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Seroprevalence of Contagious Ecthyma and Its Associated Risk Factors in Sheep and Goats of Punjab, Pakistan

PJZ_55_5_2187-2197

Seroprevalence of Contagious Ecthyma and Its Associated Risk Factors in Sheep and Goats of Punjab, Pakistan

Irtaza Hussain1, Muti ur Rehman Khan1*, Asim Aslam1, Masood Rabbani2 and Ahsan Anjum1

1Department of Pathology, Faculty of Veterinary Sciences, University of Veterinary and Animal Sciences, Lahore, Pakistan, 54000, Pakistan

2Institute of Microbiology, Faculty of Veterinary Sciences, University of Veterinary and Animal Sciences, Lahore, Pakistan, 54000, Pakistan

ABSTRACT

The objective of the current study was to determine the prevalence of contagious ecthyma along with the association of various risk factors in goats and sheep through qualitative enzyme linked immunosorbent assay (ELISA). This technique is sensitive and cost-effective for detecting disease in large no of animals. For this purpose, serum samples from 350 goats and 91 sheep were collected on the 20th day post-infection for detection of antibodies, and essential information related to potential risk factors was collected through a questionnaire from fourteen districts of Punjab, Pakistan. Serologically positive samples were processed through PCR for confirmation using scab samples by identifying the GIF/IL-2 gene. This study found an overall 13.2% seroprevalence of contagious ecthyma infection, indicating a higher percentage in goats (14.6%) than in sheep (7.7%). In goats, the significant association (P<0.0001) of contagious ecthyma infection with seroprevalence was found in 4 districts; however, contagious ecthyma antibodies titers were found positive in sheep of Muzaffargarh only. The risk factors such as young age, female gender, grazing without stall feeding, presence of lesions on the lips, and injuries on the skin caused by prickly trees and cotton stubbles were found significantly (p<0.05) associated factors in goats; and age and injuries on the skin were important associated risk factors in sheep. The maximum occurrence of contagious ecthyma infection was found from September to December in both goats and sheep; having a significant association in goats (χ2=39.2) (P<0.0001). Likewise, the purchase of new animals and mixing up with the existing animals without quarantine measures cause contagious ecthyma to prevail in the vicinity. Moreover, contagious ecthyma antibodies were detected by ELISA kits up to 50th day post-infection in the current study. This is the first study that reported the seroprevalence of contagious ecthyma in Punjab, Pakistan. Comprehension of risk variables will not only be helpful to develop awareness amongst farmers but will also provide guidelines to government officials about the prevention and control of the disease.


Article Information

Received 31 March 2022

Revised 20 April 2022

Accepted 18 May 2022

Available online 01 August 2022

(early access)

Published 31 July 2023

Authors’ Contribution

IH, MRK, AA and MR conceived and designed the study. IH and AA executed the experiments. IH, MRK and AA prepared the manuscript. MRK, AA and MR reviewed the manuscript. MRK evaluated and supervised the study. All authors have read and approved the manuscript.

Key words

Contagious ecthyma, Goats, Sheep, ELISA, PCR, Risk factors, Punjab, Pakistan

DOI: https://dx.doi.org/10.17582/journal.pjz/20220331030325

* Corresponding author: drniazi@uvas.edu.pk

0030-9923/2023/0005-2187 $ 9.00/0

Copyright 2023 by the authors. Licensee Zoological Society of Pakistan.

This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (https://creativecommons.org/licenses/by/4.0/).



INTRODUCTION

Most of the world’s population relies on agriculture and livestock to make a living (Riaz et al., 2021). In the tropical and subtropical areas, goats are becoming more attractive as a livestock species due to their low food costs and ease of rising with minimal maintenance needs (Ashraf et al., 2021). These animals also make up a large part of Pakistan’s livestock population and play a pivotal role in the provisions of hides, meat, and thus income for farmers in the rural areas of the country. Pakistan intends to boost livestock exports internationally (Rehman et al., 2020). However, various infectious and non-infectious diseases pose a constant threat to the production of these animals and thereby economic losses. Contagious ecthyma, commonly identified as contagious pustular dermatitis or orf, is among one of these diseases.

Its causative agent, parapoxvirus belongs to the sub-family Chordopoxvirinae of the Poxviridae, is a persistent issue among goats and sheep in Punjab, Pakistan. The viral genome has a linear double-stranded DNA genome. It is a particular skin disease of a wide range of ruminants including sheep and goats and is endemic worldwide (Karki et al., 2019; Zhang et al., 2015).

Animals that have been exposed to the ORF virus earlier might carry the virus in their hide or dried scabs and shed it into the environment. In the environment, the ORF virus has a higher survival, especially in tropical climates (Thurman and Fitch, 2015). Direct contact with infected animal and/or contaminated fomites containing the ORF virus causes transmission. The virus usually enters the skin through cuts or abrasions and establishes infection. From skin reddening (erythema) to macule, papule, vesicle, pustule, scab, and scar, the skin lesions develop and progress in a variety of stages (Fleming et al., 2015; Kinley et al., 2013). Although this disease is more common amongst young animals, few adult animals may also be distressed. Dehydration and malnutrition are the leading causes of death in young animals, owing to pain caused by oral cavity lesions that prohibit them from suckling their dam. Similarly, proliferative lesions, especially on the lips, badly affect the feed intake of adult animals.

Contagious ecthyma can be diagnosed in various ways like the detection of scabby lesions around the oral cavity, limbs, or teats, or through histopathology of epidermal lesions (Kumar et al., 2015; Sadiq et al., 2017). The culture of the virus on cell lines (Amann et al., 2013; Chan et al., 2007; Li et al., 2012) is also good but it is considered as strenuous and much time-consuming procedure (Li et al., 2012). Molecular tests for specific ORFV strains are also successfully used for its diagnosis but these tests are not effective for screening at the herd level (Chan et al., 2009). Contrarily, the qualitative enzyme linked immunosorbent assay (ELISA) approach is sensitive and affordable for detecting ORF viruses in a large population of animals in the field (Bala et al., 2019). The presence of antibodies (IgG) in a sero-converted animal indicates the existence of sustained infection of contagious ecthyma, which helps in distinguishing freshly infected animals from long-term contagious ecthyma infection (Bala et al., 2018). Therefore, ELISA was preferred for screening of ORFV in this study.

Normally, this disease cures on its own. Nevertheless, its economic burden is enormous in terms of mortality and wasting in severe cases due to secondary bacterial or fungal infections or delayed treatment (Bala et al., 2019). Moreover, its morbidity can also be as high as 100% (Kumar et al., 2015; Ramesh et al., 2008). In Pakistan, owing to the lack of any study on this disease, nothing can be said for sure about its exact economic repercussions. However, the disease has a high economic cost as indicated by an estimate showing a national expense of approximately ten million pounds on ORFV in the British sheep sector (Onyango et al., 2014). Because of the aforementioned context, this study was planned to estimate the rate of current ORF virus infection in goats and sheep based on detecting IgG antibodies in fourteen districts of Punjab, Pakistan. The study also attempted to estimate the association of potential risk factors with the occurrence of ORFV infection in goats and sheep. Seropositive samples were then submitted for molecular validation through PCR assay.

MATERIALS and METHODS

Ethical statement

All experimental procedures were carried out in accordance with guidelines approved by the University of Veterinary and Animal Sciences (UVAS), Lahore, Pakistan’s ethical review committee (Permit No. DR/452 dated 06/10/2020).

Study area and sample size

The study area comprised of 14 districts of Punjab having over 220,000 sheep and goats. Punjab is located at 31.1704° N, 72.7097° E.

There had been no previous reports on the prevalence of contagious ecthyma in Pakistan, consequently, the sample size was determined for a disease with a 50% predicted prevalence at a 95% confidence range and a 5% desirable absolute precision (Hussain et al., 2021). According to elaboration, the sample size was calculated via sample size calculator available at (https://www.surveysystem.com/sscalc.htm), expecting the population of goats and sheep over 220,000 yielding a total sample size of 383.

Goats and sheep that appeared to have recovered from contagious ecthyma, as well as animals with nodular to diffuse proliferative skin lesions around the lips, muzzle, teats, and nostrils, were considered for serum sample collection. We studied n=350 goats and n=91 sheep. The study was carried out for a year from July 2020 to July 2021.

Sample collection and processing for ELISA

Blood samples (3 ml) were taken aseptically from the jugular vein using sterile syringes and transferred to anticoagulant-free test tubes for serum separation (Rafique et al., 2021). Blood samples were collected at day 20 and day 50. After collection of the whole blood, allowed the blood to clot by leaving it undisturbed at room temperature for 10-20 min. The clot was removed by centrifuging at 2,000-3,000 rpm for 20 min. The serum was subsequently transferred to a fresh 1.5 ml micro-centrifuge tube and stored at -20°C until the indirect Sandwich-ELISA test was performed. The samples were again centrifuged, if any precipitations appeared during storage (Bala et al., 2018).

The serum samples were tested qualitatively for anti-contagious ecthyma IgG in animals presenting clinical indications and seemingly healthy animals in the herd using the enzyme-linked immunosorbent assay (ELISA) technique. The contagious ecthyma IgG was carried out according to the manufacturer’s instructions, using goat and sheep micro-ELISA strip plates (Catalogue Number: SL0049Gt, SL00097Sp; SunLong Biotech Co., LTD). In the microplate, micropores were labeled according to sample IDs; whereas, left two wells were designated as negative controls, two wells adjacent to negative controls as positive controls, and one empty well as a blank control. In the negative and positive control wells, 50 µl of respective controls were added. 40 µl sample dilution buffer and 10 µl sample were introduced to the sample wells. Without touching the well wall, samples were loaded onto the bottom. The samples were thoroughly mixed with gentle shaking before being sealed with the closure plate’s membrane and incubated at 37°C for 30 min. After incubation, the closure plate membrane was gently removed, and the reaction was rinsed 5 times with a wash solution at 30 second intervals. Except for the blank control well, each well received 50 µl of HRP-conjugate reagent after 5 washing cycles. The incubation and cleaning procedures were repeated once more. After that, 50 µl of each chromogen solution A and chromogen solution B were added to each well, stirred gently in a dark environment, and incubated at 37°C for another 15 min. By injecting 50 µl of stop solution into each well, the reaction was brought to a halt. In the well, there was a change in colour from blue to yellow.

A microtiter plate reader was used to read the absorbance Optical Density (O.D.) at 450 nm within 15 min of adding the stop solution (PR4100 Microplate Reader; Bio-Rad Laboratories). The test kit’s effectiveness was confirmed because the overall positive control result was larger than 1.00. The cut-off value was calculated using the following formula. Cut-off (CO) value = mean of two negative controls + 0.15 (Bala et al., 2018).

Study of risk factors

The well-structured questionnaire was distributed to farmers and personnel working in the field to study the prevalence of contagious ecthyma regarding the presence of IgG antibodies. The potential risk factors studied in goats and sheep included area (different districts), species, age, gender, breed, presence or absence of gross lesions, presence of orf lesions on different body parts, feeding, injuries on skin, faring system, purchase of new animals.

Molecular confirmation by PCR

The dermal tissue samples were collected from sheep and goats with possible diagnostic lesions on the oral commissure, muzzle, lips, and nose. Samples were taken from animals having nodular and widespread proliferative cutaneous lesions. Skin tissue samples exhibiting nodular lesions were gathered in a sterile polystyrene vial having antibiotics (penicillin 1,000 IU/mL, streptomycin 1,000 g/mL, kanamycin 500 g/mL) and antifungal (amphotericin B 25 mg/mL) reagents. The obtained samples were kept at -20°C until they were analyzed in the laboratory. The GeneJET Genomic DNA Purification Kit was used to extract genomic DNA (Thermo Fisher Scientific, Catalog Number: K0722). ORFV’s GIF/IL-2 gene was amplified using forward (5’-GCTCTAGGAAAGATGGCGTG-3’) and reverse (5’-GTACTCCTGGCTGAAGAGCG-3’) primers previously described (Kumar et al., 2015).

The PCR procerdure was carried out with a total volume of 40 µL reaction mixture, that included 20 µL master mix (PrimeSTAR Max DNA polymerase, Catalog Number: R045A), 2 µL of DNA template, 2 µL each forward and reverse primers and 14 µL PCR grade water. The PCR reaction setting were adjusted as initial denaturation (95°C, 5 min), afterwards 35 cycles of denaturation (94°C, 30 sec), annealing (58°C, 30 sec), and extension (72°C, 45 sec), subsequently a final extension (72°C, 7 min). Amplicons were seen on 1.5 percent agarose gel, stained with GelRed™ Nucleic Acid Gel Stain during gel electrophoresis (110V, 230mA, 30 min) and being recorded in a gel documentation system (Bio-Rad Laboratories, United States).

Statistical analysis

The Pearson Chi-square (χ2) test was applied to evaluate the association between potential risk factors. The odds ratio was calculated using Fisher’s exact test to evaluate the probability of risk factors within the research region. The level of significance was recognized at a 95 percent confidence interval in each procedure. For statistical analysis, SPSS version 22 was employed.

RESULTS

Overall sero-prevalence of contagious ecthyma

The sero-prevalence of contagious ecthyma was studied in a total of 441 sheep and goats samples from 14 different districts of Punjab province, Pakistan. The results revealed that the overall 58 samples were detected seropositive for orf virus, which show overall 13.2% seroprevalence in the Punjab province, Pakistan (Table I). Goats had a percentage positivity of 14.57, whereas sheep had a percentage positivity of 7.71. Moreover, the findings revealed that species were not significantly (χ2=2.9) (P=0.08) linked to contagious ecthyma. Goats had a 2.04 times higher chances of having contagious ecthyma than sheep. The commercially available ELISA kits detected IgG as early as 20th day post infection and level of antibodies was identified till 50th day post infection. Serologically positive samples were processed through PCR for confirmation. Positive amplified bands typical for GIF/IL-2 gene were revealed as shown in Figure 3 and Table I. Approximately 408 bp PCR amplified products of GIF/IL-2 gene of contagious ecthyma virus were produced in the procedure. Overall sero-prevalence of contagious ecthyma has been shown in Table I.

 

Sero-prevalence of contagious ecthyma virus among various districts

The results showed that the sero-positive samples for contagious ecthyma in goats were highest in districts Lahore, Lodhran and Dera Ghazi Khan (48.57, 42.42 and 41.38%, respectively). There was significant difference (χ2=112.5) (P<0.0001) in sero-positive samples of orf virus in goats among various districts, as shown in Figure 1A. The contagious ecthyma in sheep was sero-positive (53.8%) only in Muzaffargarh among various districts, as shown in Figure 2B.

 

Sero-prevalence of contagious ecthyma in goats based on risk factors

The higher sero-prevalence of contagious ecthyma in goats was found in 0-4 months kids (45.6%), as shown in Table II. The association amongst age groups for contagious ecthyma was significant (χ2=65.2) (P<0.0001) and young kids were 10.9 times more sero-positive than adults goats. The total of 46 (16.8%) female goats samples were sero-positive for contagious ecthyma, as shown in Table II. Gender based results showed significantly greater contagious ecthyma cases in female goats (χ2=4.9) (P=0.02). Female goats had 0.3 times larger probability of having contagious ecthyma than the males. The highest sero-prevalence of orf virus was in non-descript breed of goats (18.3%) and 5.4 times more orf virus sero-positive as compared to other breeds of goats, as shown in Table II. Whereas, the breed-wise prevalence was significantly associated with occurrence of contagious ecthyma in cases of goats (χ2=8.1) (P=0.04). The highest sero-prevalence of orf virus was in Non-descript breed of goats (18.3%) and non-descript breeds were 5.4 times more likely to have contagious ecthyma than Nachi, Deera Din Pananh, and Beetal, as shown in Table II. contagious ecthyma lesions, as well as their distribution on different body parts, were evaluated in relation to the occurrence of contagious ecthyma in goats. The higher percentage (21.8%) of contagious ecthyma was found in goats having gross lesions as shown in Table II. In goats, the presence of lesions were found to be significantly (χ2=19.9) (P<0.0001) associated with occurrence of contagious ecthyma. The percentage sero-positivity of contagious ecthyma in goats was significantly higher in animals that had lips lesion (19.5 %) as compared to infected animals having lesions on muzzle or nostril. The location of lesions on various body parts was significantly (χ2=11.3) (P=0.004) associated in goats. The occurrence of contagious ecthyma in goats was 3.7 times higher with lesions on their lips. Sero-prevalence of contagious ecthyma in goats based on risk factors has been shown in Table II.

Sero-prevalence of contagious ecthyma in sheep based on risk factors

The higher percentage (85.7 %) of sero-positivity was found in young lambs as shown in Table III. The association amongst age groups for contagious ecthyma was significant (χ2=65.2; P=0.0001) and the odd ratio (OR) showed that contagious ecthyma infect young lambs 498 times higher than adults, as shown in Table III.The association of sero-positivity of ORF virus among male

 

Table I. Overall sero-prevalence of contagious ecthyma.

Species

Total sample (n)

Seropositive %(n) IgG

Confirmation through

PCR (%) n

Chi-square

value

P value

OR

CI

Goat

350

14.6(51)

14.6(51)

2.9

0.08

2.04

(0.8,4.6)

Sheep

91

7.7(7)

7.7(7)

Overall

441

13.2(58)

13.2(58)

 

OR show odd ratio, CI show confident intervals, which was 95%.

 

Table II. Association of sero-prevalence of contagious ecthyma with relative risk factors in goats.

Variables

Categories

n

Sero-positive % (n)

Chi-square value

P value

OR

CI

Age

Young (0-4 months)

68

45.6(31)

65.2***

0.0001

10.9

(5.6, 21.1)

Adults (5 months-3 years)

282

7.1(20)

Gender

Male

76

6.6(5)

4.9*

0.02

Female

274

16.8(46)

0.3

(0.1, 0.9)

Breeds

Beetal

51

3.9(2)

8.1*

0.04

Dera Din Panah

34

8.8(3)

2.3

(0.3, 15.0)

Nachi

46

13(6)

3.6

(0.7, 19.1)

Non Descript

219

18.3(40)

5.4

(1.2, 23.2)

Orf lesions

Present

202

21.8(44)

19.9***

0.0001

5.6

(2.5, 13.2)

Absent

141

4.7(7)

Lesions on body parts

Lips

214

19.5(42)

11.3**

0.004

3.7

(1.1, 12.7)

Muzzle

104

6.7(7)

1.1

(0.2, 5.5)

Nostril

32

6.3(2)

 

n, total sample size; OR, odd ratio; CI, 95% confident intervals; * indicated P=0.02-0.04; ** indicated P=0.004 and *** indicated P=0.0001.

 

Table III. Relative risk factors association with sero-prevalence of contagious ecthyma in sheep.

Variables

Categories

n

Sero-positive % (n)

Chi-square value

P value

OR

CI

Age

Young (0-4 months)

7

85.7 (6)

65.2*

0.0001

498

(32.6, 851.1)

Adults (5 months-3 years)

84

1.2 (1)

Gender

Male

12

8.3 (1)

0.009

0.9

Female

79

7.6 (6)

1.1

(0.3, 10.9)

Breeds

Kajli

9

22.2 (2)

3.6

0.1

Thalli

7

14.3 (1)

1.1

(0.1, 25.1)

Non Descript

75

5.3 (4)

2.3

(0.2, 16.8)

Orf lesions

Present

68

8.8 (6)

0.5

0.4

2.1

(0.5, 7.2)

Absent

23

4.3 (1)

Lesions on body parts

Lips

31

16.1 (5)

4.7

0.09

5.5

(0.6, 62.7)

Muzzle

30

3.3 (1)

1.1

(0.2, 20.5)

Nostril

30

3.3 (1)

 

n, total sample size; OR, odd ratio; Cl, 95% confident intervals, * indicate P=0.0001

 

 

and female sheep was not significant (χ2=0.009) (P=0.9).Female sheep had 6 times larger probability of having contagious ecthyma than the males. Similarly, the association of sero-prevalence of contagious ecthyma was not significant among various breeds of sheep (χ2=3.6) (P=0.1). However, according to OR chances of contagious ecthyma was 2.3 times higher in Non-descript breed as compared to other breeds of sheep in Punjab Province. In sheep, the presence of lesions were found to be non-significantly (χ2=0.5) (P=0.4) associated with occurrence of contagious ecthyma. The location of lesions on various body parts was non-significantly (χ2=0.5) (P=0.4) associated in sheep. The percentage sero-positivity of contagious ecthyma in sheep was significantly higher in animals that had lips lesion (16.1 %) as compared to infected animals having lesions on muzzle or nostril. The occurrence of contagious ecthyma in sheep was 5.5 times higher with lesions on their lips. Sero-prevalence of contagious ecthyma in sheep based on risk factors has been shown in Table III.

Association of sero-prevalence of contagious ecthyma with months in sheep and goats

The higher percentage (78.4 and 71.4%) of sero-positivity was found in goats and sheep respectively from September to December months. The association for occurrence of contagious ecthyma was significant (χ2=78.4) (P=0.0001) in goats from September to December, as shown in Figure 2A. However, the association for prevalence of contagious ecthyma was non-significant (P=0.7) in sheep. Moreover, lower seroprevalence of contagious ecthyma from the months of May to August in goats, while in sheep sero-prevalence of contagious ecthyma was remain constant from January to August, as shown in Figure 2B. Association of sero-prevalence of contagious ecthyma with months has been shown in Figure 2A, B.

Association of sero-prevalence of contagious ecthyma with management risk factors in goats and sheep

The higher percentage (20 %) of sero-positivity was found in grazing goats. The association amongst various management risk factors for contagious ecthyma were significant (χ2=7.6) (P=0.002) as shown in Table IV and Figure 4. However, association for seroprevalence of contagious ecthyma in sheep was non-significant (χ2=0.42)

 

Table IV. Association of sero-prevalence of contagious ecthyma with management risk factors in goats.

Risk factor

Categories

n

Seroprevalence % (n)

Chi square value

P value

OR

CI

Feeding

Grazing

160

20(32)

7.6*

0.02

3.3

(1.6, 9.1)

Grazing + Stall

133

11.3(15)

1.6

(0.6, 5.4)

Stall feeding

57

7(4)

Injuries on skin

Present

200

20(40)

11.05**

0.001

3.1

(1.8, 12.6)

Absent

150

7.3(11)

Farming system (goat/sheep)

Mixed

186

15.1(28)

0.07

0.7

1.1

(0.1, 3.4)

Separated

164

14(23)

Purchase of new animals

Yes

250

19(40)

8.4**

0.004

2.7

(1.1, 10.3)

No

100

7.9(11)

 

n, total sample size; OR, odd ratio; Cl, 95% confidant intervals; * indicate significance value P=0.02 and ** indicate significance value P=0.004-0.001

 

Table V. Association of sero-prevalence of contagious ecthyma with management risk factors in sheep.

Risk factor

Categories

n

Seroprevalence % (n)

Chi square value

P value

OR

CI

Feeding

Grazing

55

9.1(5)

0.42

0.8

2.0

(0.41, 5.22)

Grazing + Stall

15

6.7(1)

1.4

(0.35, 4.61)

Stall feeding

21

4.8(1)

Injuries on skin

Present

44

13.6(6)

4.23*

0.04

3.1

(1.45, 8.11)

Absent

47

2.1(1)

Farming system (goat/sheep)

Mixed

57

8.8(5)

0.25

0.6

1.5

(0.2, 3.8)

Separated

34

5.9(2)

Purchase of new animals

Yes

44

13.6(6)

4.23*

0.04

3.1

(1.45, 8.11)

No

47

2.1(1)

 

n, total sample; OR, odd ratio; CI, 95% confident intervals; * indicate significance value P= 0.04

 

 

(P=0.8) amongst various groups: grazing, stall feeding and grazing and stall feeding animals, as shown in Table V. The seroprevalence of contagious ecthyma highly depends on cuts on skin as shown in findings: The seroprevalence of contagious ecthyma was significantly high in injured goats (χ2=11.05) (P=0.001) and sheep (χ2=4.23) (P=0.04) as compared to non-injured animals, as shown in Tables IV, V. There was no significant (P>0.05) association between seroprevalence of contagious ecthyma with farming system in both goats and sheep. The purchase of new animals was highly associated (P<0.05) with sero-prevalence of contagious ecthyma a in both goats and sheep. Association of sero-prevalence of contagious ecthyma with management risk factors in goats and sheep has been shown in Tables IV, V. Animals grazing areas and lips lesion in infected animals as shown in Figure 4.

DISCUSSION

This is the first study in Pakistan to present a detailed description of the prevalence of contagious ecthyma in goats and sheep using ELISA to detect antibodies and potential risk factors. Lahore, Lodhran, Dera Ghazi Khan, Multan, and Muzaffargarh had the most seropositive goats and sheep. In order to gain a clearer picture, sampling from a wider population of different areas of Punjab, Pakistan was conducted.

The prevalence of contagious ecthyma is higher in other parts of the world as compared to our findings, i.e., 13.2 percent ORF infection in our study as compared to 19.51 percent of lambs in England (Onyango et al., 2014), 34.89 percent in China (Gao et al., 2016), 98 percent in the Nilgiri Hills in Tamil Nadu, India (Balakrishnan et al., 2017), and 54 percent in Saudi Arabia (Housawi et al., 1992).

Our results showed that seroprevalence of contagious ecthyma were higher in goats (14.57%) than in sheep (7.71%). The prior studies also showed this trend. For example, prevalence of contagious ecthyma in sheep was 1.9 percent in England (Onyango et al., 2014), 34.9 percent in goats in China (Gao et al., 2016), 25.1-36.4 (Jesse et al., 2018) in Malaysia and 76.6 percent in Indian goats (Bora et al., 2016). The higher prevalence of contagious ecthyma in goats might be due to the fact that caprine are naturally more aggressive than ovine and consequently caprine are more likely to injure one another, making themselves more susceptible to ORF virus (Delhon et al., 2004; Orgeur et al., 1990). In goats and sheep, age was found to be a key driver of infection, suggesting that young goats and sheep are sensitive to ORF virus infection (Tables II, III). This conclusion is consistent with that of (Onyango et al., 2014), who discovered that contagious ecthyma is more common in lambs. Besides, age was also observed to be a significant determinant of infection in goats and sheep and our study indicated that kids and lambs are more susceptible to ORF virus infection (Tables II, III). This result is in agreement with the findings of (Onyango et al., 2014), who found that contagious ecthyma is more prevalent in lambs. Because of their immature immune systems, young animals were more susceptible to infection and acquired more serious lesions, which sometimes resulted in death (Spyrou and Valiakos, 2015). However, another study reported higher prevalence of contagious ecthyma in goats older than 8 months (Bora et al., 2016). Therefore, further studies are required to establish the role of age in the occurrence of contagious ecthyma.

In our study, gender was also found a significant driver of infection with females having higher seroprevalence of contagious ecthyma than males. An older study conducted by (Bora et al., 2016; Orgeur et al., 1990) also reported a similar observation. However, some researchers showed that ORF virus infection does not discriminate between males and females (Bora et al., 2016; Kumar et al., 2015). So, future studies should focus on establishing the role of gender in the susceptibility of contagious ecthyma in small ruminants. Male animals are usually slaughtered earlier as compared to female which are kept for longer period for breeding purpose and for yielding milk, male animals’ number is usually low in the area as compared to female animals.

To some extent, breed was also established as a risk factor for ORF virus infection in our study. Non-Descript goats and sheep had a greater prevalence of contagious ecthyma in this investigation. Worldwide, the findings of different researchers showed that contagious ecthyma is more common in some distinct breeds. For example, the seroprevalence of contagious ecthyma in Damara sheep and Indian, Chinese, and Boer goat breeds showed their higher susceptibility to ORF virus infection (Bora et al., 2016; Gao et al., 2016; Kumar et al., 2015). Therefore, future studies based on sampling from a wider population of various breeds would provide necessary data to establish the role of breed as a risk factor of contagious ecthyma.

As far as association of lesions with occurrence of disease is concerned, very interesting results were found. In few animals, gross lesions were not found but the animals found positive for contagious ecthyma via ELISA test. This might be due to the presence of IgG antibodies in animals as these antibodies are usually produced after three weeks of initiation of infection and wounds are mostly cured till that time. Conversely, a large no of animals was found negative although gross lesions were present. The reason in those cases would also be the same i.e., IgG did not start developing as samples of sera were taken in the first week of the disease outbreak.

The results of different months showed the highest occurrence of contagious ecthyma in the months from September to December (Fig. 2). Bora et al. (2016) and Chi et al. (2013) reported that production of antibodies against orf infection in infected animals does not give long-term protection. Higher incidence in these months might be due to the fact that cotton crop is ready in the month of September and cotton stubbles are present along with the leaves to be consumed by small ruminants in our study area. These cotton stubbles cause wounds, cuts, and abrasions, all of which serve as a predisposing factor for the virus penetration through the skin (Delhon et al., 2004; Orgeur et al., 1990) (Fig. 4). The high prevalence of orf infection might be due to shedding of viruses from injure animals in the environment, which is viable for long time (Bora et al., 2016) and they served as a source of seasonal outbreaks among same herd and also transmitted to neighbouring herds (Hota et al., 2018). The high prevalence of this disease highlights the infectious nature of ORF virus and its impact on the small ruminant industry (Housawi et al., 1992; Kumar et al., 2015). The high prevalence of this disease highlights the infectious nature of ORF virus and its impact on the small ruminant industry (Abd Elgowad et al., 2021; Kumar et al., 2015). Our study also reported that brining new animals in a herd increased the susceptibility of animals to ORF virus infection. We propose that the stress of traveling caused sickness and these stressed animals become more prone to ORF virus infection. However, Bala et al. (2019) reported that the infection could spread to other herds by moving infected animals. The both possibilities might be true in different cases.

PCR assay was used as confirmatory diagnostic tool for diseases. This assay has helped to distinguish ORF virus infection from other similar diseases affecting sheep and goats. All the serologically positive animals were confirmed through PCR assay on the scab or skin tissues samples (Kumar et al., 2015). Skin/scab tissue from the nostrils, lips, oral commissure, and muzzle showing nodular and diffuse proliferative cutaneous lesions (various stages of lesions formation like papules followed by vesicles, pustules, and finally scab formation) were collected for sampling.

It is concluded that the prevalence of contagious ecthyma infection by detecting IgG antibodies in sheep and goats in Punjab, Pakistan, was (13.2%). It was also noted that goats (14.57%) had higher prevalence of contagious ecthyma than sheep (7.71%). The occurrence of contagious ecthyma was found to be significantly associated with a number of risk factors, including species, gender, age, breed, presence or absence of lesions, seasons, and portable methods of transmission. The findings of study will serve as a baseline for future studies and will provide essential information for policy makers and epidemiologist for controlling contagious ecthyma in study area and beyond.

ACKNOWLEDGEMENTS

Authors are highly thankful to Prof. Dr. Aneela Zameer Durrani, Department of Clinical Medicine, Dr. Arfan Ahmed, University Diagnostic Laboratory, Institute of Microbiology, University of Veterinary and Animal Sciences Lahore for technical assistance.

Financial support

This study was supported by the Higher Education Commission of Pakistan under the project Faculty Development Program for Pakistani Universities Batch II (17-5/FVS2-001/HEC/Sch-FDP/2019).

Statement of conflict of ınterest

The authors have declared no conflict of interest.

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