Overview on the mastitis syndrome in cattle in Al-Sharkia governorate

Document Type : Original researches

Abstract

This study was conducted to determine bovine mastitis resistance genes of common etiological agents in Al-Sharkia province. In addition to monitor the changes in antioxidants profile, oxidative stress status and some of biochemical markers in dairy cows suffered from clinical mastitis. It was carried out on forty dairy cattle (40) aged from 4 – 6 years (20 healthy and 20 mastitic) from dairy farms and individual cases in Al-Sharkia Governorate, dependent on the findings of the clinical examination, the cattle were divided into 3 groups. Gp1 healthy dairy cattle (control), Gp2 mastitic dairy cattle before treatment, Gp3 mastitic dairy cattle after treatment. The clinical symptoms of mastitis including milk and udder were reported in Gp2. Within the bacterial isolates (20) it was noticed that the highest spread was of Staphylococcus aureus (10) followed by E.coli (6) and Klebsiella Spp. (4). Antibiotic sensitivity test displayed that gentamycin, streptomycin were the more sensitive antibiotics for S. aureus, E.coli and Klepsiella. While amoxicillin and clavulanic acid, tetracycline, florfenicol and cefotaxime were the more resistant antibiotics. Enrofloxacin was moderate sensitive in s. aureus and E.coli while more resist in Klebsiella. Real time PCR assay was used for detection of antimicrobial resistance genes. Eleven isolates representing, 5 S. aureus, 3 Klebsiella and 3 E.coli were selected for detection of multi drug resistant (MDR) genes. The blaTEM gene was detected in all isolates of S. aureu, E. coli and 2 isolates of Klebsiella. While, the tetA gene was detected in 4 out of 5 isolates of S.aureus and all isolates of E.coli and Klebsiella. Moreover, floR gene was detected in 3 isolates of S.aureus, 2 isolate of E.coli and all isolates of Klebsiella. Biochemically, there were significantly increases in serum AST, ALT, ALP, urea, creatinine, Na, Mg, NO, PH, beta 1, total beta, total globulin and milk MDA associated with non-significant increases in t.protien, alpha 1, total alpha, gamma 1, gamma 2 and total gamma. Meanwhile, there were a significant decrease in serum Cl, Ca, K, TAC, beta 2, A:G ratio and milk SOD, CAT, GSH, associated with non-significant decrease in alpha 2. On the other hand, there were significant increases in serum albumin, immune-globulin and other proteins in whey milk, meanwhile, there were a significant decrease in α–lactoglobulin and ß- lactoglobulin in whey milk in mastitic group when compared with normal healthy cows. The results of the current investigation suggested that the body antioxidant defense system was compromised in dairy cows with clinical mastitis generating a state of oxidative stress.

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Overview on the mastitis syndrome in cattle in Al-Sharkia governorate

Nour E.M.*, Marwa F. Hassan**, Taha M.F.***, Asmaa G. Abd El Monsef*, Nermin F. El Zohairy*, Al.Afifi, S.H.H.**** and Azza Zakaria***.

* Biochemistry, Toxicology and Feed Deficiency Dept., Animal Health Research Institute (AHRI), Agriculture Research Center (ARC), Zagazig branch, Egypt.

**Biochemistry, Toxicology and Feed Deficiency Dept, Animal Health Research Institute (AHRI), Agriculture Research Center (ARC), Dokki, Giza, Egypt.

***Bacteriology Dept., Animal Health Research Institute (AHRI), Agriculture Research Center (ARC), Zagazig branch, Egypt.

**** Biochemistry Dept., Animal Health Research Institute (AHRI), Agriculture Research Center (ARC), Tanta Provincial Lab, Egypt.

ABSTRACT

This study was conducted to determine bovine mastitis resistance genes of common etiological agents in Al-Sharkia province. In addition to monitor the changes in antioxidants profile, oxidative stress status and some of biochemical markers in dairy cows suffered from clinical mastitis. It was carried out on forty dairy cattle (40) aged from 4 – 6 years (20 healthy and 20 mastitic) from dairy farms and individual cases in Al-Sharkia Governorate, dependent on the findings of the clinical examination, the cattle were divided into 3 groups. Gp1 healthy dairy cattle (control), Gp2 mastitic dairy cattle before treatment, Gp3 mastitic dairy cattle after treatment. The clinical symptoms of mastitis including milk and udder were reported in Gp2. Within the bacterial isolates (20) it was noticed that the highest spread was of Staphylococcus aureus (10) followed by E.coli (6) and Klebsiella Spp. (4). Antibiotic sensitivity test displayed that gentamycin, streptomycin were the more sensitive antibiotics for S. aureus, E.coli and Klepsiella. While amoxicillin and clavulanic acid, tetracycline, florfenicol and cefotaxime were the more resistant antibiotics. Enrofloxacin was moderate sensitive in s. aureus and E.coli while more resist in Klebsiella. Real time PCR assay was used for detection of antimicrobial resistance genes. Eleven isolates representing, 5 S. aureus, 3 Klebsiella and 3 E.coli were selected for detection of multi drug resistant (MDR) genes. The blaTEM gene was detected in all isolates of S. aureu, E. coli and 2 isolates of Klebsiella. While, the tetA gene was detected in 4 out of 5 isolates of S.aureus and all isolates of E.coli and Klebsiella. Moreover, floR gene was detected in 3 isolates of S.aureus, 2 isolate of E.coli and all isolates of Klebsiella. Biochemically, there were significantly increases in serum AST, ALT, ALP, urea, creatinine, Na, Mg, NO, PH, beta 1, total beta, total globulin and milk MDA associated with non-significant increases in t.protien, alpha 1, total alpha, gamma 1, gamma 2 and total gamma. Meanwhile, there were a significant decrease in serum Cl, Ca, K, TAC, beta 2, A:G ratio and milk SOD, CAT, GSH, associated with non-significant decrease in alpha 2. On the other hand, there were significant increases in serum albumin, immune-globulin and other proteins in whey milk, meanwhile, there were a significant decrease in α–lactoglobulin and ß- lactoglobulin in whey milk in mastitic group when compared with normal healthy cows. The results of the current investigation suggested that the body antioxidant defense system was compromised in dairy cows with clinical mastitis generating a state of oxidative stress.

    Key words:  Cattle - Mastitis- Oxidative stress - Electrophoresis- gene resistance.

INTRODUCTION

The economic value of dairy cows is especially de­termined via the milk yield and longevity. The main important factor affecting the quantity and quality of the produced milk is the manifestation of produc­tion diseases, mainly mastitis (Zajac et al. 2012). Bovine mastitis still one of the most serious conditions of dairy cows globally (FAO 2014; Abebe et al. 2016). Aside from the significant economic losses related to the disease, mastitis has dangerous zoonotic potential and has been linked to the increasing development and the rapid emergence of multidrug resistance strains globally (Oliver et al. 2011; Beyene et al. 2017). Such hazards can mainly occur through the ingestion of contaminated milk, milk derivatives or direct contact with infected animals (Maity and Ambatipudi 2021).

Mastitis, which is the inflammation of the udder and teats, prevails in two primary forms: clinical as well as subclinical mastitis (reduction in milk production without clinical anomalies in udder or milk) (Ndahetuye et al. 2019). Clinical mastitis, which is less predominant, is distinguished by systemic indications in the cow and notable abnormalities in the milk and udder (Jamali et al. 2018), involving fever, depression, anorexia, lethargy, additionally a reduction in grooming could also transpire (Medrano Galarza et al. 2012; Dittrich et al. 2019).

Mastitis is more predominant when the mammary gland's immunological and antioxidant defense mechanisms are compromised. Dairy cows are subjected to numerous physiological, genetic, and environmental factors related to both the host and pathogens, which can suppress the host’s immunity, hence, mastitis incidence increase (Andrei et al. 2016). Wide ranges of microbes have been registered as causative agents of mastitis worldwide (Jamali et al. 2018). These involve both environmental and contagious bacteria, as well as algae, fungi and viruses. Evidence-depended on research studies have revealed marked variance in the distribution of mastitis-causing pathogens and mastitis between countries, regions, and farms (Gao et al. 2017). These variances are affected by farm management practices with regional environmental factors (Amer et al. 2018).

Bacteria are the primary source of mastitis, and more than 140 different pathogenic species have been mentioned (Motaung et al. 2017). Staphylococcus aureus the most widespread contagious agent linked with mastitis, because this bacterium is persistent inside the udder (Rainard et al. 2018; Lamari et al. 2021). Escherichia coli is the most prevalent gram-negative coliform responsible for inducing environmental clinical mastitis (Campos et al. 2022), essentially because of high genotypic variation (Bag et al. 2021). Klebsiella pneumoniae is the second most prevalent cause of mastitis and, is assumed the most detrimental in dropping milk production and quality, as well as in economic terms. Even so it is categorized as an environmental pathogen, it has additionally been found to be transferred from infected to healthy animals (Cheng et al. 2021; Fu et al. 2022). Immediate identification as well as understanding diversity of pathogens related to mastitis is crucial for successful prevention and control (Bi et al. 2016). Antibiotics are being used indiscriminately as a result of improperly identifying the cause of mastitis, resulting in higher development rates and the quick generation of multidrug resistance strains (Sharma et al. 2018). Crucially, the indiscriminate applied of antibiotics to treat bovine mastitis has led to the generation of antibiotic-resistant bacteria in milk and dairy products, which is a critical concern (Singh et al. 2018). Therefore, this study aims to identify the bacteriological mastitis causative agent and antibiotic resistance genes, additionally to determinate the biochemical alteration, antioxidant enzymes and oxiditive stress role  associated with clinical mastitis in the Sharkia governorate.

MATERIAL AND METHODS

Ethical consent:

The experimental protocol was accepted by AHRI in conformity with the ARC and IACUC committee (ARC, AHRI, IACUC, 17/24).

AHRI approved the experimental protocol in accordance with the ARC and IACUC committee guidelines.

 

Materials:

Eosin Methylene Blue (EMB) Agar, Brain Heart Infusion (BHI) Agar, Mac-Conkey Agar, Manitol salt agar, Blood Agar, Baird Parker Agar (BPA) incorporated with egg-yolk tellurite emulsion and Muller-Hinton agar (MHA) (Hi Media, Mumbai) were purchased from Arena BioScien Company, Egypt. Antibiotics disks gentamicin (CN, 10 μg),  tetracycline (TE, 30 μg),Amoxicillin + clavulanic acid (Amc,30 μg), Cefotaxim (CTX,30 μg), Enrofloxacin (ENR,5 μg ), florfenicol(FFC,30) and Streptomycin (S,10 μg ) were obtained from Oxid Ltd. UK for microbiology media culture and diagnostic products. Different isolates that displayed phenotypic resistance were selected for the existence of anti-microbial resistant genes (5 S. aureus, 3 E.coli and 3 Klebsiella). For that purpose, Real Time PCR was applied to estimate the existence of genes encoding resistance to B-lactams (blaTEM), tetracycline (tetA) and florfenicol (floR), Oligonucleotide primers used were supplied from Metabion, Germany (table 1). Extraction of DNA from different isolates was applied using QIAamp DNA Mini kit (Qiagen, Germany, GmbH) Cat. No. 51304. Real Time PCR was performed using PanGreen™ Universal SYBR® Green Master Mix (purchased from Bio Helix) (table 2), the reaction was performed in a StepOne real time PCR system (table 3).

Table (1): Primers sequences, target genes and Ref.

Target gene

Primers sequences 5′- 3′

Reference

blaTEM

ATCAGCAATAAACCAGC0

Colom et al. 2003

CCCCGAAGAACGTTTTC

floR

GAACACGACGCCCGCTAT

Wang et al. 2013

TTCCGCTTGGCCTATGAG

tetA

GGTTCACTCGAACGACGTCA

Ng et al. 2001

CTGTCCGACAAGTTGGGTAA

 

Table (2): Reaction mix used for qPCR

Component

Volume

PanGreen™ Universal SYBR ® Green Master Mix (2x)

10 µl

Forward primer

1 µl

Reverse primer

1 µl

DNA template

5 µl

Nuclease-Free water

Up to 20  µl

Table (3): Thermal profile used in qPCR:

Stage

No of cycles

Program

primary denaturation

1

95°C for 5 min

Denaturation

40

95°C for 15 sec

Annealing

60°C for 60 sec

Extension

72°C for 10 sec

 

Treatment trails:

Mastitic cows were treated by the most sensitive antimicrobials in addition to non-steroidal anti-inflammatory drug.

  • BANAMINE® (flunixin meglumine, Merck Animal Health CO.) 1ml/45 kg b.wt., slow intravenous once daily for up to 3 days.
  • Gentamycin: (Gentamycin 10%, El Nasr pharmaceutical Chemicals Co.) each ml contains gentamycin 100mg.the recommended dose is 4ml/ 100 kg b. wt., i.m. twice daily for 3 successive days injection.
  • Streptomycin: (Pen and Strep, Norbrook Company) each ml contains: procaine penicillin 200mg, dihydrostreptomycin sulphate 250mg, was. The recommended dose rate is 4 ml / 100 kg.b.wt., i.m. for Three consecutive day.

Experimental design:

Forty cattle aged 4 – 6 years (20 healthy and 20 mastitic) from dairy farms and individual cases in Sharkia Governorate were divided into 3 groups. Gp1 healthy cattle (control), Gp2 mastitic cattle before treatment, Gp2 mastitic cattle after treatment. The clinical symptoms of mastitis were reported in Gp2.

Clinical assessment

All cattle were thoroughly checked according to Radostits et al. (2000), then the clinical findings were reported. Udder examination involved inspection with palpation of the udder to ascertain the size and consistency of different quarters additionally if any possible anomalies were present. The supra mammary lymph nodes were manually palpated to assess their size and look for any noticeable indurations.

Samples collection:

Collection of blood samples:

     Blood samples (about 7 ml), for serum obtaining, were collected from jugular vein from each group. Serum samples were obtained by centrifuging the blood samples at 3000 rpm for 7 minutes. Sera were separated and stored at -20°C until biochemical analysis.

Collection of milk samples:

Milk samples were taken from the affected quarters, while in healthy cow's milk sampling was taken from any quarter of the mammary gland. Teats were prepared aseptically before sample collection, according to the National Mastitis Council (1999). After cleaning and drying the mammary teats, we sprayed 70% ethanol and discarded some streams of milk. 50 ml of milk samples were collected in sterile screw-capped bottles and were targeted for the subsequent examinations and immediately transferred to the laboratory of bacteriological examination for isolation of the causative microorganisms, and also for biochemical analysis.

 

 

Microbiological examinations:

Milk samples delivered to the laboratory were mixed accurately and one loop full of the milk sample was inoculated on EMB Agar, BHI Agar, MacConkey Agar, Manitol salt agar, BPA incorporated with egg-yolk tellurite emulsion and Blood Agar. Then, these inoculated plates were incubated at 37˚C for 16-24 hours. The isolated bacterial colonies were exposed to gram’s staining for the identification of gram-positive and negative and were exposed to distinct biochemical tests (oxidase, catalase,  indole, Voges Proskauer’s, methyl red, triple sugar iron, citrate, etc) for assurance. The bacteriological culture and biochemical estimation for isolates were done according to National Mastitis Council (1999).

Antimicrobial susceptibility examinations:

Susceptibility was examined via Kirby–Bauer disk diffusion method on MHA. Pure cultures of S. aureus, Klebsiella spp and E coli were grown in brain heart infusion (BHI) broth, and then incubated at 37 °C for 18 hours. BHI broth cultures were additionally equally spread on MHA plates. After that, inoculated antimicrobial disks were left at room temperature for 30 min then incubated at 37 °C for 24 hours for inhibition zone diameter measurement. Strains were divided as resistant, susceptible, or intermediate based on the size of the inhibition zone (in millimeters) as well as minimum inhibitory concentrations (MICs) used for interpretation the diameters of inhibition zones were as depending on Clinical and Laboratory Standards Institute (2014).

Physical and biochemical examination of milk samples:

Whole milk pH

Fresh milk was used for pH analysis, pH reading was reported by digital pH meter (JENWAY,3510 manufactured in EU.)

Skimmed milk:

Milk samples were centrifuged at 3000 rpm for 15 min. The fat layer in each sample was removed, and the defatted milk was immediately stored at -20°C until analysis of some antioxidant and oxidative parameters (Colakoglu et al. 2017).

Whey milk:

     Whey milk was prepared from a 40-ml of skimmed milk sample by adding 0.6 ml of a 1:50 dilution of rennin and 0.4 ml of saturated calcium chloride, keeping at 37 °C for 30 min., then centrifuging for 5 min at 3000 rpm. Then whey was filtered and frozen till used (Kumar and Mikolajcik 1972).

Biochemical Analysis:

Activities of aspartate amino transferase (AST) and alanine amino transferase (ALT) were determined according to (Reitman and Frankel 1957), alkaline phosphatase (ALP) was estimated according to EL-Aaser and EL-Merzabani (1975). Level of urea and creatinine  assayed be method described with Wybenga et al. 1971; Henry 1974 respectively. Serum sodium (Na), chloride (Cl) and potassium (K) concentration was estimated with electrolyte analyzer model number PL1000 A. Calcium (Ca) and magnesium (Mg)  was estimated using a kit reagent test (Biodiagnostic, Giza, Egypt) Gindler and King 1972; Chauhan and Sarkar (1969)  respectively. The concentration of nitric oxide (NO) and total antioxidant capacity (TAC) in serum were assyed by Montgomery and Dymock 1961; Koracevic et al. 2001 respectively. l-malonaldehyde (L-MDA), reduced glutathione (GSH),  catalase (CAT)  and superoxide dismutase (SOD)  in skimmed milk were estimated according to Okhawa et al. (1979), Beutler et al. (1963), Aebi (1974)  and Nishikimi et al. (1972) respectively. Serum and whey milk of total protein and their electrophoretic pattern were determined according to Sonnenwirth et al. 1980 and Davis 1964, respectively and calculated based on SynGene S.No. 17292*14518 sme*mpcs.

Statistical Analysis:

The obtained data were statistically analyzed by One-Way ANOVA test. The results were given as mean ± standard error using SPSS 14 (2006). Results at P<0.05 was considered significant.

RESULTS

The cows of the mastitic group displayed rise body temperature, dullness, anorexia, congested mucus membranes, dropped milk production, the affected quarters of the udder were swelled, redness, hot, and firm in consistency. The supra mammary lymph nodes were enlarged. The milk secreted from the mastitic cattle appeared physical alteration likewise discoloration, alterations in consistency and flakes, beside there was an increase in pH of mastitic milk (average 7.5) in comparison to normal milk (average 6.7). Meanwhile, the control cows showed absence of systemic reaction and udder inflammatory signs with normal excreted milk.

Bacteriological examination of milk samples illustrated that, out of 20 tested samples, 10 isolates were identified as S. aureus, 6 isolate as E.coli and 4 isolates were identified as Klebsiella sp. The results of in-vitro antimicrobial susceptibility tests in table (4) revealed that, staphylococcus aureus showed the highest sensitivity to gentamycin and streptomycin followed by enrofloxacin and resistance to amoxycillin & clavulanic acid, cefotaxime and tetracycline and moderate resistance to florfenicol. Moreover, E.coli was more sensitive to gentamycin followed by streptomycin and enrofloxacin and resistant to amoxycillin & clavulanic and tetracycline followed by florfenicol and cefotaxime. Also, Klebsiella was sensitive to gentamycin, streptomycin and resistant to amoxycillin & clavulanic acid, tetracycline, cefotaxime, enrofloxacin and florfenicol.

Results concerning detection of antimicrobial resistance genes using Real time PCR assay showed that, the blaTEM gene was detected in all 5 selected isolates of S. aureu and 3 isolates of E. coli while it was detected in 2 out of 3 isolates of Klebsiella. The tetA gene was detected in 4 out of 5 isolates of S.aureus, all isolates of E.coli and Klebsiella. Moreover, floR gene was detected in 3 isolates of S.aureus, 2 isolates of E.coli and all isolates of Klebsiella (Fig.1-3).

The results of our study in Table (5) showed that mastitic group indicated a significant elevation in serum AST, ALT, ALP, urea, and creatinine when compared with normal healthy cows. All these parameters return to normal levels after treatment.

The results of our study in Table (6) showed that, the mastitic group indicated a significant elevation in serum Na, Mg and NO associated with a significant decline in serum Cl, Ca, K and TAC when compared with normal healthy cows. All these parameters return to normal levels after treatment.

pH and oxidative stress markers in milk illustrated in Table (7), there were a significant (P<0.05) increase pH and MDA, which associated with a significant (P<0.05) decrease in SOD, CAT and GSH in mastitic cows when compared with healthy cows, and all these parameters return to normal after treatment.

Serum biochemical analysis of serum T. protein and its main fractions showed in Table (8a), revealed a non-significant increase in t. protein, total alpha, total gamma associated with a significant increase in total beta and total globulin, meanwhile, there were a significant decrease in albumin and A:G ratio in mastitic group compared with normal control group, and all these biochemical parameters improved after treatment by the tested drugs.

The present results presented in Table (8b), revealed a non-significant increase in alpha 1, gamma 1 and gamma 2 associated with a significant increase in beta 1, meanwhile, there were a non-significant decrease in alpha 2 associated with a significant decrease in beta 2 in serum mastitic group compared with normal healthy cows. All these biochemical parameters improved after treatment by the tested drugs.

The present data which recorded in table (9) showed a notable increase in serum albumin, Immune-globulin and other proteins associated with non-significant increase in t. protein, meanwhile, there were significant decreases in α–lactoglobulin and ß- lactoglobulin in whey milk in mastitic group when compared with normal control groups, and all these parameters improved after treatments.

Table (4): Antibiotic sensitivity results of isolated bacteria

 

Antimicrobial agent

 

Code and potency

Staph. Aureus

No. 10

E coli

NO. 6

Klebsiella spp.

No. 4

Sens.

resist

Sens.

resist

Sens.

resist

Enrofloxacin

ENR10

7

3

4

2

-

4

Gentamycin

CN10

8

2

6

-

3

1

Streptomycin

S10

8

2

4

2

3

1

Amoxycillin+Clavulenic acid

AMC30

-

10

-

6

1

3

Florfenicol

FFC30

5

5

2

4

-

4

Cefotaxime

CTX30

3

7

2

4

-

4

Tetracycline

TE30

2

8

-

6

-

4

 

 

Fig. 1 Amplification Plot OF blaTEM gene.

 

Fig. 2 Amplification Plot of tetA gene.

 

Fig. 3 Amplification Plot of floR gene.

Table (5): liver and kidney function in serum cattle suffering from mastitis.

Groups

Parameters

Gp1:

normal control

Gp2: mastitis gp before treatment

Gp3: mastitis gp after treatment

AST (U/L)

43.5 ± 0.87b

52.5 ± 2.02a

44.5 ± 2.29b

ALT (U/L)

26.00 ± 0.29b

28.5 ± 0.29a

26.00 ± 0.58b

ALP (IU/L)

77.33 ±  1.76b

93.00 ± 1.73a

73.67 ± 2.03b

Urea (mg/dl)

29.57 ± 1.66b

52.00 ± 1.96a

32.13 ± 1.59b

Creatinine (mg/dl)

0.75 ± 0.03b

0.96 ± 0.07a

0.75 ± 0.02b

Results are represented as (Mean±SE); Mean value in the same raw with different letter is significantly different at (P < 0.05)

Table (6): Electrolytes, nitric oxide and total antioxidant capacity in serum cattle suffering from mastitis.

Groups

Parameters

Gp1:

normal control

Gp2: mastitis gp before treatment

Gp3: mastitis gp after treatment

Na (mEq/L)

140.00 ± 1.15b

154.00 ± 1.15a

144.00 ± 2.58b

Cl (mEq/L)

116.67 ± 2.91a

96.00 ± 4.04b

115.67 ± 1.86a

Ca (mg/dl)

10.00 ± 0.12a

8.73 ± 0.15b

9.70 ± 0.17a

Mg (mg/dl)

2.73 ± 0.03c

3.13 ± 0.03a

2.93 ± 0.03b

K (mEq/L)

5.50 ± 0.06a

4.40 ± 0.21c

4.93 ± 0.15b

NO (µmol/L)

13.57 ± 0.78b

59.61 ± 0.85a

10.86 ± 0.39c

TAC (Mm/l)

0.97 ± 0.01a

0.86 ± 0.01b

0.94 ± 0.005a

Results are represented as (Mean±SE); Mean value in the same raw with different letter is significantly different at (P < 0.05)

Table (7): PH and oxidative stress marker in milk in cattle suffering from mastitis.

Groups

Parameters

Gp1:

normal control

Gp2: mastitis gp before treatment

Gp3: mastitis gp after treatment

pH

6.67 ± 0.07b

7.50 ± 0.06a

   6.73 ± 0.09b

 

MDA (nmol/ml)

5.83 ± 0.05b

7.15 ± 0.35a

   6.20 ± 0.34ab

 

SOD (u/ml)

5.18 ±  0.55a

3.63 ± 0.15b

 5.38 ± 0.18a

 

CAT (u/ml)

2.53 ± 0.15a

2.00 ± 0.10b

 2.45 ± 0.05a

 

GSH (u/ml)

2.88 ± 0.17a

2.24 ± 0.11b

 3.09 ± 0.07a

 
               

Results are represented as (Mean±SE); Mean value in the same raw with different letter is significantly different at (P < 0.05)

 

Table (8a): Serum T. protein and its fractions (g/dl) in cattle suffering from mastitis.

Groups

parameters

Gp1:

normal control

Gp2: mastitis gp before treatment

Gp3: mastitis gp after treatment

T.protein

7.96 ± 0.09a

8.24 ± 0.11a

8.14 ± 0.23a

Albumin

2.49 ± 0.09a

2.10 ± 0.02b

2.39 ± 0.11ab

Total alpha

1.17 ± 0.05a

1.33 ± 0.05a

1.28 ± 0.14a

Total beta

1.27 ± 0.03b

1.43 ± 0.01a

1.33 ± 0.02b

Total gamma

3.03 ± 0.17a

3.38 ± 0.07a

3.14 ± 0.11a

Total globulin

5.47 ± 0.18b

6.14 ± 0.11a

5.76 ± 0.23ab

A:G ratio

0.46 ± 0.03a

0.34 ± 0.01b

0.42 ± 0.03ab

Results are represented as (Mean±SE); Mean value in the same raw with different letter is significantly different at (P < 0.05)

Table (8b): Serum protein sub-fraction (g/dl) in cattle suffering from mastitis.

Groups

parameters

Gp1:

normal control

Gp2: mastitis gp before treatment

Gp3: mastitis gp after treatment

Alpha 1

0.74 ±  0.03a

0.97 ±  0.01a

0.82 ±  0.13a

Alpha 2

0.43 ± 0.03a

0.36 ± 0.04a

0.46 ± 0.03a

Beta 1

0.89 ± 0.02b

1.13 ± 0.01a

0.91 ± 0.03b

Beta 2

0.38 ± 0.01a

0.30 ± 0.02b

0.42 ± 0.03a

Gamma 1

2.63 ± 0.18a

2.96 ± 0.07a

2.56 ± 0.11a

Gamma 2

0.39 ± 0.02a

0.43 ± 0.03a

0.59 ± 0.11a

Results are represented as (Mean±SE); Mean value in the same raw with different letter is significantly different at (P< 0.05)

Table (9): T. protein and its fractions (g/dl) in Whey milk.

Groups

parameters

Gp1:

normal control

Gp2: mastitis gp before treatment

Gp3: mastitis gp after treatment

T.protein

1.37 ± 0.05a

1.44 ± 0.04a

1.37 ± 0.01a

ß- lactoglobulin

0.52 ± 0.04a

0.37 ± 0.01b

0.44 ± 0.02ab

α - lactoglobulin

0.25 ±  0.01a

0.21 ±  0.005b

0.23 ±  0.01ab

Serum albumin

0.14 ± 0.01b

0.19 ± 0.01a

0.16 ± 0.01ab

Immune-globulin

0.36 ± 0.02b

0.50 ± 0.01a

0.40 ± 0.04b

Other proteins

0.08 ± 0.01c

0.16 ± 0.01a

0.12 ± 0.004b

Results are represented as (Mean±SE); Mean value in the same raw with different letter is significantly different at (P< 0.05)

 

DISCUSSION

Mastitis might be identified as inflammation of the parenchyma of the udder tissue despite the cause which causes economic losses in dairy industry (Radostits et al. 2006 and De Vliegher et al. 2012 ). When a pathogenic bacterium penetrates the mammary gland, it usually occurs because physical barriers as the teat canal are disrupted (Goldammer et al. 2004). Whenever the barrier is compromised, a rapid and influential defense response is needed to inhibit the prevalence of pathogenic organisms with additional harm to mammary gland tissue (Aitken et al. 2011). It cuased physical as well as chemical changes in the secreted milk, resulting in pathological alters in the mammary gland tissue (Babaei et al. 2007). In the present study,   mastitic group cattle appreared increased in body temperature, loss of appetite and dullness, additionally inflammatory udder signs involving pain reaction, hotness, redness, and swelling. Furthermore, the secreted milk displayed physical alterations such as discoloration, existence of flakes, consistency changs with sometimes contained purulent materials. Meanwhile, neither of these signs were noted in the  normal control cattle which showed normal excreted milk and absence of udder inflammatory signs. Such clinical findings were in agreement with Radostits et al. (2006) and Abdel-Hamied and Mahmoud (2020).

In the current study, we examined the existence of S. aureus,Klebsiella and E.coli related to cattle mastitis with general study of antibiotic resistance patterns in the isolates. S. aureus is one of the most usually recorded bacteria in cattle mastitis cases. it is the most usuall etiological pathogen of bovine mastitis possessive several virulent pathogens and multidrug resistant make the disease difficult to treat increasing global problem which has become a major concern for dairy industry worldwide. So detect the antimicrobial susceptibility profiles is needed not only for effective therapy but also for monitoring the diffusion of resistant strains in defined ecological niches (Coelho et al. 2009). The major frequency of S. aureus in current study may be because of absence of regular post milking teat dip, routine hand milking practice and lack of information about dry cattle therapy between the dairy owners. Spread of staphylococci from contagious to healthy udder quarters usually occurs among animals during the milking process via the milker’s hands (Constable et al. 2017; Sharma et al. 2007). The selected MDR Bacteria as S.aureus, Klebsiella and E.coli were applied for detection of resistant genes by PCR  to find out the mechanism of resistant. our results are indicated the resistant mechanism  of S.aureus, klebsialla sp and E.coli to tetracyclines may be due to the presence of Tet, resistance to floramphenicol due to the presence of flor and gene responsible for antibiotic resistance against β-lactam antibiotics due to presence of  bla TEM. blaTEM was the most usually detected gene in gram-negative and gram-positive bacteria isolated from cattle sampled. This confirms the apparent expression of resistance of isolates to beta-lactam antibiotics. An increasing amount of beta-lactam variants have been revealed that differs in amino acid sequences as well as their catalytic activity against β-lactam antibiotics (Bush and Jacoby 2010). The usage of tetracyclines as animal growth promoters is a greater contentious matter. The usage of tetracyclines in food production is numerous and contributes to the worldwide exposure of bacteria to tetracyclines. There is no suspicion that this practice results in the selection of resistant organisms and that in some cases these may be transmitted to humans. Moreover, since tet genes may be present in integrons. Eliminating the usage of tetracyclines and other antibiotics at subtherapeutic levels in animal feeds in other countries should also be a priority for feed producers and policy makers, in the hope that these alters will help to limited the incidence of resistant bacteria in the environment (Sousa et al. 2018). Additionally, there are reports on other phenicol resistance systems, like the inactivation via mutations of the target site,  phosphotransferases, efflux systems and permeability barriers (Schwarz et al. 2004), of the latter mechanism, floR and chloramphenicol resistance (cmlA) are the most usually known genes in gram-negative bacteria (Briggs and Fratamico 1999).

The present study displayed a significant elevated in ALP, ALT and AST activities in mastitic group. These results were in agreement with those recoded by (Saleem et al. 2021), Mastitis caused highly elevation in ALT, AST and ALP (Murphy 2005), and these increases may be because of hepatic tissues damage by bacterial toxins (Ismail and Hatem 1998).

Urea  and creatinine in current study showed a significant elevated in mastitic cows compared with control group. Our results were agreed with those stated by Mosallam et al. (2014), this increase may be due to decrease renal perfusion (reduced glomerular filtration) which can cause azotemia, in which the tubular flow rate is lower and urea reabsorption is greater, this alteration in kidney may be due to the toxins that produced from the pathogenic bacteria (Atroshi et al. 1996).

In current study, there were an increase in sodium levels in milk samples from mastitic animals, meanwhile other minerals involving potassium and calcium were decreased. Similar observation have previously been recorded for cattle (Rashed et al. 2002; Ahmad et al. 2007). The alter in milk pH in present study is thus linked with the elevated sodium levels in milk. Additionally, pH of mastitic milk was significantly higher due to the presence of clinical infections which can be used as a test for diagnosis of mastitis in animals which might be becouse of higher salts concentrations liberated due to increased permeability of cell membrane associated with inflammatory process and this might be responsible for elevate of pH in milk samples (Hussain et al. 2012). On the other hand, the result show significant decrease in Ca, K, and Cl these results were agreed with Hanan and Israa  (2019); Hussain et al. (2012), they suggested that the declined mineral level might be linked to the mineral losses from blood into the mastitic udder (El-Zubeir et al. 2005). Mastitis induces reduction in serum mineral due to anorexic condition and decreased intestinal absorption of mineral (Naresh et al. 2001). Anorexia in mastitic animals may be responsible for reduction in serum mineral (Abd Elazem et al. 2015).

Free radicals are produced naturally becouse of the intensive metabolism that exists in the cells of all living organism, mainly dairy cows. Oxidative stress commences when imbalance occurs in the homeostasis which caused via free radicals liberation which may ultimately lead to dairy cows being susceptible to mastitis. The discontinuity in the blood-milk barrier and the reduced secretory activity of the mammary gland's epithelial cells cause changes in the levels of most blood components during mastitis (Krishnappa et al. 2016). Greater liberation of free radicals with decreased TAC through clinical and subclinical mastitis in dairy cattle was mentioned (Atakisi et al. 2010), with resultant occurrence of oxidative stress (Lykkesfeldt and Svendsen 2007). Nitric oxide is one of the most critical reactive nitrogen radicals; which operate in different tissues like epithelial cells and macrophage of mammary gland, producing a notable amount of NO that mediates inflammation during mastitis (Bouchard et al. 1999). In this study, there was a highly increase in serum NO level in dairy cows with acute clinical mastitis in comparing to control group, similar to that observed by Atakisi et al. (2010). In livestock suffering mastitis, neutrophils produce large amount of NO and the myeloperoxidase enzyme, i.e. substances that together can cause nitrotyrosine formation, which has the ability to crumble proteins and have a destructive influnce on tissues (Jóźwik et al. 2012). Also, the elevated in  nitric oxide in present study might be due to the increased permeability of microcirculatory vessels and oxidative stress due to free radical injury (Qayyum et al. 2016 ).

The current study revealed a significant increase in skimmed milk L-MDA, meanwhile, a significant decreases in GSH levels in mastatic group comparing with normal control, illustrating the contribution of udder allied oxidative stress with potential oxidative damage, these results are in agreement with previous results recorded by Ranjan et al. (2005) and Kizil et al. (2007). L-Malondialdehyde the intermediate product of lipid peroxidation is being considered as a reliable index of oxidative stress (Esterbauer et al. 1991). The increase in L-MDA concentration may be becouse of extreme free radical liberation from neutrophils in the infected mammary gland which in turn lead to peroxidative injury to mammary cells (Boulanger et al. 2002), enhancing the incidence of oxidative stress in the udder tissue, which may caused increased permeability of microcirculatory arteries owing to free radical injury (Huma et al. 2020 and Carvalho-Sombra et al. 2021). Oxidative stress might be one of the primary reasons in drooping in quantity and quality of milk in dairy livestock (Kumar et al. 2022).

Antioxidants prevent oxidative deteriorate caused by free radicals through either directly scavenging them or via inhibiting enzymes oxidizing action (Jóźwik et al. 2012). It has been noticed that milk has antioxidant effects because of existence of enzymatic such as (SOD and CAT) and non-enzymatic (glutathione and protein) defence mechanism (Silanikove et al. 2014). Oxidative stress occurs because of elevated generation of ROS and increased lipid peroxidation products (MDA) concentration accompanied with reduced antioxidant protection defence mechanism, caused imbalance between ROS liberation and anti-oxidant defence system. Moreover, there is a failure of replacement and/or repair systems as well as increase levels of oxidative stress biomarkers responsible for mastatic disease (Kumar et al. 2022; Ali et al. 2022).

The our data  displayed that acute clinical mastitis is accompanied with a declined antioxidant defense. This might be observed through the notable increase concentrations of MDA along with the significant reduce in TAC, GSH, SOD and CAT activities. Such findings might indirectly indicate increased free radical action that reflect oxidative stress satate that occurs in such cases (Celi 2011).

Glutathione is a primary intracellular reducing factor for maintenance of thiol groups on intracellular proteins or for antioxidant molecules. GSH serves considerable functions involving detoxification of electrophiles and scavenging of free radicals, also it include in phase II conjugation and other reactions (Ribas et al. 2011). GSH concentration, in the current study,  was highly decrease in whey milk of mastitis cows when comparing with healthy cows suggestive of oxidative stress. Similarly, Jhambh et al. (2013) recorded that notable reduce in GSH level in mastitic cows becouse of conversion of reduced form to oxidized form (GSSH) via ROS overproduction from damage mammary gland.

Superoxide dismutase antioxidant enzyme is localized in cytoplasm and caused dismutation of superoxide to hydrogen peroxideswhich in turn is scavenged via CAT and glutathione peroxidases (GPx) (Kohen and Nyska 2002). CAT activity was highly reduced (P<0.05) in mastitic group. Similar observes were previously mentioned (Jhambh et al. 2013 and Sadat et al. 2023). Moreover, such decrease in CAT might be attributed to its increased consumption to counteract ROS generated from inflamed mammary glands, indicating an impairment in antioxidant defense of the body (Jhambh et al. 2013). Also, Sharma et al. (2010) recorded that CAT has exerted protective influences in cattle neutrophil induced model of mammary cellular injury in staph aureus infected mastitis. Lipid peroxidation is the indicator applied to determined cellular membrane injury caused via oxidative stress (Ranjan et al. 2005).

The biochemical investigation of serum samples in this study revealed, a significant decreased in serum albumin, Beta 2 and A:G ratio levels in the mastitic group. Similar observation were recorded by Ali et al. (2017a); Abdel-Hamied and Mahmoud (2020). This might be attributed to the decreased albumin concentrations caused through the immune response linked with udder infection (Singh, 2000). The hypoalbuminaemia  could be attributed to the stress condition that happens during mastitis which induce the protein catabolism. Albumin is a negative acute-phase systemic protein that migrates to inflamed tissues by increased vascular permeability and performs a diversity of physiological activities, involving antioxidant, and is regarded as an immune-inflammatory biomarker (Singh 2000). Because of vascular permeability is enhanced as a result of inflammation, this decline may be related to leakage of immunoglobulins, albumin and other serum proteins into milk (Krishnappa et al. 2016), or/and because of damage of hepatic tissues by bacterial toxins (Coles 1986).

Also, the present study revealed a significant increase in serum total globulin in mastitis group comparing with control one. Likewise, previous records reported high globulin concentrations in mastitic cattle (Ali, et al. 2017b and Singh et al. 2014). Elevated serum globulin concentrations might be linked to antibodies development in the form of gamma-globulin, which is responsible for neutralizing the invading microorganism’s influence (Chaplin, 2010).

Moreover, T. protein and its fractions in whey milk showed a significant increase in serum albumin, immune-globulin and other proteins, meanwhile, there were significant decreases in main whey protein (α–lactoglobulin and ß- lactoglobulin) in whey milk comparing with healthy cows. These observations are in agreement with the previous data recorded in milk from cows with clinical mastitis by Rashed et al. 2002; Le Maréchal et al. 2011). These findings may be attributed to both inflamatory injury of the mamary secretory tissues and devastation of blood-milk permeability barriers which limits in transfer of protein from interstitial fluid in to milk (Olumee-Shabon et al. 2013). Also, elevated total protein may be due to leakage of blood proteins such as immunoglobulins and serum albumin into milk as a response to immunological reactions during mastitis (Gráff and Miko 2015).

CONCLUSION

There was an unexpectedly high prevalence of resistance to different antimicrobials. The most surprising fact was the high incidence of high spread of resistant genes towards tetracyclines, Florphenicol and Beta lactam. The researchers hypothesized that factors other than antimicrobial medication, as feed, environment, farm type, and/or management practices, may play a role in the development and diffusion of AMR in E. coli, S. aureus and Klebsiella sp. Regular monitoring would enable timely identification of both emerging and current forms of resistance and AMR genes in bacteria originating from food-producing animals, involving those on dairy cow farms. Additionally, our results concluded that there are alterations in some constituent of serum and milk in normal and mastitic cattle. Moreover, oxidative stress play a serious role in mastitis, may be used as a potential biomarker for diagnosing and monitoring of mastitis.

References

Abd Elazem MA, and Seham YA. 2015. Adverse effects of Diclofenac Potassium and Dexamethason on some hematobiochemical and immunological parameters in Egyptian goat bucks. J Am Sci, 11(7): 92-99.
Abdel-Hamied E, Mahmoud MM. 2020. Antioxidants profile, oxidative stress status, leukogram and selected biochemical indicators in dairy cows affected with mastitis. J. Anim. Health Prod. 8(4): 183-188.
Abebe R,  Hatiya H, Abera M, Megersa B, Asmare K.  2016. “Bovine mastitis: prevalence, risk factors and isolation of Staphylococcus aureus in dairy herds at Hawassa milk shed, South Ethiopia,” BMC Veterinary Research, 12,270.
Aebi H (1974): Catalase in vitro assay methods. Methods Enzymol, 105: 121-126, 1984.
Ahmad TM, Bilal S, Uallah  ZU, Rahman NE, Muhammad G. 2007. Impact of mastitis severity on mineral contents of buffalo milk. Pak J Agri Sci, 44: 176-178.
Aitken SL, Corl CM, Sordillo LM. 2011. Immunopathology of mastitis: Insights into disease recognition and resolution. J. Mammary Gland. Biol. Neoplasia, 16, 291–304.
Ali A, Mir BA, Bhat RR, Baba OK, Hussain I, Rashid SM, Muzamil S, Ahmad SB, Mir MR. 2017a. Metabolic profiling of dairy cows affected with subclinical and clinical mastitis. J. Entomol. Zool. Stud., 5(6): 1026–1028.
Ali HR, Ali SF, Abd-Algawad RH, Sdeek FA, Arafa M, Kamel E, Shahein MA. 2022. Impact of udder infections on biochemical composition of milk in context of pesticides exposure, Veterinary World, 15(3): 797-808.
Ali T, Rahman SU, Zhang L, Shahid M, Han D,  Gao J, Zhang S, Ruegg PL, Saddique U, Han B. 2017b. Characteristics and genetic diversity of multi-drug resistant extended-spectrum beta-lactamase (ESBL)-producing Escherichia coli isolated from bovine mastitis. Oncotarget, 8, 90144–90163.
Amer S,  G´alvez F L,  Fukuda Y.  2018. “Prevalence and etiology of mastitis in dairy cattle in El Oro Province, Ecuador,” Journal of Veterinary Medical Science, 80 (6): 861–868.
 Andrei S, Matei S, Rugină D,  Bogdan L, ¸Stefănut C. 2016. Interrelationships between the content of oxidative markers, antioxidative status, and somatic cell count in cow’s milk. Czech J. Anim. Sci., 61(9): 407–413.
Atakisi E, Bozukluhan K, Atakisi O,  Gokce HI. 2010. Total oxidant and antioxidant capacities and nitric oxide levels in cattle with traumatic reticuloperitonitis. Veterinary Record, 167(23): 908-909.
Atakisi O, Oral H, Atakisi E, Merhan O, Pancarci SM, Ozcan A, Marasli S, Polat B, Colak A, Kaya S. 2010. Subclinical mastitis causes alterations in nitric oxide, total oxidant and antioxidant capacity in cow milk. Res. Vet. Sci., 89: 10–13.
Atroshi F, Parantainen J, Sankari S, Järvinen M, Lindberg LA, Salonimei H. 1996. Changes in inflammation-related blood constituents of mastitic cows. Veterinary Research,  27 (2) :125-132.
Babaei H, Mansouri-Najand L, Molaei MM, Kheradmand A, Sharifan M. 2007. Assessment of lactate dehydrogenase, alkaline phosphatase and aspartate aminotransferase activities in cow’s milk as an indicator of subclinical mastitis. Vet. Res. Commun., 31: 419–425.
Bag MAS, Khan MSR, Sami MDH, Begum F, Islam MS, Rahman MM, Rahman MT,  Hassan J. 2021. Virulence determinants and antimicrobial resistance of E. coli isolated from bovine clinical mastitis in some selected dairy farms of Bangladesh. Saudi Journal of Biological Sciences, 28(11), 6317–6323.
Batavani RA, Asri S, Naebzadeh H. 2007. The effect of subclinical mastitis on milk composition in dairy cows. Iran J Vet Res, 8: 205- 211.
Beutler E, Duron O, Kelly MB. (1963): Improved method for the determination of blood glutathione. J Lab Clin Med, 61: 882-888.
Beyene T, Hayishe H, Gizaw F.  2017. “Prevalence and antimicrobial resistance profile of Staphylococcus in dairy farms, abattoir, and humans in Addis Ababa, Ethiopia,” BMC Research Notes, 10(1): 1–9.
Bi Y, Wang YJ, Qin Y, Vallverd´u RG, Garc´ıa JM. 2016. “Prevalence of bovine mastitis pathogens in bulk tank milk in China,” PLoS One, vol.11, Article ID e0155621,5;1–13.
Bouchard L, Blais S, Desrosiers C, Zhao X, Lacasse P. 1999. Nitric oxide production during endotoxin-induced mastitis in the cow. Journal of Dairy Science, 82(12): 2574-2581.
Boulanger V, Zhao X, Lacasse P. 2002. Protective effect of melatonin and catalase in bovine neutrophil-induced model of mammary cell damage. Journal of Dairy Science. 85:562-569.
Briggs CE, Fratamico PM. 1999. Molecular characterization of an antibiotic resistance gene cluster of Salmonella typhimurium DT104. Antimicrob. Agents Chemother. 43, 846–849.
Bush K, Jacoby GA. 2010. MINIREVIEW Updated Functional Classification of -Lactamases, 54; 969–976 (3).
Campos FC, Castilho IG, Rossi BF, Bonsaglia ´ECR, Dantas ST, Dias RC, Fernandes B, Júnior A, Hernandes RT, Camargo CH, Ribeiro MG, Pantoja JCF, Langoni H, Rall VLM. 2022. Genetic and antimicrobial resistance profiles of mammary pathogenic E. coli (MPEC) isolates from bovine clinical mastitis. Pathogens (Basel, Switzerland), 11(12). 10.3390/pathogens11121435.
Carvalho-Sombra TCF, Fernandes DD, Bezerra BMO, Nunes-Pinheiro DCS. 2021. Systemic inflammatory biomarkers and somatic cell count in dairy cows with subclinical mastitis. Vet.Anim. Sci. 8;11:100165.
Celi P. 2011. Biomarkers of oxidative stress in ruminant medicine. Immunopharmacol. Immunotoxicol., 33: 233–240.
Chaplin DD. 2010. Overview of the immune response. J. Allergy Clin. Immunol., 125, S3–S23.
Chauhan UP, Sarkar BC. 1969. Use of calmagite for the determination of traces of magnesium in biological materials. Anal. Biochem. 32, 70–80.
Cheng J, Zhou M, Nobrega DB, Barkema HW, Xu S, Li M, Kastelic JP, Shi Y, Han B, Gao J. 2021. Genetic diversity and molecular epidemiology of outbreaks of Klebsiella pneumoniae mastitis on two large Chinese dairy farms. Journal of Dairy Science, 104(1);762–775. 10.3168/jds.2020-19325.
CLSI. 2014. Evaluation of precision of quantitative measurement procedure; approved guideline, 3rd ed. CLSI document EP05-A3. Wayne, PA: Clinical and Laboratory Standards Institute.
Coelho SMO, Reinoso E, Pereira IA, Soares LC, Demo M, Bogni C, Souza M. 2009. Virulence factors and antimicrobial resistance of Staphylococcus aureus isolated from bovine mastitis in Rio de Janeiro.Pesquisa Veterinaria Brasileira, 29, 369–374.
Colakoglu HE, Kuplulu O, Vural MR, Kuplulu S, Yazlik B, Polat MO, IM, Oz B, Kaya U, Bayramoglu R. 2017. Evaluation of the relationship between milk glutathione peroxidase activity, milk composition and various parameters of subclinical mastitis under seasonal variations. Vet. arhiv 87, 557-570.
Coles EH. 1986. Veterinary Clinical Pathology.(4th Edn.).W.B.Saunders Company, London, U.K:
Colom K, PèrezJ, Alonso R, Fernández-Aranguiz A, Lariňo E, Cisterna R. 2003. Simple and reliable multiplex PCR assay for detection of blaTEM,blaSHV and blaOXA-1 genes in Enterobacteriaceae. FEMS Microbiology Letters 223,  147.
Constable PD, Hinchcliff KW, Done SH, Grunberg W. 2017. Veterinary Medicine: a textbook of the diseases of cattle, horses, sheep, pigs and goats.; 11th Edition, Elsevier
Davis B((1964): Disk electrophoresis. II Method and application to human serum protein. Ann N Y Acad Sci, 121(2): 404-427.
De Vliegher S, Fox LK, Piepers S, McDougall S, Barkema HW. 2012. Invited review: Mastitis in dairy heifers: Nature of the disease, potential impact, prevention, and control. J. Dairy Sci, 95, 1025–1040.
Dittrich I, Gertz M,  Krieter J. 2019. Alterations in sick dairy cows’ daily behavioural patterns. Heliyon 5:e02902. doi: 10.1016/j.heliyon.2019.e02902.
EL-Aaser AA, EL-Merzabani MM. 1975. Simultaneous determination of 5'-nucleotidase and alkaline activities in serum. Z. Klin. Chem. Klin.Biochem., 13:453- 460.
El-Zubeir IEM, Elowni OAO, Mohamed GE. 2005. Effect of mastitis on macro-minerals of bovine milk and blood serum in Sudan. J. South Afr. Vet. Assoc., 76: 22–25.
Esterbauer H, Schaur RJ, Zollner H. 1991. Chemistry and biochemistry of 4-hydroxynonenal, malonaldehyde and related aldehydes. Free Radical Biology and Medicine.; 11:81-128.
FAO Food and Agriculture Organization, 2014. “Impact of mastitis in small scale dairy production systems,” Animal Production and Health Working Paper, No. 13, Rome, Italy.
Fu S, Wen C, Wang Z, Qiu Y, Zhang Y, Zuo J, Xu Y, Han X, Luo Z, Chen W, Miao J. 2022. Molecular epidemiology and antimicrobial resistance of outbreaks of Klebsiella pneumoniae clinical mastitis in Chinese dairy farms. MicrobiologySpectrum,, 10(6), Article e0299722. Article 10.1128/spectrum.02997-22.
Gao J, Barkema HW, Zhang L, Liu G, Deng Z, Cai L. 2017. Incidence of clinical mastitis and distribution of pathogens on large Chinese dairy farms. J Dairy Sci. 100:4797–4806. doi: 10.3168/jds.2016-12334
Gindler M King JD. 1972. Rapid colorimetric determination of calcium in biologic fluids with methylthymol blueAm. J. Clin. Path. 58(4), 376-382.
Goldammer T, Zerbe H, Molenaar A, Schuberth HJ, Brunner RM, Kata SR, Seyfert HM. 2004. Mastitis increases mammary mRNA abundance of beta-defensin 5, toll-like-receptor 2 (TLR2), and TLR4 but not TLR9 in cattle. Clin. Diag. La. Immunol., 11, 174–185.
Gráff M, Miko E. 2015. Analysis of mastitis in Holstein-Fresian cows and economic effects of masti­tis. Lucrari Stiintifice Seria I, Manage. Agricol., 17(1): 294-297.
HananYJ, Israa A. 2019. Efficacy of reliable milk and blood biomarkers for diagnosing clinical and subclinical bovine mastitis. Adv. Anim. Vet. Sci. 7(10): 898-903.
Henry RJ. 1974. "Clinical chemistry, principles and techniques." 2nd Ed., Harport and Rowhogerstown, M.D. 862.
Huma IZ, Sharma N, Kour S, Tandon S, Guttula KP, Kour S, Singh AK, Singh R, Gupta KM. 2020. Putative biomarkers for early detection of mastitis in cattle. Anim. Prod. Sci. 60(14): 1721-1736.
Hussain R, Javed MT, Khan A. 2012. Changes in some biochemical parameters and somatic cell counts in the milk of buffalo and cattle suffering from mastitis. Pak Vet J, 32(3): 418-421.
Ismail TM, Hatem ME. 1998 Prevalence of sub clinical mastitis in a dairy cottle herd in the eastern region of Saudi Arabia. Proc. 8th Sci. Cong., Fac. Vet. Med., Assiut Univ., Egypt.          
Jamali H, Barkema HW, Jacques M. 2018. “Invited review: incidence, risk factors, and effects of clinical mastitis recurrence in dairy cows,” Journal of Dairy Science, 101(6): 4729–4746.
Jhambh R, Dimri U, Gupta VK, Rathore R. 2013. Blood antioxidant profile and lipid peroxides in dairy cows with clinical mastitis. Vet. World, 6: 271–273.
Jóźwik A, Krzyżewski J, Strzałkowska N, Poławska E, Bagnicka E. 2012. Relations between the oxidative status, mastitis, milk quality and disorders of reproductive functions in dairy cows - a review. Animal Science Papers and Reports 30(4): 297-307.
Kizil O, Akar Y, Saat N, Kizil M, Yuksel M. 2007. The plasma lipid peroxidation intensity (MDA) and chain-breaking antioxidant concentrations in the cows with clinic or subclinic mastitis. Revue Med. Vet. 158:529-533.
Kohen R, Nyska A. 2002. Oxidation of biological systems: oxidative stress phenomena, antioxidants, redox reactions, and methods for their quantification. Toxicologic Pathology. 30:620-650.
Koracevic D, Koracevic G, Djordjevic V, Andrejevic S, Cosic V. 2001. Method for the measurement of antioxidant activity in human fluids. J of Clin Pathol, 54(5):356-361. DOI: 10.1136/jcp.54.5.356.
Krishnappa S, Satyanarayana ML, Narayanaswamy HD, Rao S, Yathiraj S, Isloor S, Mukartal SY, Gupta S, Singh SV, Elattuvalappil AM. 2016. Haemato-biochemical profile and milk leukocyte count in subclinical and clinical mastitis affected buffaloes. Adv. Anim. Vet. Sci., 4: 642–647.
Kumar S, Mikolajcik EM. 1972. Electrophoretic, immunoelectrophoretic and ultracentrifugal characterization of protein in whey fractions. J. Dairy Sci.,9: 1237-1242.
Kumar S, Varma R, Mandil R, Verma H, Anand S. 2022. Alteration in oxidative-stress biomarkers in bovine sub-clinical mastitis. The Pharma Innovation Journal. 11(12S): 95-99.
Lamari I, Mimoune N,  Khelef D. 2021. Effect of feed additive supplementation on bovine subclinical mastitis. Veterinarskastanica,52(4); 445- 460.
Le Maréchal C, Thiéry R, Vautor E, Le Loir Y. 2011. Mastitis impact on technological properties of milk and quality of milk products—A review. Dairy Sci. Technol, 91, 247–282.
Lykkesfeldt J, Svendsen O. 2007. Oxidants and antioxidants in disease: oxidative stress in farm animals. Vet. J., 173: 502–511.
Maity, S., and Ambatipudi, K. (2021). Mammary microbial dysbiosis leads to the zoonosis of bovine mastitis: a One-Health perspective. FEMS Microbiol. Ecol. 97(1):fiaa241.
Medrano-Galarza C, Gibbons J, Wagner S, de Passillé,AM,  Rushen J. 2012. Behavioral changes in dairy cows with mastitis. J. Dairy Sci. 95, 6994–7002. doi: 10.3168/jds.2011-5247.
Montgomery HAC, Dymock JF. 1961. The determination of nitrite in water. Analyst, 86: 414-416.
Mosallam TE, Hanaa A, Allam Safaa YS, Ahmed AR. 2014. Clinical and Bacteriological and Biochemical Studies on Mastitis in dairy cattle. Zag. Vet. J. 42(3):124-132.
Motaung TE, Petrovski KR,  Petzer IM, Ekisoe O, Tsilo TJ. 2017. “Importance of bovine mastitis in Africa,” Animal Health Research Reviews, 18 (1): 58–69.
Murphy S. 2005. Raw milk bacteria tests: Standard plate count and coliform count. Proc. National Mastitis Council Regional Meeting, Syracuse, Ny. 36-46.
Naresh R, Dwivedi S, Dey S, Swarup D. 2001. Zinc, copper and cobalt concentration in blood during mastitis in dairy cows. Asian Aust J Anim Sci, 14(4)564-566.
National Mastitis Council (NMC). 1999. Laboratory handbook on bovine mastitis. Madson: 145-147.
Ndahetuye JB, Persson Y, Nyman AK, Tukei M, Ongol MP,  Båge R. 2019. Aetiology and prevalence of subclinical mastitis in dairy herds in peri-urban areas of Kigali in Rwanda. Tropical Animal Health and Production, 51(7), 2037–2044.
Ng LK, Martin I, Alfa M, Mulvey M. 2001. Multiplex PCR for the detection of tetracycline resistant genes. Molecular and cellular probes15(4), 209-215.‏
Nishikimi M, Roa NA, Yogi K (1972): Occurrence of superoxide anion in the reaction of reduced phenazine methosulfate and molecular oxygen. Bioch and Biophy Res Commun, 46: 849-854.
Okhawa H, Ohishi N, Yagi K (1979): Assay for lipid peroxides in animal tissues by thiobarbituric acid reaction. Anal Biochem, 95(2):351-358.
Oliver SP, Murinda  SE, Jayarao BM. 2011. “Impact of antibiotic use in adult dairy cows on antimicrobial resistance of veterinary and human pathogens: a comprehensive review,” Foodborne Pathogens and Disease, 8(3): 337–355.
Olumee-Shabon Z, Swain T, Smith EA, Tall E, Boehmer JL. 2013. Proteomic analysis of di_erentially expressed proteins in caprine milk during experimentally induced endotoxin mastitis. J. Dairy Sci., 96, 2903–2912.
Qayyum A, Khan JA, Hussain R, Avais M, Ahmad N, Khan MS. 2016. Investigation of milk and blood serum biochemical profile as an indicator of sub-clinical mastitis in Cholistani cattle. Pak Vet J, 36(3): 275-279.
Radostits OM, Gay CC, Hinchcliff KW, Constable PD. 2006. Veterinary Medicine E-Book: A textbook of the diseases of cattle, horses, sheep, pigs and goats. Elsevier Health Sciences.
Radostits OM, Mayhew IG, Houston DM. 2000. Veterinary clinical examination and diagnosis. WB Saunders.
Rainard P, Foucras G, Fitzgerald JR, Watts JL, Koop G,  Middleton JR. 2018. Knowledge gaps and research priorities in Staphylococcus aureus mastitis control. Transboundary and Emerginf Diseases, 65, 149–165.
Ranjan R, Swarup D, Naresh R, Patra RC. 2005. Enhanced erythrocytic lipid peroxides and reduced plasma ascorbic acid and alteration in blood trace elements level in dairy cows with mastitis. Veterinary Research. Comun., 29:27-34.
Rashed MA, Mogda K, Mansour M, Korietum Kh. 2002. Biochemical changes in blood and milk of mastitic cows. Egypt. J. Comp. & Clinic. Path. 15 (1):74—83.
Reitman S, Frankel S. 1957. "Acolorimetric determination of serum glutamic oxaloacetic acid and glutamic pyruvic transaminase." Am. J. Clin. Path., 28: 56- 58.
Ribas V, Ruiz CG, Checa JCF. 2011. Glutathione and mitochondria. Front.Pharmacol.00151; c2014.
Sadat A, Farag AMM Elhanafi D AwadA, Elmahallawy EK, Alsowayeh N, El-khadragy MF, Elshopakey GE. 2023. Immunological and Oxidative Biomarkers in Bovine Serum from Healthy, Clinical, and Sub-Clinical Mastitis Caused by Escherichia coli and Staphylococcus aureus Infection. Animals, 13, 892. doi.org/10.3390/ani13050892.
Saleem H, Razooqi M, Gharban HA. 2021. Cumulative Effect of Subclinical Mastitis on Immunological and Biochemical Parameters in Cow Milk. Archives of Razi Institute, 76 (6): 1629-1638.
Schwarz S, Kehrenberg C, Doublet B,  Cloeckaert A. 2004. Molecular basis of bacterial resistance to chloramphenicol and florfenicol. FEMS Microbiol. Rev. 28, 519–542.
Sharma C,  Rokana N, Chandra  M. 2018. “Antimicrobial resistance: its surveillance, impact, and alternative management strategies in dairy animals” Frontiers in Veterinary Science,4:1–27.
Sharma N, Maiti SK, Sharma KK. 2007. Prevalence, etiology and antibiogram of microorganisms associated with Sub-clinical mastitis in buffaloes in Durg, Chhattisgarh State (India). Int J Dairy Sci.; 2(2):145-151.
Sharma N, Mukherjee R, Ingale SL, Jadhav RK. 2010. Therapeutic and anti-oxidant activity of vitamin E and selenium in bovine Staphylococcal mastitis. Indian Journal of Veterinary Research. 19(1):25-31.
Silanikove N, Merin U, Leitner G. 2014. Nitrite and catalase levels rule oxidative stability and safety properties of milk: a review. RSC Advances.;4:26476-26486.
Singh K, Chandra M, Kaur G, Narang D, Gupta DK. 2018. Prevalence and antibiotic resistance pattern among the mastitis causing microorganisms. Open J. Vet. Med. 8, 54–64.
Singh R, Bhardwaj RK, Azad MS, Beigh SA. 2014. Effect of mastitis on haemato-biochemical and plasma mineral profile in crossbred cattle. Indian J. Anim. Res., 48, 63–66.
Singh SV. 2000. Udder health profiles with special reference to acute phase proteins and supplementation therapy. MV Sc thesis submitted to the GB Pant University of Agriculture and Technology, Pantnagar, India.
Sonnenwirth, A.C., Gradwohl, R.B.H., Jaret, L., 1980. Gradwohl′s Clinical Laboratory Methods and Diagnosis. 8th ed., 258-259, St. Louis, Toronto, London; the C.V. Mosby Co.
Sousa JCG, Ribeiro AR, Barbosa MO, Pereira MFR, Silva AMT. 2018. A review on environmental monitoring of water organic pollutants identified by EU guidelines. Journal of Hazardous Materials, 344, 146–162.
Wang JY, Tang P, Cui EH, Wang LQ, Liu WH, Ren JJ, Wu N, Qiu YH. 2013. Characterization of antimicrobial resistance and related resistance genes in Escherichia coli strains isolated from chickens in China during 2007-2012. Afr J Microbiol Res 7, 5238–5247.
Wybenga DR, Digigorgio J, Piliggi VJ. 1971. "Automated method for urea measurement in serum." Clin. Chem., 97: 891- 895.
Zajac P, Tomaska M, Murarova A, Capla J, Curlej J. 2012. Quality and safety of raw cow’s milk in Slovakia in 2011. Potravinárstvo 6, 64–73.

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