Front Microbiol. 2017; 8: 828.
Published online 2017 May 12. doi: 10.3389/fmicb.2017.00828
PMCID: PMC5427123
Abstract
The
poultry reservoir, especially broiler meat, is generally recognized as
one of the most-important sources for human Campylobacteriosis. The
measures to control Campylobacter targeted essentially the
primary production level. The aim of this work was to evaluate the
effectiveness of different treatments against natural Campylobacter
colonization in a French experimental farm of free-range broilers
during the whole rearing period. Five commercial products and a
combination of two of them were tested and all the products were added
to feed or to water at the dose recommended by the suppliers. Campylobacter
loads in caeca and on carcasses of broilers at the slaughter were
determined by culture methods. Natural contamination of the flock
occurred at the end of the indoor rearing period between day 35 and day
42. At day 42, the multispecies probiotic added to the feed reduced the
contamination of 0.55 log10 CFU/g (p = 0.02) but was not significant (p
> 0.05) at the end of rearing at day 78. However, another treatment,
a combination of a cation exchange clay-based product in feed and an
organic acid mixture (formic acid, sodium formate, lactic acid,
propionic acid) in water, led to a slight but significant reduction of
0.82 ± 0.25 log10 CFU/g (p = 0.02) compared to the
control group at day 78. Testing this combination in field conditions in
several flocks is needed to determine if it is biologically relevant
and if it could be a valuable measure to reduce Campylobacter in broiler flocks.
Keywords: Campylobacter, control measure, feed additive, broiler, free-range
Introduction
Campylobacteriosis
is the most commonly reported zoonosis in the EU since 2005 and 229 213
confirmed cases were reported in 2015 (European Food Safety Authority [EFSA], and European Centre for Disease Prevention and Control [ECDC], 2016). The infectious agent is Campylobacter spp. mainly Campylobacter jejuni (90%) and Campylobacter coli
(10%), which cause an acute gastrointestinal infection in humans. The
poultry reservoir, especially broiler meat, is generally recognized as
one of the most-important source for human campylobacteriosis (European Food Safety Authority [EFSA], 2010b). In Europe, the mean prevalence of Campylobacter
in primary poultry production is very high, up to 70% of broiler
batches being contaminated with large differences ranging between 2 and
100% observed between countries (European Food Safety Authority [EFSA], 2010a). Moreover high numbers, up to 8 log CFU/g, of Campylobacter can be enumerated from broiler caecal contents (Hansson et al., 2010; Hue et al., 2010).
However, to date, no criteria have been established in the European legislation for Campylobacter spp. load in foodstuffs, and then a preventative approach is considered. Indeed, according to the study of Romero-Barrios et al. (2013), reducing Campylobacter spp. loads by 3-log10 in broilers’ gut would reduce the public health risk by at least 90%.
Evaluation of different potential interventions to prevent or to reduce Campylobacter
colonization in broilers is still in progress, as there is no
effective, reliable and practical strategy available so far. Some of
them have been reviewed recently (Robyn et al., 2015; Sahin et al., 2015; Meunier et al., 2016a; Saint-Cyr et al., 2016a).
Vaccination and the use of bacteriocins are not currently available,
but they could represent promising measures in the future (Svetoch and Stern, 2010; Meunier et al., 2016a,b). Feed additives with non-antibiotic products such as probiotic bacteria, prebiotics, plant extracts or organic acids against Campylobacter colonization are still extensively studied. They give some promising results in experimental trials leading to at least 2 log10 CFU/g reduction or more in Campylobacter colonization for some of them (Skanseng et al., 2010; Ghareeb et al., 2012; Guyard-Nicodeme et al., 2016; Saint-Cyr et al., 2016b).
In these studies testing feed additives, trials were generally
performed using conventional production conditions: indoor rearing,
broiler breeds, whole rearing (Hilmarsson et al., 2006; Thibodeau et al., 2015; Gracia et al., 2016; Guyard-Nicodeme et al., 2016), or shorter periods (Solis de Los Santos et al., 2008; Skanseng et al., 2010; Ghareeb et al., 2012).
However, there is an increasing consumer interest in free-range
poultry. In France, the free-range Label Rouge traditional poultry,
accounted for 15% of the production and 60% of the consumption of whole
broiler carcasses by French household (Salvat et al., 2017).
Breeding conditions of free–range broilers are different from those of
conventional production and vary according to the European Member
States. According to the French Label Rouge specifications, slow growing
breeds of broilers are reared with a lower breeding density indoor from
1 to 42 days old, and have access to an outdoor range from 6 weeks
until depopulation at 81 days old at least. As for the conventional
broilers, the free-range broiler flocks can be colonized by Campylobacter (Rivoal et al., 2005; Huneau-Salaün et al., 2007; Allen et al., 2011; Economou et al., 2015; Salvat et al., 2017). However, to the best of our knowledge the effect of feed additives against Campylobacter
in free-range broilers has not been yet studied. The aim of this work
was to evaluate the effectiveness of different additives against natural
Campylobacter colonization in a French experimental farm of free-range broilers.
Materials and Methods
Ethics Statements
This
study was carried out in an approved establishment for animal
experimentation under the “Label Rouge” program specifications for
rearing conditions by the aaa Direction Départementale de la Cohésion
Sociale et de la Protection des Populations des Landes bbb (agreement
number A-40-037-2). The protocol was designed and all practices were
performed according to the 2010/63/EU regulation about animal welfare.
Experimental Design
One day-old male chicks of strain T44 N x SA 51 (n
= 1440), purchased from a commercial hatchery, were reared in the
facilities of the Nutricia experimental farm (Benquet, Southwest of
France). This facility is designed to replicate rearing conditions
according to the Label Rouge program. At the hatchery, the birds were
vaccinated against Marek’s Disease, Bronchitis infectious, Gumboro and
Newcastle diseases and Coccidiosis. A booster vaccination for Bronchitis
infectious was carried out at 21 days. Rearing temperature was held
constant at 28°C during the first 3 days and then, it was gradually
reduced until the fourth week to reach 20°C. This temperature was
maintained until access to outdoor range after 42 days (according to the
criteria of the Label Rouge specifications). A continuous light was
applied during the first 48 h and was then reduced to 12 h per day.
Upon arrival, chicks were randomly allocated to one of the 36 pens (n
= 40 chicks per pen). Six pens were randomly assigned to the control
group, without any treatment (T1), and five pens were randomly assigned
per treatment (T2–T7).
Five commercial
products and a combination of two of them were tested and all the
products were added to feed or to water at the dose recommended by the
suppliers (Table Table11).
According to suppliers’ recommendations, treatments T3, T4, and T7 were
distributed throughout the trial; treatments T2, T5, and T6 were
distributed only from day 71 to day 78 (Table Table11). Food and water were available ad libitum.
Individual feeders and drinkers were displayed in each pen, avoiding
feed contamination from one pen to the others. The birds were fed from
day 1 to day 28 with a starter crumble, from day 29 to 49 with a grower
mash and from day 50 to day 78 with a finisher mash (Supplementary Table
S1).
Formulation of the different diets were iso-caloric and
iso-nitrogenous. Birds were slaughtered at D79 in a conventional
slaughterhouse where skin sampling was performed (first broiler batch of
the day).
Tested products, doses, and period of distribution.
Sampling and Microbiological Analyzes
Different types of samples were collected and analyzed during the course of the trial according to Figure Figure11.
The sampling included the collection of cardboards at the bottom of the
transport crates, fresh fecal material (pool of feces), caecal material
(caeca or pool of caeca) after euthanasia (electronarcosis followed by
bleeding) and neck skin samples. Until day 71, treatments T1, T2, T5,
and T6 were not distributed, therefore, animals in these groups were
confounded in a single control group called treatment T0.
Timeline of sampling and microbiological analyzes performed during the trial.
The
caecum was separated from the rest of the intestinal package through
sterile scissors and placed in hermetically sealed plastic bags. Neck
skin samples were collected from carcasses taken from the processing
line after chilling at the slaughterhouse. After collection, samples
were shipped in an insulated box to the ANSES laboratory (Ploufragan,
Northwest, France) within 24 h with a cooler carrier (4°C). Samples were
processed and analyzed upon arrival depending on the sample as
following:
Absence of Campylobacter from cartons on the bottom of transport crates was assessed after enrichment according to part 1 of the ISO 10272 (Anonymous, 2006).
Samples were weighed and diluted 1:10 (wt:vol) in Bolton broth and the
mix was homogenated in a peristaltic homogenizer (AES, Bruz, France).
For detection purposes, 10 ml of the homogenate was added to 90 ml of
Bolton broth (Oxoid, Dardilly, France). The inoculated broth was then
incubated under microaerophilic conditions for 4 h at 37°C and then for
44 ± 4 h at 41.5 ± 1°C.
Fecal materials were weighed
and diluted 1:10 (wt:vol) in tryptone salt broth and the mix was
homogenized in a peristaltic homogenizer (AES, Bruz, France). Presence
or absence of Campylobacter was assessed after direct plating
of the homogenate on mCCDA plates (modified Charcoal, Cefoperazone,
Desoxycholate Agar, Oxoid, Dardilly, France), and incubation as above.
Characteristic colonies were confirmed with optical microscopy analysis.
Campylobacter from caecal contents were recovered using direct plating and/or enumeration. Direct isolation of Campylobacter
was assessed by direct seeding of the caecal content on mCCDA and 44 ± 4
h of incubation at 41.5 ± 1°C in a microaerophilic atmosphere (85% N2, 10% CO2, 5% O2). In order to assess Campylobacter’s
counts, caecal contents were weighed, diluted in tryptone salt broth,
and homogenized in a peristaltic homogenizer (AES, Bruz, France). Serial
dilutions of the homogenate in tryptone salt broth, were plated on
selective mCDDA plates and enumeration was assessed after incubation as
above. The threshold for enumeration was 2 × 102 CFU/g (2.3 log10 CFU/g) of caecal content.
For the neck skin samples, detection after enrichment and enumeration of Campylobacter was performed according to part 1 and 2 of the ISO 10272 (Anonymous, 2006)
respectively. Samples were weighed and diluted 1:10 (wt:vol) in
tryptone salt broth and the mix was homogenated in a peristaltic
homogenizer (AES, Bruz, France). For detection purposes, 10 ml of the
homogenized was added to 90 ml of Bolton broth (Oxoid, Dardilly,
France). The inoculated broth was then incubated under microaerophilic
conditions for 4 h at 37°C and then for 44 ± 4 h at 41.5 ± 1°C. The
culture in Bolton broth was subsequently plated onto mCCDA and Butzler
agar (Virion N°2) (Oxoid, Dardilly, France) and incubated for 44 ± 4 h
at 41.5 ± 1°C. Characteristic colonies were confirmed with optical
microscopy analysis. For the quantification, Campylobacter were
enumerated by plating 1 ml of the homogenate onto three plates of
mCCDA. Tenfold serial dilutions of the homogenate in tryptone salt broth
were also prepared and plated onto mCCDA plates. All plates were
incubated under microaerophilic conditions for 44 ± 4 h at 41.5 ± 1°C.
The threshold for enumeration was 10 CFU/g (1 log10 CFU/g) of neck skin.
Performance
Animal
weights were recorded individually at days 14, 28, 53, 72, 79 and at
the slaughterhouse. The record of food consumption took place weekly and
at the day of weighing. Daily consumption, daily gain and feed
conversion ratio (FCR) were calculated for 3 periods: from D1 to D28,
D29 to D72 and D73 to slaughter. Mortality was recorded daily and dead
animals were weighted individually.
Statistical Analysis
Campylobacter
loads in caeca, weight and feed consumption were analyzed using an
ANOVA model including the treatment as a fixed effect and the pen as a
random effect; post hoc tests were carried out for mean comparisons (Tukey test, P < 0.05). For comparison of Campylobacter loads on neck skin, the ANOVA model only included the treatment as a fixed effect.
Results
Effect of Treatments on Campylobacter Colonization
No Campylobacter was detected on chick transport crate. From day 1 to day 35, Campylobacter was not recovered from the samples, whatever the treatment was (data not shown). Campylobacter
was detected in samples from day 42 onward. Therefore, natural
contamination of the flock occurred between day 35 and day 42, and the
treatments T3, T4, and T7 did not prevent colonization of the broilers.
At day 42, enumeration of Campylobacter in caecal contents was performed to determine if the treatments T3, T4, and T7 distributed from day 1 impacted Campylobacter loads in caeca, compared to the control group T0 (constituted of samples from the T1, T2, T5, and T6 groups). As shown in Table Table22, broilers that received the treatment T3 (Multispecies probiotic) had significantly lower Campylobacter counts than the control group (P = 0.02). However, the observed mean reduction was less than 1 log10
CFU/g. Treatments T4 (prebiotic-like) and T7 (fermented product) did
not lead to a significant reduction compared to the control group.
Effect of dietary treatment on Campylobacter counts (Log10CFU/g, mean ± standard deviation) in the caeca of broilers at 42, 71, and 78 days of age.
A
second sampling was carried out at day 71 to determine the
contamination levels in the groups T2, T5, and T6 before application of
the treatments and to check the effect of the treatments T3, T4, and T7
compared to the control group T1. At day 71, the contamination level was
not significantly different in the groups T2, T5, and T6 before
application of treatments compared to the control group T1. Campylobacter
loads in the three treated groups T3, T4, and T7 were not significantly
different than the one observed in the control group T1.
Otherwise, the mean Campylobacter loads in all treatment decreased from 8.08 log10 CFU/g (CI95% [7.93–8.22]) at D42 to 6.69 log10 CFU/g (CI95% [6.50–6.88]) at D71. The decrease was also observed in the control treatment (8.43 log10 CFU/g (CI95% [8.15–8.72]) at D42 vs. 6.83 log10 CFU/g (CI95% [6.24–7.42]) at D71).
Results
at day 78 revealed that the three groups receiving a treatment since
the beginning of the trial (T3, T4, and T7) did not show a significant
reduction of the colonization compared to the control group. Among the
three groups receiving a product only during the last week of rearing
(T2, T5, and T6), only T6 (combination T2 + T5: a clay-based product in
feed, and an organic acid mixture in water, respectively) showed a
significant reduction estimated at 0.82 ± 0.25 log10 CFU/g (p = 0.02) compared to the control group.
Effect of Treatments on Campylobacter Contamination of Carcasses (Neck Skin)
At slaughter, carcasses from treatment T6 showed a slight but significant (p = 0.01) reduction estimated at 0.68 ± 0.24 log10 CFU/g in Campylobacter counts on neck skin samples compared to the control group T1 (Table Table33).
No other significant difference was observed between the control group
and the other treatments. Nevertheless, these results need to be
confirmed using a higher number of samples, as only five carcasses per
group were sampled in this study.
Campylobacter loads (log10 CFU/g) on neck skin at D81.
Effect of Treatments on Growth Performance
Broilers
from T3, T4, and T7 showed a higher daily weight gain in comparison
with the ones from treatments with no additive during the first rearing
period but their FCR was not significantly improved (Table Table44).
Over the whole rearing period no constant effect of the treatments were
observed on daily feed consumption, daily weight gain and FCR. The mean
mortality rates varied from 0.07% in T6 (1/240) to 3.8% (7/200) in T1
with no significant difference between treatments (data not shown).
Daily
feed consumption (g), daily body weight gain (g) and feed conversion
ratio (FCR) from D1 to D28, from D29 to D72, from D73 to slaughter and
over the whole rearing period according to the treatments (Least Squares
Mean ± Standard Error).
Discussion
Animal welfare is an increasing important issue for the consumers (Napolitano et al., 2010)
and therefore there is a growing interest for free range and/or
organically ranged broilers. However, the free-range rearing conditions
bring together several of the known risk factors favoring Campylobacter
colonization in broilers with for example the contact of the birds with
an open environment and the age of the birds at slaughter (Huneau-Salaün et al., 2007; Newell et al., 2011). In France a representative study conducted in 2008 demonstrated that prevalence of Campylobacter in caecal contents of slaughtered batches was 100.0% for the Label chickens compared to 69.7% for the standard chickens (Hue et al., 2010).
During this study, broilers were naturally colonized by Campylobacter at the end of the indoor rearing period between day 35 and day 42. These results are in agreement with those of Huneau-Salaün et al. (2007) who reported that 71.2% of French free-range flocks are positive for Campylobacter at the end of the indoor rearing period. However, in some cases, broilers become colonized by Campylobacter after 6 weeks of rearing inside the building, when they can have access to the outdoor range (Rivoal et al., 2005).
Developing a control strategy against Campylobacter
in the primary production is needed. Finding an effective product to be
added to feed or water among the already marketed products could be a
rapid solution. The tested products of this study were chosen based on a
claimed activity, such as reducing pathogen, limiting bacterial growth
or digestive pathogens, and/or improving immune functions. Five products
and a combination of two of them were evaluated in the same trial. They
were added according to the manufacturer’s conditions. None of the
three treatments (T3, T4, and T7) used from day 1 was able to prevent Campylobacter
colonization detected at day 42. Similar results were observed in
previous works testing several feed additives in experimental facilities
with artificial Campylobacter contamination on fast-growing broilers (Gracia et al., 2016; Guyard-Nicodeme et al., 2016; Saint-Cyr et al., 2016b). Moreover, no treatment using single product (T2, T3, T4, T5, and T7) led to a significant reduction of Campylobacter
in caeca, compared to the control group at the end of the rearing
period. Treatment T2 (clay-based product) was previously tested in
experimental facilities with artificial Campylobacter challenge and a mean reduction of 2.5 log10
CFU/g was observed in fast-growing birds after 36 days of rearing,
although it failed to reduce the pathogen in slow growing birds in the
same conditions (Guyard-Nicodème et al., 2014). It could be hypothesized that product efficacy could be impacted by the broiler breeds. However, Gormley et al. (2014) demonstrated that Campylobacter colonization is not affected by the broiler breeds (fast or slow growing breeds).
On
the contrary, treatment T6, using the combination of the clay-based
product (T2) in feed and an organic acid mixture in water (T5), led to a
significant reduction of Campylobacter spp. counts in the
caeca, and this reduction was also observed on neck skin at the
slaughterhouse. Reduction in the caeca was low, as less than 1 log10
CFU/g (0.82 ± 0.25 log10 CFU/g) was observed. Several previous studies
presented results of feed or water additives leading to a reduction of Campylobacter colonization higher than 2 log10 CFU/g but they were performed in experimental facilities with an artificial Campylobacter challenge (Nishiyama et al., 2014; Arsi et al., 2015; Gracia et al., 2016; Guyard-Nicodeme et al., 2016; Saint-Cyr et al., 2016b).
However, these controlled conditions cannot reflect the field
conditions, especially free-range conditions exposed to multiple sources
of contaminations and contaminated with genetically diverse Campylobacter isolates (Rivoal et al., 2005). Anyway, the reduction of Campylobacter obtained with T6 was less than 1 log10
CFU/g at the flock, and the slight reduction observed at the
slaughterhouse, could have an impact on public health. Indeed, reduced
colonization in caecal contents of flocks by 1 log10 unit could reduce the number of campylobacteriosis cases from 48 to 83% (Romero-Barrios et al., 2013).
Moreover this combination was used only the last week of rearing and
had no impact on performance parameters. Therefore, these results need
to be confirmed in other field trials using several other flocks to
determine if it could be applied as an efficient control measure.
Author Contributions
MG-N,
AH-S, MQ, and MC contributed to the conception and design of the study.
FT, SQ, and TP performed the experiments and MQ supervised the trial in
the experimental farm. MG-N, AH-S, and FT analyzed the results and
wrote the paper. FS and MC critically analyzed and revised the
manuscript.
Conflict of Interest Statement
The
authors declare that the research was conducted in the absence of any
commercial or financial relationships that could be construed as a
potential conflict of interest.
Footnotes
Funding.
This study is part of the project “CAMCHAIN.” This project has received
funding from the European Union’s Seventh Framework Programme for
research, technological development and demonstration under grant
agreement no 291815.
Supplementary Material
The Supplementary Material for this article can be found online at: http://journal.frontiersin.org/article/10.3389/fmicb.2017.00828/full#supplementary-material
Click here for additional data file.(23K, DOCX)
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