Effects of cLFchimera peptide on intestinal morphology, integrity, microbiota, and immune cells in broiler chickens challenged with necrotic enteritis

Three hundred and sixty 1-day-old male broiler chicks were randomly allocated to 4 treatments of 6 replicates to evaluate the effects of cLFchimera, a recombinant antimicrobial peptide (AMP), on gut health attributes of broiler chickens under necrotic enteritis (NE) challenge. Treatments were as follows: (T1) unchallenged group fed with corn-soybean meal (CSM) without NE challenge and additives (NC); (T2) group fed with CSM and challenged with NE without any additives (PC); (T3) PC group supplemented with 20 mg cLFchimera/kg diet (AMP); (T4) PC group supplemented with 45 mg antibiotic (bacitracin methylene disalicylate)/kg diet (antibiotic). Birds were sampled for villi morphology, ileal microbiota, and jejunal gene expression of cytokines, tight junctions proteins, and mucin. Results showed that AMP ameliorated NE-related intestinal lesions, reduced mortality, and rehabilitated jejunal villi morphology in NE challenged birds. While the antibiotic non-selectively reduced the count of bacteria, AMP restored microflora balance in the ileum of challenged birds. cLFchimera regulated the expression of cytokines, junctional proteins, and mucin transcripts in the jejunum of NE challenged birds. In conclusion, cLFchimera can be a reliable candidate to substitute growth promoter antibiotics, while more research is required to unveil the exact mode of action of this synthetic peptide.

AMP production. cLF chimera was derived from camel lactoferrin (cLF) consisting of 42 amino acids and has primary sequence of DLIWKLLVKAQEKFGRGKPSKRVKKMRRQWQACKSSHHHHHH. In addition, the results of our previous study showed that cLFchimera had antioxidant activity (IC50: 310 μ/ml) and its activity was not affected after 40 min of boiling 17 (for more details regarding production process, please review previous papers 12,13,17 ). Briefly, preparation of recombinant plasmid vector was conducted through transforming recombinant expression vector harboring synthetic cLFchimera into DH5α bacterium 12,13 . Next, the latter bacterial colonies were cultured to harvest plasmid extraction. The recombinant vector was then transferred into E. coli BL21 (DE3) as an expression host and cultured in 2 ml Luria-Bertani broth (LB) medium for overnight according to standard protocol 18 . In the next step, cultured materials were inoculated in 50 ml LB and incubated at 37 °C with shaking at 200 rpm. Then, isopropyl-β-d-thiogalactopyranoside (IPTG) was added to a final concentration of 1 mM and incubated at 37 °C for 6 h after IPTG induction. Periplasmic protein was collected at different times after IPTG induction (2, 4, and 6 h) according to the method described by de Souza Cândido et al. 19 and analyzed on 12% SDS-PAGE. To purify expressed peptide, Ni-NTA agarose column was used based Table 1. Composition of experimental diets. 1 Antibiotic (45 mg bacitracin methylene disalicylate/kg diet) and peptide (20 mg/kg diet) were added on top and thoroughly mixed. 2 Added per kg of feed: vitamin A, 7,500 UI; vitamin D3 2100 UI; vitamin E, 280 UI; vitamin K3, 2 mg; thiamine, 2 mg; riboflavin, 6 mg; pyridoxine, 2.5 mg; cyanocobalamin, 0.012 mg, pantothenic acid, 15 mg; niacin, 35 mg; folic acid, 1 mg; biotin, 0.08 mg; iron, 40 mg; zinc, 80 mg; manganese, 80 mg; copper, 10 mg; iodine, 0.7 mg; selenium, 0.3 mg. Ingredient (%) 1 Starter (0-10 days) Grower ( www.nature.com/scientificreports/ on manufacturer's instruction (Thermo, USA). The quality of purified recombinant peptide was assessed on a 12% SDS-PAGE gel electrophoresis, while the Bradford method was used to analyze the quantity of recombinant peptide. More recently, an E. coli expression system was developed in our laboratory that is able to produce 0.42 g/L of recombinant peptide. Finally, four grams of peptide previously obtained from the recombinant E. coli were purified, lyophilized, and thoroughly mixed with 1 kg soybean meal and then supplemented to the relevant experimental diets.
NE challenge. A previously described method of inducing NE was used with some modifications 20 . Briefly, on day 16, chicks in NC group were administered a single 1 ml oral dose of sterile phosphate-buffered saline (PBS) (uninfected) as a sham control, while PC, peptide and the antibiotic groups were orally inoculated with 5,000 attenuated vaccine strain sporulated oocysts each of E. maxima, E. acervulina, and E. tenella (Livacox T, Biopharm Co., Prague, Czech Republic) in 1 mL of 1% (w/v) sterile saline. On days 20 and 21, birds in the NE groups were orally inoculated with 1 ml of broth containing C. perfringens isolated from broilers meat 21 , CIP (60.61) containing 10 7 cfu/ml in thioglycollate (Thermo-Fisher Scientific Oxoid Ltd, Basingstoke, UK) supplemented with peptone and starch. Inoculated C. perfringens was analysed using PCR to confirm the presence of netB gene required for inducing NE in broilers according to Razmyar et al. 22 . The unchallenged group received the same dose of sterilized broth.
Growth performance. On days 10 and 22, average daily gain (ADG), average daily feed intake (ADFI) and feed conversion ratio (FCR) were calculated using body weight (BW) and the weight of feed which remained in each pen. The ADG, ADFI and FCR were calculated over the specific and comprehensive periods of the study (0-10, 11-22, and 0-22 days). The feed conversion ratio for each period was readjusted based on the mortality data per pen per day, if any.
Sample collection and lesion score. On days 10 and 22, two birds from each pen (12 birds/treatment) were randomly selected for euthanasia by cervical dislocation. The viscera was excised from the specimens, the intestine discretely separated and the adherent materials were precisely removed. The ileum was gently pressed to aseptically collect ileal content into sterile tubes for microbiological analysis. A section of approximately 5 cm from mid-jejunal tissues was meticulously separated for morphological analysis. A 2 cm section from the mid-jejunum was detached, rinsed in cold phosphate-buffered saline (PBS), immediately immersed in RNAlater (Qiagen, Germantown, MD), and stored at − 20 °C for subsequent gene expression determination. On day 22, NE lesions of duodenum, jejunum, and ileum from 2 birds per pen were scored on a scale of 0 (none) to 6 (high) as described previously 23 .
Intestinal morphology. The method used to prepare samples for morphometry analysis was previously described by Daneshmand et al. 24 . Briefly, jejunal samples were stored in a 10% formaldehyde phosphate buffer for 48 h. The samples were then processed on a tissue processor (Excelsior AS, Thermo Fisher Scientific, Loughborough, UK), fixed in paraffin using an embedder (Thermo Fisher Histo Star Embedder, Loughborough, UK), and cut with a microtome (Leica HI1210, Leica Microsystems Ltd., Wetzlar, Germany) to a length of 3 cm per slice. The slices were placed on a slide and dehydrated on a hotplate (Leica ASP300S, Leica Microsystems Ltd., Wetzlar, Germany) and dyed with hematoxylin and eosin. Finally, the dyed slices of jejunal were examined under a microscope (Olympus BX41, Olympus Corporation, Tokyo, Japan). A total of 8 slides were prepared from the jejunal segment per bird, and ten individual well-oriented villi were measured per slide (80 villi/bird). The average of each measurement per sample was reported as the respective a mean for each bird. Villus width (VW) was measured at the base of each villus; villus height (VH) from the top of the villus to the villus-crypt junction, crypt depth (CD) from the base of the adjacent villus to the sub-mucosa, the ratio of VH/CD and villus surface area were calculated.
Microbial count. The methods used to count the populations of E. coli, Clostridium spp., Lactobacillus spp., and Bifidobacterium spp. in the ileal content were described elsewhere 25 . In summary, the ileal contents of a sample were thoroughly mixed, serially diluted tenfold from 10 −1 to 10 −7 with sterile PBS, and homogenized for 3 min. Next, dilutions were plated on different agar mediums. Regarding the enumeration of bacteria, Lactobacillus spp. and Clostridium spp. dilutions were plated on MRS agar (Difco, Laboratories, Detroit, MI) and SPS agar (Sigma-Aldrich, Germany) and anaerobically cultured at 37 °C for 48 h and 24 h, respectively. Black colonies of Clostridium spp. on SPS agar were counted. MacConkey agar (Difco Laboratories, Detroit, MI) and BSM agar (Sigma-Aldrich, Germany) were used to cultivate E. coli and Bifidobacterium spp. respectively, and incubated at 37 °C for 24 h. All microbiological analyses were performed in triplicate, and average values were used for statistical analyses and results were expressed in colony-forming units (Log 10 cfu/g of ileal content).

RNA extraction and gene expression.
The procedure of RNA extraction and gene expression was previously explained 26 . In summary, total RNA was extracted from chicken jejunum sampled on day 22 using the total RNA extraction kit (Pars Tous, Iran) following the manufacturer's instructions. The purity and quality of extracted RNA were evaluated using an Epoch microplate spectrophotometer (BioTek, USA) based on 260/230 and 260/280 wavelength ratios, respectively. Genomic DNA was removed using DNase I (Thermo Fisher Scientific, Austin, TX, USA). The complementary DNA (cDNA) was synthesized from 1 µg of total RNA using the Easy cDNA synthesis kit (Pars Tous, Iran) following the manufacturer's protocol.  27 . Each reaction was performed in a total volume of 20 μl in duplicate using an ABI 7300 system (Applied Biosystems, Foster City, CA) and 2 × SYBR Green Real Time-PCR master mix (Pars Tous, Iran). Primer details are shown in Table 2. All primers were designed according to MIQE criteria 27 regarding amplification length and intron spanning. All efficiencies were between 90 and 110%, and calculated R 2 was 0.99 for all reactions. The method 2 −ΔΔCt Ct was used to calculate relative gene expression in relation to the reference genes 28 (GAPDH and β-actin).
Statistical analysis. Data were statistically analyzed in a completely randomized design by ANOVA using the General Linear Model (GLM) procedure of SAS (SAS Inst., Inc., Cary, NC). Tukey's test was used to compare differences among means of treatments, and P values < 0.05 were considered to be significant.

Results
Lesion score and mortality. Table 3 shows the effects of experimental treatments on NE-inducing lesion scores in different segments of the intestine and mortality rate of broiler chickens. The results showed that none of the additives could rehabilitate the NE-inducing lesions in the intestine compared to NC. While the highest lesion scores in the intestine of PC group showed that NE was efficiently induced in broilers, AMP decreased (P < 0.05) lesions in duodenum, jejunum, and ileum of broilers compared to the challenged group.
Inducing NE in broilers increased (P < 0.05) mortality, while birds fed with peptide showed lower (P < 0.05) mortality rate compared to PC group and interestingly had similar results to NC group. Table 2. Sequences of primer pairs used for amplification of target and reference genes. 1 1 For each gene the primer sequence for forward and reverse (5´ → 3´), the product size (bp), and the annealing temperature (Ta) in °C are shown. 2 ANXA1, annexin A1; TRAF3, tumor necrosis factor receptor associated factor 3; MUC2, mucin2; CLDN1, claudin1; OCLDN, occludin; GAPDH, Glyceraldehyde 3-phosphate dehydrogenase.   Table 4 represents the effects of experimental diets on growth performance of broilers. While the antibiotic improved (P < 0.05) birds' ADG at first 10 days of age, peptide showed the best FCR at the end of starter period when no challenge was induced yet. At d 22, NE challenge decreased (P < 0.05) ADG and increased (P < 0.05) feed intake, which devastated (P < 0.05) FCR in broilers. In the latter phase, peptide showed similar effects to NC group, while improved (P < 0.05) performance indices compared to PC group.
Jejunal villi morphology. The effects of treatments on jejunal morphology are shown in Table 5. On day 10, experimental diets had no significant effects on the morphometry of the intestine. NE challenge significantly demolished villi structure and morphology, while AMP enhanced (P < 0.05) villus height, width, and surface area (VSA) compared to PC group and had a similar effect to NC group at 22 days of age. Experimental diets had no significant effects on CD and VH/CD at d 22. Although the antibiotic improved (P < 0.05) villi morphology compared to NE-challenged birds, it could not restore villi characteristics to those of NC.
Bacterial colonization. Table 6 summarizes the effects of experimental diets on ileal bacterial populations.
At d 10, the antibiotic decreased (P < 0.05) the population of all bacteria compared to other groups. NE challenge increased (P < 0.05) the count of E. coli and expectedly Clostridium spp. and also decreased (P < 0.05) the number of Lactobacillus spp. and Bifidobacterium spp. in the ileum of birds. In the same period, the antibiotic had the lowest (P < 0.05) population of all cultured ileal bacteria compared to both PC and NC groups. Interestingly, AMP had similar effects to NC group, while it increased (P < 0.05) the population of Lactobacillus spp. and Bifidobacterium spp. and also decreased (P < 0.05) the colonization of E. coli and Clostridium spp. in the ileum of chickens compared to the challenged birds at 22 days of age.

Gene expression of immune cells and tight junctional proteins.
The effects of treatments on the expression level of immune and tight junction genes are presented in Fig. 1. While NE challenge increased (P < 0.05) TRAF3 and ANXA1 transcripts, adding the antibiotic and AMP to the diet reduced (P < 0.05) the www.nature.com/scientificreports/ expression of immune genes compared to PC group and the antibiotic had similar effects to those of nonchallenged birds. While NE challenge increased the expression of MUC2 in the jejunum of birds, AMP decreased (P < 0.05) the level of MUC2 trasncripts compared to PC group and had similar levels to NC group. Birds challenged with NE had the lowest expression levels of CLDN1 and OCLN genes in their jejunum. AMP increased (P < 0.05) expression patterns of CLDN1 in the jejunum of birds compared to PC group and had similar effects to those of non-challenged birds. Although birds fed with AMP had higher (P < 0.05) OCLN mRNA in the jejunum compared to PC group, this group had lower (P < 0.05) expression of this transcript compared to NC group. The antibiotic did not affect the level of tight junctions transcripts in the jejunum of NE challenged birds compared to both NC and PC groups.

Discussion
Necrotic enteritis is still a global concern with drastic losses in poultry farms, mainly due to retarded growth performance, increased mortality, and veterinary costs 23 . The outbreak of disease and consequently economic losses have been more prominent in the post-antibiotic era 23 . Recently, research focus has shifted to AMPs due to their beneficial roles on health attributes and their prophylactic effects against pathogenic invasion 12,13,17 . Therefore, the principal objective of the current study was to investigate the effects of antimicrobial peptide, cLFchimera, on various productive and health parameters in chickens challenged with NE.
Results of the current study showed that AMP decreased gut lesions and mortality induced by NE. Additional benefits include also improved growth attributes in challenged chickens similar to birds fed antibiotic, confirming the results of previous studies 9, 10 . While most of the previous researches have studied the effects of AMPs in chickens in normal conditions, Hu et al. 29 demonstrated that supplementing broilers diet with AMP improved their weight gain and FCR under heat stress. In another challenge study, Wu et al. 30 inoculated weanling pigs with E. coli and supplemented the diet with AMP. The autors reported that AMP reduced the incidence of diarrhea and improved weight gain and FCR compared to the challenged group, which is similar to the present findings regarding the reduction in gut lesion and improvement of performance. Previous studies attributed the beneficial effects of AMPs on growth performance of chickens to their fundamental roles in maintaining microbial balance in the gut and consequently improvement in the intestinal morphometry 9, 10 .
It has been well-documented that the villi play the critical roles in absorbing nutrients from the intestinal tract; consequently the morphometry of these villi can drastically affect the host's performance and health 31 . The present study confirmed, AMP significantly improved the morphometry of villi in the jejunum of challenged chickens, similar to that of NC group 9,10 . It has been reported that AMPs extracted from pig intestine 32 and rabbit sacculus rotundus 33 enhanced jejunal villi characteristics in broiler chickens, which is in line with the present results. Generally, the critical strategy in maintaining villi structure in an infectious disease like NE is the elimination or minimization of the pathogens through provision of antimicrobial additives and manipulation of the intestinal microbiome 34,35 . Previous studies showed that the antibiotic and AMPs could improve villi morphology and nutrient absorption and consequently increase growth performance in chickens under disease conditions by manipulating the intestinal microflora 9,10,17 .
The intestinal commensal microbiome interacts with the host through different processes, including nutrients absorption, villi morphology, intestinal pH, and mucosal immunity 36,37 . In the current study, the supplementation of the antibiotic reduced the colonization of all bacteria, while AMP significantly enhanced the microflora balance in the ileum. In agreement with the present study, Tang et al. 7 and Ohh et al. 38 reported that AMPs significantly enhanced the microflora balance in the ileum of piglets and broilers, respectively. The antimicrobial action of Bacitracin Methylene Disalicylate (BMD) involves blocking the bacterial ribosome subunits and subsequently impeding protein synthesis, which finally reduces the colonization of the microbial community in the intestine 39 . Unfortunately, this antibiotic does not differentiate between commensal vs. pathogenic bacteria and may perturb microbial balance in the intestine and deprive the host of benefits of microbes' roles and products 39,40 . There is no consensus on the mechanism by which AMPs influence bacterial colonization in the intestine, while two Table 6. Effects of treatments on ileal microflora (log 10 CFU g -1 ) in broilers at 10 and 22 days of age. a-c Values within a column with different letters differ significantly (P < 0.05). 1 NC: negative control group received cornsoybean meal diet without challenge and additives; PC: positive control group received NC diet experimentally challenged with necrotic enteritis; AMP: PC received group supplemented with 20 mg antimicrobial peptide/ kg diet; Antibiotic: PC received group supplemented with 45 mg antibiotic (bacitracin methylene disalicylate)/ kg diet. 2 SEM: standard error of means (results are given as means (n = 12) for each treatment). www.nature.com/scientificreports/ direct and indirect mechanisms have been proposed based on the physiological properties of peptides. The direct antimicrobial effect of AMPs has been attributed to different surface charges of peptides and pathogens 41 . In other words, AMPs possess positive charges contributing to electrostatically adhere to negatively charged bacterial Samples were analyzed using qPCR, and GAPDH and β-actin were used as the reference genes. Abbreviations as follows: ANXA1, annexin A1; TRAF3, tumor necrosis factor receptor associated factor 3; MUC2, mucin2; unchallenge, control birds received a corn-soybean meal basal diet without AMPs, antibiotic and necrotic enteritis (NE) challenge; challenge, control birds challenged with NE; peptide, birds challenged with NE and supplemented with 20 mg cLFchimera/kg diet; Antibiotic, birds challenged with NE and supplemented with 45 mg antibiotic (bacitracin methylene disalicylate)/kg diet; The letters on the bar mean show significant difference (P < 0.05).
In the indirect mode, AMPs might manipulate the microbial community of the intestine in favor of the colonization of beneficial bacteria (e.g. Lactobacillus spp. and Bifidobacterium spp.) and enhance the host health through various physiological mechanisms (e.g. competitive exclusion, secretion of short-chain fatty acids, activation of intestinal immune system, etc.) 42 . Previous findings suggested that cLF36 could attach to the bacterial membrane through electrostatic interactions and physically disrupt bacterial bilayer membranes 12,13,16 . In line with the previous reports 44 , the current results demonstrate that AMP can selectively prevent the bacterial growth in the intestine of NE challenged chickens, which may prove the competitive advantage of cLFchimera compared to antibiotics. Furthermore, previous research reported that the antimicrobial activities of AMPs against pathogens in the intestine might alert the host immune system to fight against invading agents 45,46 .
Mucosal immunity plays an important role in host defense against pathogens 47 . In broiler chickens, when Toll-like receptor (TLR)4 engages to microbe-associated molecular patterns (MAMP), it transmits the information to the cytoplasm of the phagocytes, which in turn leads to the expression of cytokines 48,49 . Different research groups have reported the controversial results regarding the effects of C. perfringens challenge on gene expression of TLR4 in the intestine of broiler chickens. For instance, while some researchers reported that C. perfringens upregulated the TLR4 gene expression in the intestine of chickens 50,51 , other investigators reported no apparent alteration of the TLR4 gene expression in C. perfringens challenged chickens 52 . Therefore, in the current study, we decided to analyze the gene expression of TRAF3, which is one step ahead of TLR4 activation to overcome the possible interference of other immune cells 53 . TRAF3 is a cytoplasmic protein that controls signal transduction from different receptor families, especially TLRs 53 . Following the activation of TLR4 with pathogen attachment, TRAF3 is recruited into signaling complexes, and its activation increases vital pro-inflammatory cytokines production 54,55 . Results of the present study showed that NE upregulated the expression of TRAF3 transcript in the jejunum of chickens, while the antibiotic and AMP significantly decreased the gene expression of this cytokine in the challenged birds, which is consistent with the results of previous studies 54,56 .
On the other hand, excessive and long-term production of pro-inflammatory cytokines might result in the gut damage and high energy demand 57 . To prevent the adverse effects of extra pro-inflammatory cells, pro-resolving mediators such as ANXA1 are released into the epithelial environment to orchestrate clearance of inflammation and restoration of mucosal homeostasis 58,59 . ANXA1 is a 37 kDa protein expressed in the apical and lateral plasma membrane in the intestinal enterocytes that facilitates the resolution of inflammation and repair 60 . In the current study, C. perfringens upregulated the expression of ANXA1 mRNA in the jejunum of PC group, which is in agreement with previous report 54,61 , while the antibiotic and AMP significantly decreased the expression of this cytokine, which is firstly reported herein. While there is no well-documented evidence to explain the results of cytokines expression, it could be inferred that antimicrobial activities of the antibiotic and AMP in the current study resulted in the reduction of invading pathogens (based on abovementioned microbial results) in the intestine of PC birds and possibly downregulating the expression of both pro-and anti-inflammatory (i.e. TRAF3 and ANXA1, respectively) cytokine-producing cells.
The epithelial barrier consists of tight junction proteins forming the primary lines of defence against a wide range of stimuli from feed allergens to commensal and pathogenic bacteria 62,63 . The disruption of these proteins may result in increasing the intestinal permeability to luminal pathogens 62,63 . Previous studies showed that C. perfringens might attach to the junctional proteins to form gaps between the epithelial cells and disrupt the intestinal integrity 63,64 . In the present study, NE challenge reduced the jejunal expression of OCLN and CLDN1 transcripts, which is in agreement with previous studies 64,65 . Previous studies showed that tight junction proteins, especially CLDN1 and OCLN, have a specific region (i.e. ECS2) containing a toxin-binding motif, NP (V/L)(V/L)(P/A), that is responsible for binding to C. perfringens 63,66 . Following attachment to junctional proteins, C. perfringens could digest these proteins 67 and open the intracellular connection between adjacent epithelial cells resulting in more penetration of pathogens to deeper layers of lamina propria and transmitting to other organs 63,68 . AMP significantly upregulated the expression of these genes in PC group and the antibiotic had no significant effect on the gene expression of junctional proteins. In agreement with the current findings, previous reports demonstrated that AMPs could increase the expression of junctional proteins in different challenge conditions 17,69 . While no exact mechanism has been recognized, there are two suggested theories for the inhibitory effects of AMPs on C. perfringens regarding junctional proteins. In the first theory, it has been suggested that AMPs could directly switch on the expression of regulatory proteins (i.e. Rho family) in the intestine of challenged mice, upregulating the expression of tight junction proteins and ameliorating leaky gut 69,70 . The second theory attributed the beneficial effects of AMPs on tight junctions to their indirect roles in manipulating microflora populations in the intestine. In detail, previous studies showed that the intestinal commensal bacteria like Bifidobacteria and Lactobacilli secrete butyric acid that regulates epithelial O 2 consumption and stabilization of hypoxia-inducible factor. This transcription factor protecting the epithelial barrier against pathogens, resulting in higher expression of junctional proteins 71,72 . Therefore, it can be hypothesized that AMP in the current study upregulated the expression of junctional proteins by both reducing the number of C. perfringens and inhibiting protein disruption by bacterial toxins. Surprisingly, the antibiotic did not change the expression of CLDN1 and OCLN transcripts in the jejunum of chickens, while it could be expected that the antibiotic upregulated the junctional proteins due to the antibacterial nature of antibiotics. In line with the current results, Yi et al. 69 reported that antibiotics might not affect the gene expression of junctional proteins of the epithelial cells after pathogen removal, maybe because of controlling the microbial balance in the intestine.
Along with junctional proteins, the luminal mucus layer comprising of mucins plays a defensive role against invasive pathogens 73 . MUC2 widely expresses in goblet cells and secretes into the intestinal lumen to stabilize mucosal layer 73,74 . Any damage to the mucosal layer stimulates the expression of MUC2 to secrete more mucin Scientific Reports | (2020) 10:17704 | https://doi.org/10.1038/s41598-020-74754-x www.nature.com/scientificreports/ and prevent further destruction 74,75 . In the current study, NE significantly increased the gene expression of MUC2 in the jejunum, which is in agreement with the results of previous studies 76,77 . On the other hand, the antibiotic and AMP significantly downregulated the level of this transcript, while the results for AMP was similar to those of NC group. According to the bacterial results in the present study, it could be inferred that the inhibitory effects of AMP on the population of C. perfringens and E. coli might reduce the colonization of these bacteria in the intestine, decrease the destruction of the mucosal layer, and subsequently lessen the expression of MUC2 transcript. The exact mechanism of these effects has not yet been revealed.
In conclusion, results of the current study propose that cLFchimera, an antimicrobial peptide originating from camel milk, could reduce mortality and attenuate NE-induced lesions in broilers. Beneficial consequences of AMP use include better growth performance and recovery of villi morphology in the jejunum of NE-imposed chickens. Further, supplementing NE challenged birds with cLFchimera restored the ileal microflora and consequently regulated the expression of cytokines, MUC2, and tight junctional proteins. Therefore, according to the desired results obtained in the present study, cLFchimera can be nominated as a candidate for replacing growthpromoting antibiotics against NE in chickens, while further studies may find other favourable effects of this AMP.

Data availability
All generated and analysed data in the current study are included in this article, and also cited data were included in the reference list.