a bird had been positive at this stage, the experiment could have been stopped three days after the experimental challenge, when results of sampling would have been confirmed. This procedure has to taken place to ensure absolutely comparable starting conditions, i.e. Campylobacter-free status as a result of the second pre-sampling. The experimental challenge with C. jejuni took place at d 21 in all subgroups. In each subgroup, three out of 15 broilers in a box were administered orally with a C. jejuni inoculum. When using pathogens with a low infection dose and a high tendency to spread and simultaneously keeping the birds in small groups, it is legally obliged to reduce the number of primary-infected birds to the lowest necessary level. This is preferable because the process of application of the pathogen can be seen as a burden. Therefore, only three out of 15 chickens were experimentally infected. In the case of natural infection in a flock it can also be assumed that the entry of the pathogen takes place at one location. Therefore, additionally the spread within the groups in case of partial infection is a particularly interesting parameter to test the efficiency of a dietetic concept as a model for the situation in practice. A direct comparison of the dietary concepts with respect to the quantitative excretion of Campylobacter was carried out exclusively by determining the number of Campylobacter in the excreta of primarily infected birds. A field strain of C. jejuni was used for the experimental challenge [28]. This isolate was identified as C. jejuni both culturally and mass-spectrometrically (MALDI-TOF MS) in a commercial laboratory (AniCon Labor GmbH, Hoeltinghausen, Germany). The advantage of this procedure is that only previously cultivated bacteria can be used for identification using MALDI-TOF. In our case, this means that we have also reliably identified the "infectious agent". Only one strain of Campylobacter was used for inoculation. This was done because muscle samples from the experiments should still be used for further questions [24]. Muscle samples from the experiment were spiked with a Campylobacter coli strain (Campylobacter coli strain DSM 4689). Lauric acid was present in higher concentrations in the muscle samples of birds offered the lauric acid supplement. In these in vitro experiments reduction of viable Campylobacter coli's was tested on the meat surface. In order to simplify the diagnosis of exclusion (possible contamination of the sample material with Campylobacter jejuni), only one pathogen was used in our inoculation model. The conserved strain for experimental inoculation was recultivated on solid selective culture media (mCCD agar; Oxoid Germany GmbH, Wesel, Germany). After incubation at 41.5°C in a microaerobic atmosphere for 43.5 hours, the challenge strain was used in its stationary growth phase (24 h to 48 h) for preparing the challenge inoculum. An isotonic 0.9% sodium chloride solution was used as the basis for the infection bouillon. A defined density of C. jejuni was adjusted (0.5 McFarland units corresponding to about 1 × 107 CFU C. jejuni per mL) using a densitometer (DEN 1B, biosan SIA, Riga, Latvia). To obtain a challenge dose of about 10,000 CFU/1 mL of challenge inoculum, the inoculum was further diluted with sodium chloride. Three parallel batches were prepared. For the experimental challenge, three out of 15 birds were randomly selected. Infection bouillon was administered orally by means of a button cannula (single-button cannula, sterile, 1.0×100 mm, Meiser Medical GmbH, Neuenstein, Germany). Each of the three identically prepared challenge inocula was used for only one bird per subgroup. In the experimental period, qualitative detection of C. jejuni took place on the day of experimental challenge (d-21), at further sampling points (d-19, d-17, d-14, d-7) and on the day of dissection (d0) in all birds (Fig 1). Quantitative detection of C. jejuni was done three times in seeder birds (three birds per subgroup) at d-19, d-10 and d-4. For excreta collection, the corresponding chickens were individually placed in purified, disinfected 10 L plastic buckets (ᴓ 26.5 cm) to collect fresh excreta. At dissection, samples of ceacal content were taken to analyse the counts of C. jejuni in this material. In sentinel birds (five birds per repetitions, housed in a separate box in the security level 2-flock) regular spotchecks were carried out on the excretion of C. jejuni. Dissection. Following the experimental period (d-28–d0), all chickens were dissected. Anaesthesia and killing of birds were carried out in accordance with EC 1099/2009. Anaesthesia was done by head stroke, after that the birds were bled. The contents of the different sections were removed under sterile conditions and placed in a screw cup (screw cup 100 mL, PP, Sarstedt AG & Co., Nuembrecht, Germany) for further analysis. Bacteriological analyses The qualitative bacteriological examination was based on the DIN EN ISO 10272–1:2006, taken from the official collection of analysis methods in accordance with § 64 LFBG. First, pre-enrichment was performed in a liquid selective nutrient medium (Bolton Boullion). For this purpose, 500 mL of a basic nutrient medium (Bolton Brothbase, VWR International GmbH, Darmstadt, Germany) were first heated to 50°C in a water bath (GFL Gesellschaft fuer Labortechnik GmbH, Burgwedel, Germany). Lyophilised additives (Modified Bolton Broth Selective Supplement, Oxoid Deutschland GmbH, Wesel, Germany) were resuspended in a mixture of 2.5 mL ethanol and 2.5 mL autoclaved water. Afterwards, the additives were first transferred to the base nutrient medium, 25 mL lysed horse blood (Oxoid Deutschland GmbH, Wesel, Germany) subsequently being added. The sample matrix to be examined was incubated in a one-to-nine ratio (sample:bolton-boullion) in sterile 5 mL tubes mounted with a vent cap (Sarstedt AG & Co., Nuembrecht, Germany). Incubation lasting 4 h at 37°C was followed by 44 h±4 h at 41.5°C in a microaerobic atmosphere (oxygen content of 5%±2%, carbon dioxide content of 10%±3%) in a CO2 incubator with O2 control (CB 160, BINDER GmbH, Tuttlingen, Germany). After enrichment, the samples were streaked onto two solid selective culture media (mCCD agar and Karmali agar; Oxoid Germany GmbH, Wesel, Germany) by sterile 10 μL inoculation loops. The incubation of the inoculated selective culture was carried out again for 44 h±4 h at 41.5°C in a microaerophilic atmosphere. Individual colonies were analysed to confirm the presence of Campylobacter. This was done by phase contrast microscopy (Distelkamp-Electronic, Kaiserslautern, Germany) and biochemical methods (apiCampy, bioMérieux SA, Marcy- l`Etoile, France). For quantitative bacteriological examination a 10-fold dilution series (0.5 g sample material in 4.5 mL of sterile Phosphate Buffered Saline—PBS) was made with PBS (Phosphate Buffered Saline, Oxoid Germany GmbH, Wesel, Germany). In duplicate, 100 μL of each dilution was plated onto mCCD agar (Oxoid Germany GmbH, Wesel, Germany). After incubation in a microaerophilic atmosphere for 44 h±4 h at 41.5° C, the colonies were counted and an average value from the two duplicate experiments was taken for calculating the CFU/g intestinal content. A diagnosis of exclusion concerning Salmonella spp. was performed as previously described [29]. Detection concerning coccidia was done weekly by an already described method [30]. Statistical analyses The statistical analyses were performed using the Statistical Analysis System for Windows, version 9.3, (SAS Institute Inc., Cary, North Carolina, USA). The group comparison for lauric acid concentrations in the gut contents was performed by a one-way analysis of variance (ANOVA) for independent samples on level of the different intestinal sections. Differences in concentration between the different sections of the gastrointestinal tract at group level were examined by means of one-way analyses of variance for repeated measures. The performance data were analysed by means of analyses of variance for independent samples with regard to the influence factors “diet” at the level of the genetic breed x diet, “age” and “genetic breed”. The Ryan-Einot-Gabriel-Welsch multiple Range-Test was used for the multiple pairwise means comparisons. The distributions of the residuals from the linear models belonging to the analyses of variance were close to the normal one. The qualitative target values concerning C. jejuni prevalence were assessed with Pearson’s Chi-square-Test for homogeneity and for low frequencies with Fisher’s exact test. For the statistical evaluation of counts of C. jejuni in excreta and caecal content samples, the data were logarithmised. The possible influence of the diet or of genetic breed on C. jejuni counts in the excreta of seeder birds was first determined by means of a one-way analysis of variance (ANOVA) for independent samples for the three different measurement times. Subsequently, the influence of time was determined by means of an analysis of variance for repeated measures. The counts of C. jejuni in the caecal content were analysed with respect to the factors “diet”, “age” and “genetic breed” by one-way analysis of variance (ANOVA) for independent samples. All statements of statistical significance are based upon p-values smaller than 0.05. This approach holds the comparisonwise error rate. Results No mortality or animal health concern were recorded. Additionally, no samples were positive for Salmonella spp. or coccidia. Performance parameters Experiment 1. At the end of the 42-day rearing period, the chickens showed a BW of 2150±321 g (CON) and 2035±313 g (LA), respectively (FCR–CON: 1.97, LA: 1.90). Experiment 2. The BW and the ADWG at different time points as well as the FCR and the mortality showed no significant differences depending on diet within the specific genetic breed, with one exception among the older birds of the breed LBC-A98. Chickens which were offered a complete diet containing higher levels of lauric acid had a significantly lower weight gain in all analysed periods (Table 4). Significant differences in BW as a function of age were present (LBC-A98>LBC-A42). The ADWG for LBC-A98 was significantly lower. The FCR was significantly higher for the older birds of the genetic breed LBC-A98 (Table 5). Depending on the genetic breed, there were significant differences between all breeds depending on BW and ADWG at different time points in the following descending order: R308>Hb757>LD>LBC-A42. These differences existed at the beginning of the experimental period as well as at the end (Table 5). The FCR was significantly the highest for the group R308, the lowest for LBC-A42 and intermediate for Hb757 and LD depending on the genetic breed. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 4. Growth performance, average weight gain, feed conversion ratio and mortality rate of poultry of different genetic breeds fed a diet without or with palm kernel fatty acids (n = 45 birds per breed and diet) in the last 28 days before dissection. https://doi.org/10.1371/journal.pone.0204483.t004 Download: PPT PowerPoint slide PNG larger image TIFF original image Table 5. Growth performance, average weight gain and feed conversion ratio of poultry of different genetic breeds (n = 90 per breed) and different ages (n = 90 per age group) in the last 28 days before dissection. https://doi.org/10.1371/journal.pone.0204483.t005 Lauric acid concentration in the gastrointestinal tract In Experiment 1, the uptake of the diet containing lauric acid in relation to the control diet resulted in significantly higher lauric acid concentrations in the content of the respective section in broilers of breed CS175 (Fig 2). Download: PPT PowerPoint slide PNG larger image TIFF original image Fig 2. Concentration of lauric acid in different sections of the gastrointestinal tract of broiler chickens (n = 5/group; genetic breed: CobbSasso 175; Crop = content of the crop; Giz = content of the gizzard; ASI = content of the anterior small intestine; PSI = content of the posterior small intestine; Cae = content of the caecum; lowercase letters(a,b) describe differences between concentrations in lauric acid at one location at P<0.05; uppercase letters (A,B) describe differences between concentrations in lauric acid between locations depending on different diets at P<0.05. https://doi.org/10.1371/journal.pone.0204483.g002 The concentrations were significantly higher in the crop (CON: 0.22±0.01; LA: 6.41±2.34 g/kg fresh matter) and in the gizzard (CON: 0.19±0.05; LA: 5.53±1.91 g/kg fresh matter), anterior small intestine (ASI; CON: 0.07±0.04, LA: 1.68±0.26 g/kg fresh matter), posterior small intestine (PSI; CON: 0.03±0.01, LA: 0.88±0.39 g/kg fresh matter) and caecum (CON: 0.06±0.04; LA: 0.11±0.04 g/kg fresh matter). Campylobacter excretion The inocula for the experimental challenge contained an average of 4.46±0.35 log10 CFU C. jejuni per challenge dose (1 mL). Before and at the time of the experimental challenge (d-21), all chickens in the experiment were C. jejuni negative in cloacal swabs (N = 450). Sentinel birds (N = 15) remained negative during the whole trial. Seeder birds in the 30 experimental subgroups were inoculated at d 21 before dissection. Already two days after this challenge, an excretion of C. jejuni could be seen (Table 6). At this day (d-19), the number of chickens with a positive result concerning cloacal sampling was significantly higher in the control group receiving the CON diet (CON: 110/225 C. jejuni positive; LA: 89/225 C. jejuni positive; P = 0.0462). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 6. Prevalence of Campylobacter jejuni positive cloacal swabs depending on diet, age and genetic breeds after experimental challenge in poultry 21 days (-21 to 0) before dissection. https://doi.org/10.1371/journal.pone.0204483.t006 The number of C. jejuni positive cloacal swab samples was significantly different depending on the age of the birds (LBC-A42, LBC-A98) 19 days before dissection. The prevalence was significantly higher in older birds (LBC-A42: 34/90 C. jejuni positive; LBC-A98: 55/90 C. jejuni positive; P = 0.0017). On the day of dissection, the results were contrary because 30 out of 90 birds of LBC-A98 were C. jejuni negative, whereas only one bird of LBC-A42 showed a negative test result in the cloacal swab (P<0.0001). At the end of the experiment (dissection: d0), significant differences were found depending on genetics. Out of a total of 360 birds, 11 cloacal swabs were C. jejuni negative in direct detection. Of these, 72.7% swabs belonged to chickens of genetics LD (P = 0.0059, Table 6). The number of colony-forming units of C. jejuni in the excreta samples of experimentally infected chickens (seeder birds) did not differ depending on the feeding regime (CON, LA; Table 7). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 7. Quantitative counts of C. jejuni in excreta samples [log10 CFU/g] of experimentally infected birds depending on diet and age. https://doi.org/10.1371/journal.pone.0204483.t007 Two days after successful experimental challenge (d-19), the excretion of C. jejuni with the excreta in older birds was significantly higher (LBC-A42: 3.30±2.68 log10 CFU/g; LBC-A98: 5.24±1.56 log10 CFU/g). At the tenth (d-10) and fourth day (d-4) before dissection, however, the excretion of the older birds was significantly lower. In particular, immediately before dissection the seeder birds of LBC-A98 showed significantly lower numbers of C. jejuni in the excreta (LBC-A42: 3.77±2.02 log10 CFU/g; LBC-A98: 1.72±1.87 log10 CFU/g), resulting in differences of Δlog10 CFU/g = 2.05. The quantitative excretion over time in comparison to the two age groups reached a maximum in excretion at second sampling (d-10) in the younger birds (LBC-A42). In older birds of the same genetic breed (LBC-A98), however, excretion reduced significantly over time (Table 7). The excretion of C. jejuni with the excreta differed only just before the dissection (d-4) between the genetic breeds (Table 8). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 8. Quantitative counts of C. jejuni in excreta samples [log10 CFU/g] of experimentally infected birds depending on genetic breed. https://doi.org/10.1371/journal.pone.0204483.t008 The experimentally infected birds of the Hb757 breed showed a nearly two log step (Hb757: 5.62±0.90 log10 CFU/g; LBC-A42: 3.77±2.02 log10 CFU/g) higher excretion than birds of the LBC-A42 breed. Within the respective breeds, there were differences depending on the time of the sampling after experimental challenge. In birds off the R308 and Hb757 breeds, the excretion was less pronounced shortly after experimental challenge (d-19), whereas in birds of the laying breed (LBC-A42) the excretion was significantly the highest at the mean sampling point (d-10). There was no significant effect of diet on the number of C. jejuni in the caecal content, even when comparing the feeding concepts within the genetic breeds (Table 9). Nonetheless, the Campylobacter counts in the caecum differed significantly depending on the age of the chickens (P<0.0001). The LBC-A98 chickens had significantly lower numbers of C. jejuni in the caecum (6.66±1.43 log10 CFU/g). The difference to LBC-A42 amounted to 1.91 log10 CFU/g so that these groups differed by almost 2 log steps. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 9. Quantitative counts of C. jejuni in caecal content samples [log10 CFU/g] of experimentally infected birds depending on diet and age. https://doi.org/10.1371/journal.pone.0204483.t009 Between the breeds, there were no significant differences in the number of C. jejuni in the caecal content of the birds (Table 10). On average, 8.46±0.62 log10 CFU/g C. jejuni were present in the caecal content. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 10. Quantitative counts of C jejuni in caecal content samples [log10 CFU/g] of experimentally infected birds depending on genetic breed. https://doi.org/10.1371/journal.pone.0204483.t010 Performance parameters Experiment 1. At the end of the 42-day rearing period, the chickens showed a BW of 2150±321 g (CON) and 2035±313 g (LA), respectively (FCR–CON: 1.97, LA: 1.90). Experiment 2. The BW and the ADWG at different time points as well as the FCR and the mortality showed no significant differences depending on diet within the specific genetic breed, with one exception among the older birds of the breed LBC-A98. Chickens which were offered a complete diet containing higher levels of lauric acid had a significantly lower weight gain in all analysed periods (Table 4). Significant differences in BW as a function of age were present (LBC-A98>LBC-A42). The ADWG for LBC-A98 was significantly lower. The FCR was significantly higher for the older birds of the genetic breed LBC-A98 (Table 5). Depending on the genetic breed, there were significant differences between all breeds depending on BW and ADWG at different time points in the following descending order: R308>Hb757>LD>LBC-A42. These differences existed at the beginning of the experimental period as well as at the end (Table 5). The FCR was significantly the highest for the group R308, the lowest for LBC-A42 and intermediate for Hb757 and LD depending on the genetic breed. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 4. Growth performance, average weight gain, feed conversion ratio and mortality rate of poultry of different genetic breeds fed a diet without or with palm kernel fatty acids (n = 45 birds per breed and diet) in the last 28 days before dissection. https://doi.org/10.1371/journal.pone.0204483.t004 Download: PPT PowerPoint slide PNG larger image TIFF original image Table 5. Growth performance, average weight gain and feed conversion ratio of poultry of different genetic breeds (n = 90 per breed) and different ages (n = 90 per age group) in the last 28 days before dissection. https://doi.org/10.1371/journal.pone.0204483.t005 Experiment 1. At the end of the 42-day rearing period, the chickens showed a BW of 2150±321 g (CON) and 2035±313 g (LA), respectively (FCR–CON: 1.97, LA: 1.90). Experiment 2. The BW and the ADWG at different time points as well as the FCR and the mortality showed no significant differences depending on diet within the specific genetic breed, with one exception among the older birds of the breed LBC-A98. Chickens which were offered a complete diet containing higher levels of lauric acid had a significantly lower weight gain in all analysed periods (Table 4). Significant differences in BW as a function of age were present (LBC-A98>LBC-A42). The ADWG for LBC-A98 was significantly lower. The FCR was significantly higher for the older birds of the genetic breed LBC-A98 (Table 5). Depending on the genetic breed, there were significant differences between all breeds depending on BW and ADWG at different time points in the following descending order: R308>Hb757>LD>LBC-A42. These differences existed at the beginning of the experimental period as well as at the end (Table 5). The FCR was significantly the highest for the group R308, the lowest for LBC-A42 and intermediate for Hb757 and LD depending on the genetic breed. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 4. Growth performance, average weight gain, feed conversion ratio and mortality rate of poultry of different genetic breeds fed a diet without or with palm kernel fatty acids (n = 45 birds per breed and diet) in the last 28 days before dissection. https://doi.org/10.1371/journal.pone.0204483.t004 Download: PPT PowerPoint slide PNG larger image TIFF original image Table 5. Growth performance, average weight gain and feed conversion ratio of poultry of different genetic breeds (n = 90 per breed) and different ages (n = 90 per age group) in the last 28 days before dissection. https://doi.org/10.1371/journal.pone.0204483.t005 Lauric acid concentration in the gastrointestinal tract In Experiment 1, the uptake of the diet containing lauric acid in relation to the control diet resulted in significantly higher lauric acid concentrations in the content of the respective section in broilers of breed CS175 (Fig 2). Download: PPT PowerPoint slide PNG larger image TIFF original image Fig 2. Concentration of lauric acid in different sections of the gastrointestinal tract of broiler chickens (n = 5/group; genetic breed: CobbSasso 175; Crop = content of the crop; Giz = content of the gizzard; ASI = content of the anterior small intestine; PSI = content of the posterior small intestine; Cae = content of the caecum; lowercase letters(a,b) describe differences between concentrations in lauric acid at one location at P<0.05; uppercase letters (A,B) describe differences between concentrations in lauric acid between locations depending on different diets at P<0.05. https://doi.org/10.1371/journal.pone.0204483.g002 The concentrations were significantly higher in the crop (CON: 0.22±0.01; LA: 6.41±2.34 g/kg fresh matter) and in the gizzard (CON: 0.19±0.05; LA: 5.53±1.91 g/kg fresh matter), anterior small intestine (ASI; CON: 0.07±0.04, LA: 1.68±0.26 g/kg fresh matter), posterior small intestine (PSI; CON: 0.03±0.01, LA: 0.88±0.39 g/kg fresh matter) and caecum (CON: 0.06±0.04; LA: 0.11±0.04 g/kg fresh matter). Campylobacter excretion The inocula for the experimental challenge contained an average of 4.46±0.35 log10 CFU C. jejuni per challenge dose (1 mL). Before and at the time of the experimental challenge (d-21), all chickens in the experiment were C. jejuni negative in cloacal swabs (N = 450). Sentinel birds (N = 15) remained negative during the whole trial. Seeder birds in the 30 experimental subgroups were inoculated at d 21 before dissection. Already two days after this challenge, an excretion of C. jejuni could be seen (Table 6). At this day (d-19), the number of chickens with a positive result concerning cloacal sampling was significantly higher in the control group receiving the CON diet (CON: 110/225 C. jejuni positive; LA: 89/225 C. jejuni positive; P = 0.0462). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 6. Prevalence of Campylobacter jejuni positive cloacal swabs depending on diet, age and genetic breeds after experimental challenge in poultry 21 days (-21 to 0) before dissection. https://doi.org/10.1371/journal.pone.0204483.t006 The number of C. jejuni positive cloacal swab samples was significantly different depending on the age of the birds (LBC-A42, LBC-A98) 19 days before dissection. The prevalence was significantly higher in older birds (LBC-A42: 34/90 C. jejuni positive; LBC-A98: 55/90 C. jejuni positive; P = 0.0017). On the day of dissection, the results were contrary because 30 out of 90 birds of LBC-A98 were C. jejuni negative, whereas only one bird of LBC-A42 showed a negative test result in the cloacal swab (P<0.0001). At the end of the experiment (dissection: d0), significant differences were found depending on genetics. Out of a total of 360 birds, 11 cloacal swabs were C. jejuni negative in direct detection. Of these, 72.7% swabs belonged to chickens of genetics LD (P = 0.0059, Table 6). The number of colony-forming units of C. jejuni in the excreta samples of experimentally infected chickens (seeder birds) did not differ depending on the feeding regime (CON, LA; Table 7). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 7. Quantitative counts of C. jejuni in excreta samples [log10 CFU/g] of experimentally infected birds depending on diet and age. https://doi.org/10.1371/journal.pone.0204483.t007 Two days after successful experimental challenge (d-19), the excretion of C. jejuni with the excreta in older birds was significantly higher (LBC-A42: 3.30±2.68 log10 CFU/g; LBC-A98: 5.24±1.56 log10 CFU/g). At the tenth (d-10) and fourth day (d-4) before dissection, however, the excretion of the older birds was significantly lower. In particular, immediately before dissection the seeder birds of LBC-A98 showed significantly lower numbers of C. jejuni in the excreta (LBC-A42: 3.77±2.02 log10 CFU/g; LBC-A98: 1.72±1.87 log10 CFU/g), resulting in differences of Δlog10 CFU/g = 2.05. The quantitative excretion over time in comparison to the two age groups reached a maximum in excretion at second sampling (d-10) in the younger birds (LBC-A42). In older birds of the same genetic breed (LBC-A98), however, excretion reduced significantly over time (Table 7). The excretion of C. jejuni with the excreta differed only just before the dissection (d-4) between the genetic breeds (Table 8). Download: PPT PowerPoint slide PNG larger image TIFF original image Table 8. Quantitative counts of C. jejuni in excreta samples [log10 CFU/g] of experimentally infected birds depending on genetic breed. https://doi.org/10.1371/journal.pone.0204483.t008 The experimentally infected birds of the Hb757 breed showed a nearly two log step (Hb757: 5.62±0.90 log10 CFU/g; LBC-A42: 3.77±2.02 log10 CFU/g) higher excretion than birds of the LBC-A42 breed. Within the respective breeds, there were differences depending on the time of the sampling after experimental challenge. In birds off the R308 and Hb757 breeds, the excretion was less pronounced shortly after experimental challenge (d-19), whereas in birds of the laying breed (LBC-A42) the excretion was significantly the highest at the mean sampling point (d-10). There was no significant effect of diet on the number of C. jejuni in the caecal content, even when comparing the feeding concepts within the genetic breeds (Table 9). Nonetheless, the Campylobacter counts in the caecum differed significantly depending on the age of the chickens (P<0.0001). The LBC-A98 chickens had significantly lower numbers of C. jejuni in the caecum (6.66±1.43 log10 CFU/g). The difference to LBC-A42 amounted to 1.91 log10 CFU/g so that these groups differed by almost 2 log steps. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 9. Quantitative counts of C. jejuni in caecal content samples [log10 CFU/g] of experimentally infected birds depending on diet and age. https://doi.org/10.1371/journal.pone.0204483.t009 Between the breeds, there were no significant differences in the number of C. jejuni in the caecal content of the birds (Table 10). On average, 8.46±0.62 log10 CFU/g C. jejuni were present in the caecal content. Download: PPT PowerPoint slide PNG larger image TIFF original image Table 10. Quantitative counts of C jejuni in caecal content samples [log10 CFU/g] of experimentally infected birds depending on genetic breed. https://doi.org/10.1371/journal.pone.0204483.t010 Discussion Bacteria of the genus Campylobacter spp. are the most common causes of bacterially induced diarrhoea in humans [31, 32]. For decades, poultry meat has been assumed to be the cause of the infection behind Campylobacter enteritis in humans [33, 34]. Currently, poultry products are still the most common source of infection for humans [34–36]. Intestinal colonisation of chickens results in faecal contamination of the carcasses during the slaughtering process [37, 38]. Therefore, a reduction in the prevalence and the level of excretion of C. jejuni is strived for at production level. Performance parameters Offering a lauric acid rich diet led to significant lower ADWGs in chickens of the LBC-A98 breed (Table 4). In a previous study, a significantly concentration-dependent reduced feed intake with the use of propionic, caprylic, caprine and lauric acids starting from a concentration of 30 g/kg diet was seen [39]. As a control, maize seed oil was used [39]. Thereby, lauric acid showed the greatest negative effect on ADFI (up to d 29: 5.9 g lower feed intake per g/kg lauric acid added to the diet) presuming the taste or the hormonal regulation of intestinal motility and appetite to be responsible for these observations [39]. Consistent with reduced feed intake, growth was lower with higher concentrations [39]. In the present study, the lauric acid rich diet had no effect of on the FCR. The lauric acid concentration in the present study might be too low for the diet to have any effect on performance parameters in general. For older birds (LBC-A98) taste sensitivity might be higher and therefore the feed intake decreases. Birds of the LBC line showed significant differences in performance parameters depending on age (Table 5). The body weight, the daily weight gains as well as the FCR were always significantly higher in the older birds. This observation can be explained by the natural, genetically determined growth curve under optimal husbandry conditions. The comparison of performance parameters depending on the genetic breed showed also significantly differences between all genetics. The R308 birds had always the highest body weight, the highest daily weight gains and the lowest FCR. The genetics HB757, LD and LBC-A42 followed in descending order. These observations can also be explained by the natural, genetically determined growth curve under optimal husbandry conditions. Lauric acid concentrations in the gastrointestinal tract Using a lauric acid rich complete diet with higher levels of palm kernel fats as opposed to administrating a control diet resulted in significantly higher lauric acid concentrations at all analysed sites (crop, gizzard, anterior small intestine, posterior small intestine, caecum; Fig 2) in the gastrointestinal contents of broilers. The lauric acid concentration was significantly higher in the proximal areas than in the distal areas. Nevertheless, the average lauric acid concentrations (0.11±0.04 g/kg) achieved in the caecum in the experimental group was the lowest compared to the concentrations in the more cranial parts of the gastrointestinal tract. Lauric acid is resorbed extremely well and incorporated into the muscles [24]. Nevertheless, the concentrations were higher than effective inhibitory concentrations in vitro [6]. Concentrations less than 0.10 mg/mL lauric acid were able to reduce the bacterial DNA synthesis of C. jejuni in in vitro studies [6]. The caecal and cloacal crypts are the localisation in the intestinal tract with the highest counts of C. jejuni along the gastrointestinal tract [40]. Therefore, an effect of lauric acid on Campylobacter is fundamentally possible when taken orally, especially during the passage on the way to the main colonisation site, the caecum. Effect of lauric acid supplementation on Campylobacter challenge An effect of lauric acid on C. jejuni requires the presence of the acid in significant concentrations at the main site of colonisation, the caecum. In the present study the highest concentrations of lauric acid in the gastrointestinal tract were demonstrated in the cranial parts (Fig 2). A direct effect of the lauric acid in cranial areas is therefore only to be assumed in the initial infection. In the present investigations, in the initial phase the spread of the infection was delayed (Table 6). The proportion of cloacal swabs with positive C. jejuni detection was significantly lower in those birds receiving a lauric acid-rich complete diet. On its way to the actual colonisation site, C. jejuni comes into contact with very high lauric acid concentrations in the anterior regions of the gastrointestinal tract. Therefore, in a short time-frame of 24 hours until establishment of the infection [41], an effect might be possible. Under conditions of infection, C. jejuni recedes into the mucus layer of the crypts[40] and becomes difficult to reach for antimicrobial acting substances [42]. Although the concentrations of lauric acid in the caecal content are comparable to the inhibitory concentrations in vitro [6], it remains questionable whether these low concentrations are effective in vivo, too. We found no differences concerning C. jejuni counts in excreta samples of experimentally infected birds (Table 7) or in the intestinal content of the caecal content depending on diet (Table 9). C. jejuni is primarily found in the mucus layer of the caecal and cloacal crypts when colonising the gastrointestinal tract [40]. Some of the substances identified as effective against Campylobacter in vitro were less effective in in vivo studies [42–44]. Initially, (experimental infection with C. jejuni VFU612, 106CFU/bird) caprylic acid had a significant effect on the diet of broilers (2.5 and 5 g/kg of diet) on reducing C. jejuni excretion (up to 1.8 log10 CFU/g; [45]). However, as in our study, the dietary concept did not lead to differences in caecal content on the day of dissection (d42). Palm kernel products also contain caprylic and capric acid. However, the concentrations used in our diets were very low (0.12% based on dry matter; Table 3). These concentrations are rather low compared to the literature. Supplementing the diet with 0.35% and 0.70% caprylic acid consistently decreased (P<0.05) the colonisation of C. jejuni in the chicken caeca compared with positive control treatment [46]. To conclude, offering a lauric acid rich diet only led to low concentrations of the acid in the substantial section caecum and cloaca. Therefore, downstream effects of resorption of the acid and therefore higher lauric acid concentrations in muscles might be of greater importance. Campylobacter load in breast meat of Ross 308 broilers receiving a lauric acid rich diet was reduced during six days of storage (4°C) from initially 5.9 log10 CFU/g to 3.5 log10 CFU/g (treatment) compared to 4.3 log10 CFU/g (control; P = 0.0295; [24]). Campylobacter–age effects From the results of the present study, it is apparent that the age of birds at the time of infection has a great influence on the frequency of the excretion of C. jejuni (Table 6). In older chickens of the laying breed (LBC-A98) the spreading of the colonisation was faster as was its disappearance. The C. jejuni numbers in excreta of LBC-A90 chickens ( log10 = 5,20±0,93 CFU/g) was also in the upper range of the C. jejuni numbers in broilers which are described as log 2–6 CFU/g excreta in the literature [40, 47]. Glünder [48] already showed that ten-week-old birds compared to four- and seven-week-old birds had a lower excretion. These observations coincide with our own results (Table 7). Young starlings were more frequently infected with C. jejuni compared to adult ones [49]. According to some authors, the probability of Campylobacter colonisation also increases with age [50–53]. However, the excretion is sometimes intermittent [54], but, on the other hand, numerically lower. This agrees with the investigations of Glünder [48] and our own investigations. The age of birds at the time point of challenge had an influence on the detection of C. jejuni in the caecum 21 days after experimental challenge in our seeder model (Table 9). The C. jejuni counts in the caecum of the LBC-A98 breed were significantly lower (ΔCFU/g = log101.91) than the C. jejuni number in the caecum of LBC-A42 chickens. The C. jejuni counts in the caecum of LBC-A42 chickens averaged at log108.46±0.62 CFU/g caecal content. These concentrations are in the upper range of the C. jejuni numbers described in the literature in the caecum of log10 = 5–8 CFU/g caecal content [37, 40, 55, 56]. The reason for the lower detection rates in certain age groups is discussed; the composition of caecal flora, the developmental status of the immune system as well as the maturity of the immune system being responsible for this [57]. Also, use of these protective bacteria in poultry production can greatly reduce carriage of C. jejuni within poultry [58]. This approach may be important in the present study. Campylobacter spp. is predominantly found in the mucus layer that lies within the crypts [40]. Campylobacter is chemotactically attracted by L-fucose in the mucin, using mucin itself as a substrate for growth [59] and replicates in the mucus [60]. It is known from previous studies that bacteria that have similar properties produce metabolites antagonistic to C. jejuni [58]. Occupying the same niche in chicks can prevent colonization of most chicks by C. jejuni [58]. In that study, hens with cloacal samples negative for C. jejuni were screened for isolates expressing inhibitory metabolites to C. jejuni and simultaneously use mucin as a sole substrate for their growth [58]. The older birds in the present study might also have been the host of a more competent intestinal flora. The relative mucin availability increases with age. Therefore, perhaps the older birds (LBC-A98) already had a flora that had long been adapted to the degradation of larger amounts of mucin. Thus, there may have been some competition between the resident microflora and C. jejuni after experimental infection which led to a lower prevalence and lower counts in the caecal content. Campylobacter–effects of genetic breed In the present investigations, an influence of the genetics on the Campylobacter prevalence (Table 6), but even more clearly on the amount of the excretion of Campylobacter with the excreta could be demonstrated (Table 8). The mean logarithmic Campylobacter numbers in the excreta of the LD birds and of the laying hybrids LBC-A42 showed significant differences to the two broiler breeds R308 and Hb757 at the end of the experimental period. For LBC-A42, these differences amounted to almost 2 log steps (ΔCFU/g = log 1.85) compared to the Hb757 breed. However, the LD breed showed the lowest Campylobacter prevalence 21 days after experimental challenge. From the literature, a link between genetic breed and Campylobacter prevalence in the group and bacterial counts of C. jejuni in the caecum is demonstrated [61–63]. Modern, fast-growing breeds responded with a strong inflammatory response to C. jejuni infections [19]. This was associated with a negative effect on the function of the T-lymphocytes, which led to a reduced immune regulation and damage to the intestinal mucosa with subsequent diarrhoea [19]. This relationship is consistent with our findings. On the other hand, when comparing a broiler and a laying genetic (Ross 308 versus Lohmann Selected Leghorn), 14 days after experimental infection (day one of life), there were significantly higher counts of C. jejuni in the caecum of the laying breed [64]. However, the sample size (n = 6 per group) was very small [64]. Even if the age is identical, it may be necessary to consider indirect effects of breed. For example, mucin concentrations also depend on the relative levels of protein uptake [65], and thus may have an effect on the C. jejuni infection dynamics. Performance parameters Offering a lauric acid rich diet led to significant lower ADWGs in chickens of the LBC-A98 breed (Table 4). In a previous study, a significantly concentration-dependent reduced feed intake with the use of propionic, caprylic, caprine and lauric acids starting from a concentration of 30 g/kg diet was seen [39]. As a control, maize seed oil was used [39]. Thereby, lauric acid showed the greatest negative effect on ADFI (up to d 29: 5.9 g lower feed intake per g/kg lauric acid added to the diet) presuming the taste or the hormonal regulation of intestinal motility and appetite to be responsible for these observations [39]. Consistent with reduced feed intake, growth was lower with higher concentrations [39]. In the present study, the lauric acid rich diet had no effect of on the FCR. The lauric acid concentration in the present study might be too low for the diet to have any effect on performance parameters in general. For older birds (LBC-A98) taste sensitivity might be higher and therefore the feed intake decreases. Birds of the LBC line showed significant differences in performance parameters depending on age (Table 5). The body weight, the daily weight gains as well as the FCR were always significantly higher in the older birds. This observation can be explained by the natural, genetically determined growth curve under optimal husbandry conditions. The comparison of performance parameters depending on the genetic breed showed also significantly differences between all genetics. The R308 birds had always the highest body weight, the highest daily weight gains and the lowest FCR. The genetics HB757, LD and LBC-A42 followed in descending order. These observations can also be explained by the natural, genetically determined growth curve under optimal husbandry conditions. Lauric acid concentrations in the gastrointestinal tract Using a lauric acid rich complete diet with higher levels of palm kernel fats as opposed to administrating a control diet resulted in significantly higher lauric acid concentrations at all analysed sites (crop, gizzard, anterior small intestine, posterior small intestine, caecum; Fig 2) in the gastrointestinal contents of broilers. The lauric acid concentration was significantly higher in the proximal areas than in the distal areas. Nevertheless, the average lauric acid concentrations (0.11±0.04 g/kg) achieved in the caecum in the experimental group was the lowest compared to the concentrations in the more cranial parts of the gastrointestinal tract. Lauric acid is resorbed extremely well and incorporated into the muscles [24]. Nevertheless, the concentrations were higher than effective inhibitory concentrations in vitro [6]. Concentrations less than 0.10 mg/mL lauric acid were able to reduce the bacterial DNA synthesis of C. jejuni in in vitro studies [6]. The caecal and cloacal crypts are the localisation in the intestinal tract with the highest counts of C. jejuni along the gastrointestinal tract [40]. Therefore, an effect of lauric acid on Campylobacter is fundamentally possible when taken orally, especially during the passage on the way to the main colonisation site, the caecum. Effect of lauric acid supplementation on Campylobacter challenge An effect of lauric acid on C. jejuni requires the presence of the acid in significant concentrations at the main site of colonisation, the caecum. In the present study the highest concentrations of lauric acid in the gastrointestinal tract were demonstrated in the cranial parts (Fig 2). A direct effect of the lauric acid in cranial areas is therefore only to be assumed in the initial infection. In the present investigations, in the initial phase the spread of the infection was delayed (Table 6). The proportion of cloacal swabs with positive C. jejuni detection was significantly lower in those birds receiving a lauric acid-rich complete diet. On its way to the actual colonisation site, C. jejuni comes into contact with very high lauric acid concentrations in the anterior regions of the gastrointestinal tract. Therefore, in a short time-frame of 24 hours until establishment of the infection [41], an effect might be possible. Under conditions of infection, C. jejuni recedes into the mucus layer of the crypts[40] and becomes difficult to reach for antimicrobial acting substances [42]. Although the concentrations of lauric acid in the caecal content are comparable to the inhibitory concentrations in vitro [6], it remains questionable whether these low concentrations are effective in vivo, too. We found no differences concerning C. jejuni counts in excreta samples of experimentally infected birds (Table 7) or in the intestinal content of the caecal content depending on diet (Table 9). C. jejuni is primarily found in the mucus layer of the caecal and cloacal crypts when colonising the gastrointestinal tract [40]. Some of the substances identified as effective against Campylobacter in vitro were less effective in in vivo studies [42–44]. Initially, (experimental infection with C. jejuni VFU612, 106CFU/bird) caprylic acid had a significant effect on the diet of broilers (2.5 and 5 g/kg of diet) on reducing C. jejuni excretion (up to 1.8 log10 CFU/g; [45]). However, as in our study, the dietary concept did not lead to differences in caecal content on the day of dissection (d42). Palm kernel products also contain caprylic and capric acid. However, the concentrations used in our diets were very low (0.12% based on dry matter; Table 3). These concentrations are rather low compared to the literature. Supplementing the diet with 0.35% and 0.70% caprylic acid consistently decreased (P<0.05) the colonisation of C. jejuni in the chicken caeca compared with positive control treatment [46]. To conclude, offering a lauric acid rich diet only led to low concentrations of the acid in the substantial section caecum and cloaca. Therefore, downstream effects of resorption of the acid and therefore higher lauric acid concentrations in muscles might be of greater importance. Campylobacter load in breast meat of Ross 308 broilers receiving a lauric acid rich diet was reduced during six days of storage (4°C) from initially 5.9 log10 CFU/g to 3.5 log10 CFU/g (treatment) compared to 4.3 log10 CFU/g (control; P = 0.0295; [24]). Campylobacter–age effects From the results of the present study, it is apparent that the age of birds at the time of infection has a great influence on the frequency of the excretion of C. jejuni (Table 6). In older chickens of the laying breed (LBC-A98) the spreading of the colonisation was faster as was its disappearance. The C. jejuni numbers in excreta of LBC-A90 chickens ( log10 = 5,20±0,93 CFU/g) was also in the upper range of the C. jejuni numbers in broilers which are described as log 2–6 CFU/g excreta in the literature [40, 47]. Glünder [48] already showed that ten-week-old birds compared to four- and seven-week-old birds had a lower excretion. These observations coincide with our own results (Table 7). Young starlings were more frequently infected with C. jejuni compared to adult ones [49]. According to some authors, the probability of Campylobacter colonisation also increases with age [50–53]. However, the excretion is sometimes intermittent [54], but, on the other hand, numerically lower. This agrees with the investigations of Glünder [48] and our own investigations. The age of birds at the time point of challenge had an influence on the detection of C. jejuni in the caecum 21 days after experimental challenge in our seeder model (Table 9). The C. jejuni counts in the caecum of the LBC-A98 breed were significantly lower (ΔCFU/g = log101.91) than the C. jejuni number in the caecum of LBC-A42 chickens. The C. jejuni counts in the caecum of LBC-A42 chickens averaged at log108.46±0.62 CFU/g caecal content. These concentrations are in the upper range of the C. jejuni numbers described in the literature in the caecum of log10 = 5–8 CFU/g caecal content [37, 40, 55, 56]. The reason for the lower detection rates in certain age groups is discussed; the composition of caecal flora, the developmental status of the immune system as well as the maturity of the immune system being responsible for this [57]. Also, use of these protective bacteria in poultry production can greatly reduce carriage of C. jejuni within poultry [58]. This approach may be important in the present study. Campylobacter spp. is predominantly found in the mucus layer that lies within the crypts [40]. Campylobacter is chemotactically attracted by L-fucose in the mucin, using mucin itself as a substrate for growth [59] and replicates in the mucus [60]. It is known from previous studies that bacteria that have similar properties produce metabolites antagonistic to C. jejuni [58]. Occupying the same niche in chicks can prevent colonization of most chicks by C. jejuni [58]. In that study, hens with cloacal samples negative for C. jejuni were screened for isolates expressing inhibitory metabolites to C. jejuni and simultaneously use mucin as a sole substrate for their growth [58]. The older birds in the present study might also have been the host of a more competent intestinal flora. The relative mucin availability increases with age. Therefore, perhaps the older birds (LBC-A98) already had a flora that had long been adapted to the degradation of larger amounts of mucin. Thus, there may have been some competition between the resident microflora and C. jejuni after experimental infection which led to a lower prevalence and lower counts in the caecal content. Campylobacter–effects of genetic breed In the present investigations, an influence of the genetics on the Campylobacter prevalence (Table 6), but even more clearly on the amount of the excretion of Campylobacter with the excreta could be demonstrated (Table 8). The mean logarithmic Campylobacter numbers in the excreta of the LD birds and of the laying hybrids LBC-A42 showed significant differences to the two broiler breeds R308 and Hb757 at the end of the experimental period. For LBC-A42, these differences amounted to almost 2 log steps (ΔCFU/g = log 1.85) compared to the Hb757 breed. However, the LD breed showed the lowest Campylobacter prevalence 21 days after experimental challenge. From the literature, a link between genetic breed and Campylobacter prevalence in the group and bacterial counts of C. jejuni in the caecum is demonstrated [61–63]. Modern, fast-growing breeds responded with a strong inflammatory response to C. jejuni infections [19]. This was associated with a negative effect on the function of the T-lymphocytes, which led to a reduced immune regulation and damage to the intestinal mucosa with subsequent diarrhoea [19]. This relationship is consistent with our findings. On the other hand, when comparing a broiler and a laying genetic (Ross 308 versus Lohmann Selected Leghorn), 14 days after experimental infection (day one of life), there were significantly higher counts of C. jejuni in the caecum of the laying breed [64]. However, the sample size (n = 6 per group) was very small [64]. Even if the age is identical, it may be necessary to consider indirect effects of breed. For example, mucin concentrations also depend on the relative levels of protein uptake [65], and thus may have an effect on the C. jejuni infection dynamics. Conclusions In summary, it can be said that so far no comparable studies have been conducted that have tested, on the one hand, possible effects of lauric acid on the outcome of an experimental C. jejuni challenge in vivo, and on the other hand, effects of age for different genetic breeds under standardised conditions. The effects of the dietary concept were successful in the initial phase of the infection. This may be relevant for the practice of late infections in flocks, for example, due to pre-catch, as common found in Germany. The favourable effect of age was evident. This is in fact positive for alternative livestock systems which work with longer fattening periods. However, this only works if at the same time an entry of C. jejuni from outside can be efficiently prevented in these systems. Various risk assessment models for evaluating C. jejuni have shown that for differences of 2 log steps in C. jejuni counts in the intestine of broilers, the incidence of human campylobacteriosis is decreased by 76%–98% [66] or 44%–95% [67]. A reduction in the prevalence by a factor of two, results in a two-fold reduction of human campylobacteriosis cases since a one-to-one ratio prevails between these two parameters [68]. Thus, any reduction in the primary production level with respect to the extent of the excretion (Campylobacter numbers) and the excretion rate (Campylobacter prevalence) is to be considered successful since the risk of human campylobacteriosis is significantly reduced. Further studies with experimental challenge are necessary with the described infection model. The timespan between challenge and dissection should be shorter and possible effects of a late infection (due to pre-catch) as well as a less intensive bird to bird contact as in this experimental set-up should be proved in practice. Acknowledgments We would like to thank Frances Sherwood-Brock for proof-reading the manuscript to ensure correct English. We thank the Ahrberg-Foundation for the financial support of the investigations. This publication was supported by Deutsche Forschungsgemeinschaft and University of Veterinary Medicine Hannover, Foundation within the funding programme Open Access Publishing.
TI - Influence of lauric acid on the susceptibility of chickens to an experimental Campylobacter jejuni colonisation
JF - PLoS ONE
DO - 10.1371/journal.pone.0204483
DA - 2018-09-27
UR - https://www.deepdyve.com/lp/public-library-of-science-plos-journal/influence-of-lauric-acid-on-the-susceptibility-of-chickens-to-an-FdPRybBJ0n
SP - e0204483
VL - 13
IS - 9
DP - DeepDyve
ER -