Bacterial infection in camels causing pneumonia with special emphasis on its antibiotic resistance

Document Type : Original researches

Abstract

This study aimed to identify some of the bacterial causes of pneumonia in camel.
A total of 100 lung samples from slaughtered imported camel were taken. Samples were subjected to bacteriologi]=al examination, antibiotic susceptibility testing and molecular characterization of some antibiotic resistant genes. The results showed that the total prevalence of pneumonia in the examined lung samples were 86%. 
 
In addition, the prevalence of the isolated bacteria were; S. aureus, Streptococcus pyogenes, Klebsiella pneumonia and Mycobacterium bovis with a percentage of 38, 31, 13 and 4; respectively. Antimicrobial susceptibility testing of most isolates indicated the presence of multidrug resistant strains. Molecular characterization of some antibiotic resistance genes indicated the presence of blaz, Aac(6'), Pbp1A, erm B, Tet (B) in the examined different types of bacterial isolates. In addition, Mpb70 as a specific gene for M. bovis. Public health significance and recommendations were discussed.

Keywords

Full Text

Bacterial infection in camels causing pneumonia with special emphasis on its antibiotic resistance.

Eman Mahrous1, Enas M. Abdel Ghany2, EL-Sayed Abdel Rahmen3 and El Sayed El Sawy4

1 Bacteriology Department, Animal Health Research Institute, Agriculture Research Center (ARC)

2 Gernetic Engineering Department, Faculty of Agriculture, Munofia University.

3 General supervisor of central Abattoir of Cairo

4 Serology and Bank of isolates Unit, Animal Health Research Institute, Agriculture Research Center (ARC)

 

Abstract:

This study aimed to identify some of the bacterial causes of pneumonia in camel.

A total of 100 lung samples from slaughtered imported camel were taken. Samples were subjected to bacteriological examination, antibiotic susceptibility testing and molecular characterization of some antibiotic resistant genes. The results showed that the total prevalence of pneumonia in the examined lung samples were 86%. 

In addition, the prevalence of the isolated bacteria were; S. aureus, Streptococcus pyogenes, Klebsiella pneumonia and Mycobacterium bovis with a percentage of 38, 31, 13 and 4; respectively. Antimicrobial susceptibility testing of most isolates indicated the presence of multidrug resistant strains. Molecular characterization of some antibiotic resistance genes indicated the presence of blaz, Aac(6'), Pbp1A, ermB, Tet (B) in the examined different types of bacterial isolates. In addition, Mpb70 as a specific gene for M. bovis. Public health significance and recommendations were discussed.

Key words: Antibiogram- Antibiotic resistance genes- Camel - Pneumonia.

Introduction:

The dromedary camels in Africa represent approximately 74% of the global camel population. They have a very high socio-economic value and serve as an essential source of meat and milk for humans (Rhodes et al., 2015).

International trade has long been recognized as a vector for food born infections and has been held responsible for introducing new strains of pathogens into susceptible population; this is why many countries had introduced strict regulations for imported meat so as to save the consumers health. The problem would have a far reaching sequellae when living animals are imported and disseminate the organisms to the environment until they are slaughtered (Asadi et al., 2023 and Davis et al., 2018).

Multiple stressing factors as rearing systems, climatic changes, unhygienic conditions, and sudden changes in feed with low level herd health status were stated to be risk factors associated with bacterial and viral causes induced pneumonia with camels. Pneumonia outbreaks in camels were usually observed during the change from dry to rainy seasons (Ben Chehida et al., 2021).

However, Camels were formerly assumed to be immune to the majority of livestock illnesses; but new research has proved their susceptibility to a wide range of infections, and camels are regarded to function as a carrier or reservoir for the spread of various animal diseases and zoonoses (Mai-siyama et al., 2014)

Wide varieties of bacteria were isolated from infected lungs of diseased camels including Staphylococcus aureus , Escherichia coli , Klebsiella pneumoniae , Bacillus spp. , Streptococcus pyogenes  pyogenes , Corynebacterium spp. , Pasteurella spp. , and Arcanobacterium pyogenes (Ismael et al., 2014; wareth et al., 2014; Abd El Tawab et al., 2016; Gebru et al., 2018).

 In addition, Tuberculosis (TB) is a chronic, reportable gran­ulomatous zoonosis caused by Mycobacterium tuber­culosis complex and affects many animal species including camels (OIE, 2016).

Clinical bacterial isolates frequently exhibit resistance to these antibiotics through the enzymatic alteration. There are five kinds of aminoglycoside- modifying enzymes (AME) occurring in Staphylococci spp., AAC (6') and blaz genes were studied by Hauschild et al. (2008).

In Klebsiella pneumoniae isolates, TetA (B) gene was identified to be the most prevalent tetracycline resistance determinant (Bokaeian et al., 2014).

We have investigated the role of Pbp 1A in penicillin resistance in and erm gene renders Streptococcus pyogenes isolates resistant to most macrolides, lincosamides, and streptomycin B compounds (Uruén et al., 2022).

This study aim to demonstrate different microbial hazards from apparently healthy slaughtered imported camels and antibiogram profile for the isolated bacteria. In addition, detection of antibiotic resistance genes in the most prevalent isolates.   

Materials and Methods

Ethical approval: All procedures performed in this study, including the collection of samples, were in accordance with the Egyptian ethical stan­dards of Animal Health Research Institute, and the Animal Rights and Ethical Use Committee of Agriculture Research Center, Animal Health Research Institute, Dokki, Giza, Egypt.

Sampling: Lung samples were collected from one hundred slaughtered camels. PM examination was performed fol­lowing previously described procedures by Taiwo (2005).

Isolation and identification of Gram positive and Gram negative bacteria according to Quinn et al. (2011).

The surface of collected tissues was burned by hot scalpel blade and inoculum samples were taken from the inner part of the lung using sterile cotton swab, After 24h of incubation in broth, the cultures were mixed; aloopful of the culture was streaked over a 7% sheep blood agar, MacConkey agar, Mannitol salt agar and Edward’s media and incubated aerobically at 37°C for 24h. Primary identification of

the bacteria was performed using colony morphology, Gram reaction, cellular morphology, catalase and oxidase tests. Final identification was carried out by subjecting pure cultures of single colony type into a

series of secondary biochemical tests, namely, methyl-red, indole, citrate utilization, coagulase, motility, TSI, esculin hydrolysis, as well as sugar fermentation tests, as required for each bacterial spp. All media were purchased from Hi media®

                                            

Isolation and identification of Mycobacteria according to Marks technique (1972): The samples were examined for the isolation and identification of M. bovis using conventional methods such as direct smear, culture, and biochemistry and molecular methods such as PCR.

Antibiotic susceptibility testing: isolates cultivated into Muller Hinton broth tubes and incubated aerobically at 37 ͦ C for 18hr and then cultured into Muller Hinton agar plates and incubated as above for antimicrobial susceptibility testing, which was carried out by the standard disk diffusion method according to CLSI (2022). The following antibiotic discs were used, Ampicillin (AMP, 15µg), Cephalexin (CL, 30µg), Clindamycin (DA, 10µg), Gentamicin (CN, 10µg), Imipenem (IMP, 10µg), Ofloxacin (OFX, 10µg), Rifampicin (RF, 5µg), Streptomycin (S, 10µg) and Tobramycin (TOB, 10µg).Antibiotic sensitivity in relation to zone of inhibition interpreted by the Manufacturing Company MAST® group.

Molecular characterization of isolates:

  • For DNA isolation: from Gram negative bacteria according to Wilson (1997),5 ml of the bacterial inoculated culture was spinned in a microcentrifuge at 10000 rpm for 2mins., or until a compact pellet forms. The supernatant was discarded. The pellet was resuspended in 570μl of TE, SDS (final concentration, 0.5%), and proteinase K (final concentration, 100 mg mL−1), and incubated at 37°C for 1h. To this mixture, 100ml of 0.8 M NaCl and 80μl of CTAB/NaCl (10% CTAB in 0.7 MNaCl) were added, and the microtubes were incubated for 10min. at 65°C. An equal volume of phenol/chloroform/isoamyl alcohol was added, extracted thoroughly, and spinned in a microcentrifuge at 10000rpm at 4°C for 5min. The supernatant was transferred to a fresh tube. 0.6vol isopropanol was added to precipitate the nucleic acids and spinned in a microcentrifuge at room temperature. The DNA was washed with 70% ethanol to remove residual CTAB and respin at 10000 at room temperature rpm for 5min to re-pellet it. The pellet was re-dissolved in 100µl TE buffer. Due to a high concentration of peptide and cross-bond peptides in the cell wall, Gram positive species are often more resistant to cell lysis. It required addition of lysozymes to the lysis buffer (Schindler and Schuhardt, 1964; Ezaki and Suzuki, 1982; Zschöck et al., 2000; Mason et al., 2001).

 

  1. Oligonucleotide Primer: The primers used were provided by Metabion (Germany), and they are listed in Table (1).

Table (1): Primers sequences, target genes, amplicon sizes and cycling conditions for conventional PCR.

Bacterial Spp.

Target gene

Primers sequences

Amplified segment (bp)

Initial

denaturation

Amplification (35 cycles)

Final extension

Reference

Secondary denaturation

Annealing

Extension

Mycobacteria Spp.

Mpb70

ACCCTCAACAGCGGTCAGTAC

TTACGCCGGAGGCATTAGCAC

314

95ºC

5min

94ºC

1min

55 ºC

1min

72 ºC

1min

 

72 ºC

10min

 

Zhang et al. 2016

S. aureus

Blaz

GAAGTACGCAGAAGAGA

ACATGGCAAGCTCTAGGA

173

95ºC

5min

94ºC

1min

54 ºC

1min

72 ºC

1min

72 ºC

10min

Martineau et al. 2000

Aac(6')

ACTTCAACACCTGCTGCTTTC

TGACCACTTTTATCAGCAACC

491

95ºC

5min

94ºC

1min

57 ºC

2min

72 ºC

30S

Choi et al. 2003

Streptococcus pyogenes  Spp.

Pbp 1A

AGGGGTAGTAGCATTACCAT

CAACTATATGACTGGGATCG

939

95ºC

5min

95ºC

30S

47 ºC

30S

72ºC

30S

72ºC

10min

Kannika et al. 2017

 

ermB

GAAAAGGTACTCAACCAAATA

AGTAACGGTACTTAAATTGTTTAC

639

95ºC

15min

94ºC

20S

53ºC

20S

72ºC

40S

Sutcliffe et al. 1996

Klebsiella pneumoniae Spp.

Tet (B)

CCTCAGCTTCTCAACGCGTG

GCACCTTGCTCATGACTCTT

633

95ºC

5min

94ºC

1min

52ºC

30S

72ºC

1min

 

72ºC

10min

Walker et al. 2001

 

 

Results:

Table (2): prevalence of bacterial isolates from the examined lung samples

Total no.

Positive samples

Negative samples

100

No.

%

No.

%

86

86%

14

14%

 

This table showed the prevalence of pneumonia in the examined camel lung samples. Out of examined 100 lung sample, there were 86(86%) positive samples and 14(14%) negative for bacteriological examination.

Table (3): Frequency of bacterial isolates from lung lesions of camel (n=100)

 

Type of infection

 

Isolated Microorganism

Total Number

Percent

Single infection

Staphylococcus aureus

38

38%

Streptococcus pyogenes

31

31%

Klebsiella pneumoniae

13

13%

Mycobacterium bovis

4

4%

Mixed infections

Staphylococcus aureus & Streptococcus pyogenes  

20

20%

Staphylococcus aureus, Streptococcu and Klebsiella pneumoniae

5

5%

 

This table showed the Frequency of bacterial isolates from lung lesions of camel. Some lung lesions showed single bacterial infection others showed mixed infections. Out of examined 100 lung sample, there were 38 (38%) Staphylococcus aureus isolates; Streptococcus pyogenes 31(31%); K. pneumoniae 13(13%) and M. bovis 4(4%). Mixed bacterial infection was detected as Staphylococcus aureus and Streptococcus pyogenes as 20% and Staphylococcus aureus, Streptococcus pyogenes and K. pneumonia as 5%.

Table (4): Results of antimicrobial susceptibility for the isolates:

Antibiotic classes

Antimicrobial agents

S. aureus

(N=10)

Streptococcus pyogenes

(N=10)

K. pneumoniae

(N=10)

 

S.

R.

S.

R.

S.

R.

  

β- lactamases

  

Penicillin

Ampicillin

4

6

0

10

8

2

 

Carbapenem

Imipenem

2

8

0

10

7

3

 

Cephalosporin

Cephalexin

4

6

0

10

9

1

 

Aminoglocosides

Gentamicin

9

1

10

0

8

2

 

Streptomycin

7

3

10

0

7

3

 

Tobramycin

4

6

10

0

8

2

 

Flouroquinolone

Ofloxacin

9

1

10

0

9

1

 

Macrolids

Rifampicin

6

4

0

10

2

8

 

Clindamycin

5

5

10

0

3

7

 

 

Results in table (4) revealed that, out of tested ten S. aureus isolates, most isolates were resistant to all used β- Lactamases group of antibiotics. Concerning used Aminoglocosides antibiotics, out of tested ten isolates to Gentamicin, streptomycin and Tobramycin, there were 1, 3 & 6 resistant strains: respectively.

Only one S. auresus isolates showed resistance to Ofloxacin. In addition, in testing the sensitivity to Macrolides such as Rifampicin and Clindamycin, there were 4 and 5 resistant strains: respectively.

All isolated Streptococcus pyogenes showed resistance to all used β- lactamases group of antibiotics, sensitive to all used Aminogolcosides and Flouroquinolones.

In addition, all isolates were resistant to Rifampicin and sensitive to Clindamycin. Klebsiella pneumoniae isolates showed high sensitivity to Flouroquinolones and Cephalosporins and high resistance to Macrolides.

Table (5): Available review on bacteria isolated from camels in Egypt

Authors

Examined sample type

Most predominant isolated bacteria

Refai at al. (1984)

Lymphnodes

Salmonella spp.

Ali et al. (1987)

Uterine sample

Citrobacter spp. and E. coli

Mostafa et al. (1987)

Raw milk

Staph spp., E. coli and C. perfrengens

El- Sayed et al. (1987)

Raw milk

Salmonella spp. and Citrobacter spp.

El Seedy et al. (1990)

Uterine sample

Protus spp

Powers et al. (1990)

Uterine sample

E. coli

Tibary Anouassi (1997)

Uterine sample

Pseudomonas aeruginosa

Tibary et al. (2006)

Uterine sample

Klebsiella pneumoniae pneumonia

Hanan et al. (2010)

Uterine sample

E. coli, Salmonella spp., Pseudomonas aeruginosa, Klebsiella pneumoniae pneumoniae, Protus and Citrobacter spp.

Abo-El naga and Osman (2012)

Lung samples

Bacillus spp., Staphylococcus spp., Streptococcus pyogenes , Klebsiella pneumoniae and E. coli

Ismail et al. (2014)

Lung, blood, nasal & tracheal swabs

Bacillus spp., Staphylococcus spp., Pseudomonas spp., Klebsiella pneumoniae spp and E. coli

Wareth et al. (2014)

Lung samples

Bacillus spp., Staphylococcus spp., Streptococcus pyogenes  Spp., Klebsiella pneumoniae spp and E. coli and Corynebacterium spp.

Nahed et al. (2017)

Lung tissues, blood samples and nasopharyngeal swabs.

K. Pneumoniae, S. aureus, Shigella spp., E. coli, Proteus spp., P. aeruginosa and Pasteurella spp.

El- Harriri et al. (2017)

Meat samples

Pseudomonas spp.

Al Amery et al. (2019)

Meat samples

Staphylocoocus aurus

El- Naker (2019)

Serum samples

Mycobacterium bovis

Shahin et al. (2021)

Diarrheic neonatal camel

E. coli

 

Discussion:

The respiratory tract of apparently healthy animals acts as a reservoir for many species of microorganisms that reached the nasal cavity through various ways. This study has shown that a wide variety of bacterial species colonize the respiratory passageways of camels in the study area. This is supported by several researchers in Egypt who previously demonstrated diverse bacterial species from various regions of the camel respiratory tract: nasal tracts, tonsil, trachea and lungs (Ismail et al. 2014; Wareth et al. 2014; Ahmed and Musa 2015 and Nahed et al., 2017).

The consistent isolation of these organisms from the pneumonic lungs of various species of animals might indicate their role in causing different respiratory infections especially when the immune system of the animal is compromised by some other external factors. The normal bacterial flora of a healthy individual can be altered by several factors such as changes in the hygienic condition, environmental and climatic conditions, and nutritional and immunological status of the animal. Such factors could lower the resistance of the lung tissue and the existing organism most probable would get the upper hand, leading to the presentation of a variety of pathologies (Bosch et al. 2013).

Tables (2) and (3) showed the prevalence of pneumonia in the examined camel lung samples. Out of examined 100 lung sample, there were 86(86%) positive samples and 14(14%) negative for bacteriological examination.

In the examined lung samples, there were single bacterial infection; S. aureus, Streptococcus pyogenes, Klebsiella pneumonia and M. bovis as well as mixed bacterial infections. Similar bacterial isolates were detected by Bani Ismail (2017).

Staphylococcus aureus is known to occur as a commensal on the skin, the nose, and mucous membranes of healthy humans and animals and also an opportunistic pathogen in multiple infectious diseases (Lozano et al. 2016).                                

In this study, S. aureus was the commonest bacteria in the pneumonic lungs, 38%, which is higher when compared to the report of Azizollah et al. (2009), Wareth et al. (2014), Ismail et al. (2014), Hussain et al. (2017) and Al-Amery et al. (2019) as 14, 14.5, 37.1, 24.8 and 14.5 percentages; respectively, from lungs of apparently healthy camels.  Higher results were obtained by Ben Chehida et al. (2021) who isolated S. aureus from (95.6%) examined samples. The present and previous data suggest that the bacteria reside as a normal inhabitant of upper respiratory tract and possibly as a causative agent of secondary pneumonia.

Most species of the genus Streptococcus are considered potential pathogens, occur in nature, and some are commensal in the respiratory, genital, and alimentary tracts and skin of animals and man (Parks et al. 2015). Our results showed that, out of examined 100 lung sample, Streptococcus pyogenes were isolated from 31(31%).  Streptococcus pyogenes have been isolated from clinically healthy camels although they were not definitely identified and characterized (Azizollah et al. 2009). Lower results were obtained by Wareth et al. (2014) as 10% isolation rate. On the contrary, higher isolation rate were detected by Ahmed et al. (2015) as 94% from examined pneumonic lung.

Klebsiella pneumoniae was recovered at an enormously comparable frequency from the pneumonic and healthy lungs. Our results showed that, out of examined 100 lung sample, Klebsiella pneumonia was recovered from 13 (13%). Al-Doughaym et al. (1999) recorded similar results from the lungs of pneumonic camels 10.9%. Higher isolation rates were reported by Wareth et al. (2014) and Nahed et al. (2017) as 26.7 and 44.0%; respectively.  Lower figures have also been reported by Abubakar et al. (2010) in Nigerian and Ismail et al. (2014) and Ahmed and Musa (2015) in Egypt as 6.3, 1.8 and 0.1% percentages; respectively from apparently healthy camels.

Several studies on camel TB have been conducted in several countries, including Egypt, confirming the occurrence of TB in camel populations (Koni et al., 2016)

A high prevalence of camel TB is usually found among farmed camels and those in close proximity to cattle, which are mainly affected by Mycobacterium bovis (Bennet et al., 2014). The transmission of M. bovis between animals primarily occurs through aerosols, direct contact, sharing the same food and water and suckling (El-Sayed et al., 2016).

The prevalence of TB in camels based on bacteriological examination was 4% (Table 3). Higher TB prevalence rate were obtained by Beyi et al. (2014), Narnaware et al. (2015), Jibril et al. (2016), Ahmad et al. (2019), and Elnaker et al. (2019) who reported a prevalence rate of 8.3, 19.56, 9.82, 33.4 and 60.87 percentages; respectively. On the other hand, a lower TB rate in Egypt than that obtained in this study was reported by Manal and Gobran (2008), who concluded that the prevalence of TB in camels was 0.7%.

Concerning the mixed bacterial infection which dominated by S. aureus and Streptococcus pyogenes then S. aureus, Streptococcus pyogenes and Klebsiella pneumoniae were detected as 20% and 5% of examined lungs; respectively. These findings were explained by Mostafa (2004) who stated that, the pulmonary mixed infection is commonly detected because the respiratory air passages act as a reservoir for potential pathogenic microorganisms which develop pneumonia on the onset under stress factors, poor sanitation, and climatic conditions.

Pneumonic mixed pathogens demonstrated the complexity of the disease where S. aureus may predispose infection by other pathogens. These results agree with Taha et al. (2007), Sayed and Zaitoun (2009), Abo El naga and Osman (2012) and Gebru et al. (2018).

In addition, the failure to isolate bacteria from some examined lung tissues with lesions might be due to the involvement of other pathogens such as anaerobic bacteria, virus, Mycoplasma, fungi and may be parasites (Lopéz, 2001).

Furthermore, this study assessed the antibiotic susceptibility profiles of the bacterial isolates in order to choose the most effective antimicrobial agents that could be used to treat camels with respiratory problems as shown in table (4) which revealed that, out of tested ten S. aureus isolates, most isolates were resistant to all used β- Lactamases group of antibiotics. Concerning used Aminoglocosides antibiotics, out of tested ten isolates to Gentamicin, streptomycin and Tobramycin, there were 1, 3 & 6 resistant strains: respectively. Only one S. auresus isolates showed resistance to Ofloxacin. In addition, in testing the sensitivity to Macrolides such as Rifampicin and Clindamycin, there were 4 and 5 resistant strains: respectively.

All isolated Streptococcus pyogenes showed resistance to all used β- lactamases group of antibiotics, sensitive to all used Aminogolcosides and Flouroquinolones. In addition, all isolates were resistant to Rifampicin and sensitive to Clindamycin. Klebsiella pneumoniae isolates showed high sensitivity to Flouroquinolones and Cephalosporins and high resistance to Macrolides.

Findings in table (5) were similar to Al Amery et al. (2019) and Ben Chehida et al. (2021) who find similar antibiogram profile for isolated S. aureus. Simlar anti-biogram profile of Streptococcus pyogenes was detected by Ahmed et al. (2015) and Mutua et al. (2017). Accordingly, increased level of resistance among the respiratory pathogens against the commonly used antimicrobials in respiratory tract infections was observed. There was agreement in presence of multidrug resistant strains with the results of Elhariri et al. (2017). The high rate of resistance observed in many of the isolates could be either because they are frequently and unnecessarily prescribed or sold over the counter in the open market and private veterinary drug shops without prescription. Therefore, there is a need for practitioners and researchers to be aware of the bacterial flora of the camels and of their antibiotic sensitivities to be informed of the appropriate antibiotics to be used in the course of respiratory infections and control programs (Shryock and Richwine, 2010 and Ding and He, 2010).

Transfer of resistance in bacteria has been documented to occur between different animal species, within humans, from animals to humans, and from humans to animals (Mutu et al., 2017).

In studying the resistance pattern of the isolated bacteria Fig. (1), (2), (3), (4) and (5) showed the different amplified fragments of different detected antibiotic resistance genes. In addition,  Fig. (6) Showed the amplified fragment of M. bovis specific gene.

Clinical bacterial isolates frequently exhibit resistance to these antibiotics through the enzymatic alteration of aminoglycosides. Staphylococci, streptococci, and enterococci are gram-positive cocci. AAC (6') has a particular significance because it modifies aminoglycosides of therapeutic importance, including kanamycin, tobramycin, and gentamicin, respectively (Abo-State et al., 2018).

Penicillin resistance in staphylococci is caused by several methods. The most important method is the resistance due to a penicillin-binding protein, PBP2a, encoded by mecA, and is primarily connected to human isolates. Investigations into blaZ-encoded penicillin resistance have been considerable. Additionally, blaZ has been linked to penicillin resistance in coagulase-negative staphylococci (CoNS).

 (Liao et al., 2017).

Enterobacteriaceae family members such as Klebsiella pneumoniae often produce ESBLs; however, other genera of the Enterobacteriaceae family have recently been reported to contain some other enzymes.

Tetracycline has been used regularly to treat various diseases, but regrettably this has led to the emergence of resistance forms. In prior clinical surveys, tetA (B) gene was identified as the most prevalent tetracycline resistance determinant with a wide host range since it resides on highly mobile genetic elements that readily transfer between different bacterial genera (Bokaeian et al., 2014).

Penicillin inhibits the growth of streptococci by the inactivation of penicillin-binding proteins (PBPs). Streptococcal resistance to penicillin is due to the production of altered PBPs which have a decreased affinity for the antibiotic. We have investigated the role of PBP 1A in penicillin resistance and confirm that that alteration of PBP 1A plays a vital role in full penicillin resistance development.

In addition, Target modification occurs at the level of the ribosomes via an erm gene encoding a 23S rRNA methylase. There are currently at least eight classes of erm genes distinguishable by hybridization criteria. Erm methylases add either one or two methyl residues to a highly conserved adenine residue in domain V, the peptidyl transferase center, of 23S rRNA. Uruén et al. (2022).

In Streptococcus pyogenes, two specific primers were used, ermB and Pbp1A. ermB product was 639bp which was compatible with Uruén et al. (2022). Like Kannika et al. (2017) the amplified fragment of PbP1A gene was 939. Penicillin inhibits the growth of pneumococci by the inactivation of penicillin-binding proteins (PBPs).

Concerning S.aureus isolates, blaZ and AAC6' genes were detected. The obtained PCR product was 173bp and 491bp; respectively. Our results agreed with Martineau et al. (2000) and choi et al. (2003); respectively.

All tested Klebsiella pneumoniae isolates harbored Tet B gene. The amplified fragment was 633bp and these results agreed with Bokaeian et al. (2014).  Mpb70 gene of Mycobacteria bovis was detected in all tested isolates.  The amplified fragment was 314bp which was like Zhang et al. (2017).

Table (5) showed the available  literature for several studies on camel in Egypt. From 1967  to 2022. These studies discussied either live animal samples such as raw milk samples, diarrheic samples, Genital tract washes, nasal and tracheal swabs or slaughtered camel samples from abbattoir including meat samples, lymphnodes, lung samples and genital tract samples.

In conclusion, the present study in this area pointed out that respiratory infection is considered as the major cause of morbidity and mortality in camels. It is a multifactorial process among which a variety of bacterial species have been associated with respiratory problems. Furthermore, our isolates have shown considerable resistance to commonly prescribed antimicrobials in the country calling for the need to conduct susceptibility testing for control of camel respiratory infections in the area.

Recommendations:

  • controlling respiratory diseases of the camel’s should give due attention in alleviating stress during different managemental practices including transportation, lairaging, feeding, watering, etc. and on those measures that has to be taken during stressful conditions.
  • Transborder camel movements should be controlled.
  • Abattoir workers should be educated to avoid infecting themselves or spreading the pathogens.
  • Proper abattoir records can serve as indicators for field disease conditions and consequently aid in planning, prevention and control programs by relevant authorities.
  • Restrictions for abuse of antibiotics in livestock production to avoid the emerging of antibiotic resistant pathogens.

 

 

 

 

 

Fig. 1 Agarose gel electrophoresis of PCR products showing amplification of Streptococcus pyogenes  spp ermB gene products at 639bp. MWM-molecular weight marker (100-1000bp DNA ladder) + control (positive, negative), all Ten  isolates were positive for ermB gene.

 

 

 

 Fig. 2 Agarose gel electrophoresis of PCR products showing amplification of Streptococcus pyogenes  Pbp1A gene products at 939bp. MWM-molecular weight marker (100-1000bp DNA ladder). + control (positive, negative), all Ten isolates were positive for pbp1A gene.

 

Fig.3 Agarose gel electrophoresis of PCR products showing amplification of S. aureus blaz gene products at 173bp. MWM-molecular weight marker (100-1000bp DNA ladder) + control (positive, negative), all Ten isolates were positive for blaZ gene.

 

Fig.4 Agarose gel electrophoresis of PCR products showing amplification of S. aureus aac(6) gene products at 491bp. MWM-molecular weight marker (100-1000bp DNA ladder) + control (positive, negative), all Five isolates were positive for aac(6) gene.

 

 

Fig.7 Agarose gel electrophoresis of PCR products showing amplification of K. pneumoniae TetA(B) gene products at 633bp. MWM-molecular weight marker (100-1000bp DNA ladder) + control (positive, negative), all six isolates were positive for TetA (B) gene.

Fig.8 Agarose gel electrophoresis of PCR products showing amplification of M. bovis specific mpb70gene products at 314bp. MWM-molecular weight marker (100-1000bp DNA ladder) + control (positive, negative), all Four isolates were positive for mpb70 gene.

 

 

 

 

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