Your search keyword '"Jayarao, Bhushan M."' showing total 7 results

1. Identification and sub-typing of Mycobacterium avium subsp. paratuberculosis and Mycobacterium avium subsp. avium by randomly amplified polymorphic DNA

Author

Pillai, Shreekumar R, Jayarao, Bhushan M, Gummo, Jennifer D, Hue, Eric C, Jr., Tiwari, Deepanker, Stabel, Judith R, and Whitlock, Robert H

Published

2001

2. White Button Mushrooms Increase Microbial Diversity and Accelerate the Resolution of Citrobacter rodentium Infection in Mice.

Author

Varshney, Jyotika, Ooi, Jot Hui, Jayarao, Bhushan M., Albert, Istvan, Fisher, Jenny, Smith, Rhonda L., Patterson, Andrew D., and Cantorna, Margherita T.

Subjects

MUSHROOMS, CITROBACTER, METABOLOMICS, LABORATORY mice, CLOSTRIDIA, BACTEROIDES

Abstract

The effect of feeding C57BL/6 mice white button (WB) mushrooms or control (CTRL) diets for 6 wk was determined on the bacterial microflora, urinary metabolome, and resistance to a gastrointestinal (GI) pathogen. Feeding mice a diet containing 1 g WB mushrooms/100 g diet resulted in changes in the microfiora that were evident at 2 wk and stabilized after 4 wk of WB feeding. Compared with CTRL-fed mice, WB feeding (1 g/100 g diet) increased the diversity of the microflora and reduced potentially pathogenic (e.g., Clostridia) bacteria in the GI tract. Bacteria from the Bacteroidetes phylum increased and the Firmicutes phylum decreased in mushroom-fed mice compared with CTRL. The changes in the microflora were also reflected in the urinary metabolome that showed a metabolic shift in the WB-fed compared with the CTRL-fed mice. The WB feeding and changes in the microbiome were associated with fewer inflammatory cells and decreased colitis severity in the GI mucosa following Citrobacter rodentium infection compared with CTRL. Paradoxically, the clearance of C. rodentium infection did not differ even though Ifn-γ and II-17 were higher in the colons of the WB-fed mice compared with CTRL. Adding modest amounts of WB mushrooms (1 g/100 g diet) to the diet changed the composition of the normal flora and the urinary metabolome of mice and these changes resulted in better control of inflammation and resolution of infection with C. rodentium. [ABSTRACT FROM AUTHOR]

Published

2013

3. Spatial distribution of Burkholderia mallei in Punjab, Pakistan.

Author

Ali, Muhammad Asad, Muhammad, Khushi, Anjum, Aftab Ahmad, Ahmad, Mansur-ud-Din, Rabbani, Masood, Shabbir, Muhammad Zubair, Ahmad, Arfan, Muhammad, Javed, Chaudhry, Muhammad Hamid, Chaudhry, Haroon Rasheed, Ghori, Muhammad Tasleem, Jamil, Tariq, Haisem, Muhammad, and Jayarao, Bhushan M.

Published

2016

4. A probe-based real-time PCR assay for the detection of Neospora caninum in clinical samples from cattle.

Author

Barry, Rhiannon, Nissly, Ruth H., Feria, Willard, Thirumalapura, Nagaraja, Tewari, Deepanker, Jayarao, Bhushan M., and Kuchipudi, Suresh V.

Subjects

*NEOSPORA caninum, *GENE amplification, *BOVINE viral diarrhea, *BOVINE viral diarrhea virus, *DNA synthesis, *CATTLE

Abstract

• A probe-based real-time PCR assay for Neospora caninum detection is presented. • Assay demonstrates analytical sensitivity of 3 genomic copies of N. caninum DNA. • Assay results agree with established conventional PCR assay in bovine clinical samples. Neospora caninum is an apicomplexan protozoan parasite that is a leading cause of abortion in cattle. Detection of parasite-specific DNA by PCR is a highly sensitive method for identifying the presence of N. caninum in a variety of tissues. We developed and validated a probe-based real-time PCR assay targeting the conserved Nc5 gene of N. caninum. Using N. caninum strain Nc-1 genomic DNA and a synthetic gene fragment as amplification standards, we determined the PCR amplification efficiency and the limit of detection to be 95.60% and 3 copies, respectively. Five pathogens frequently associated with bovine abortions, namely bovine viral diarrhea virus types I and II, bovine alphaherpesvirus-1, Chlamydia, and Leptospira , were tested to ensure analytical exclusivity. A total of 103 clinical samples from aborted fetuses were tested concurrently with a standard conventional PCR and the new probe-based real-time PCR assay. All tested samples showed 100% agreement between these two assays. In conclusion, the probe-based real-time PCR assay facilitates accurate and rapid detection of N. caninum from abortions in cattle. [ABSTRACT FROM AUTHOR]

Published

2019

5. Seroprevalence and risk factors of glanders in working equines – Findings of a cross-sectional study in Punjab province of Pakistan.

Author

Ghori, Muhammad Taslim, Khan, Muhammad Sarwar, Khan, Jawaria Ali, Rabbani, Masood, Shabbir, Muhammad Zubair, Chaudhry, Haroon Rashid, Ali, Muhammad Asad, Muhammad, Javed, Elschner, Mandy Carolina, and Jayarao, Bhushan M.

Subjects

*BACTERIAL diseases in animals, *SEROPREVALENCE, *HORSE diseases, *DISEASE prevalence, *CROSS-sectional method

Abstract

Glanders is an infectious and contagious bacterial disease of equines. A little is known about its seroprevalence and risk factors in working equines in countries where the disease is endemic. Also, there are no reports on prevalence of the disease in areas where there is a prior evidence of Burkholderia (B.) mallei detection in soil. A cross-sectional study was conducted in selected districts (n = 09) of Punjab province of Pakistan during 2014–2015. A total of 1008 serum samples were screened for detection of antibodies to B. mallei with complement fixation test followed by western blot. The overall seroprevalence was found to be 3.17% (95% CI: 2.25–4.44). The seropositivity was significantly higher from the sampling sites where B. mallei was detected in soil [OR: 10.66 (95% CI: 4.42–31.66), p = 0.00]. Other risk factors significantly associated with animal seropositivity were: age group [OR: 1.78 (95% CI: 4.58–15.56), p = 0.00], location in urban area [OR: 2.99 (95% CI: 1.46–6.51), p = 0.00],body condition [OR: 3.47 (95% CI: 1.64–7.99), p = 0.00], presence of farcy lesion[OR: 7.71 (95% CI: 3.47–19.50), p = 0.00], proximity to water bodies [OR: 7.71 (95% CI: 3.47–19.50), p = 0.00]; domestic animal population [OR: 3.20 (95% CI: 1.24–10.87), p = 0.03] and number of households in sampling area [OR: 4.18 (95%CI: 1.82–11.30), p = 0.00]. The study provides an estimate of prevalence of glanders and a potential link between animal seropositivity and presence of B. mallei in soil. The risk factors identified in this study can be used in surveillance and disease awareness. The high prevalence of disease in draught horses and contact of infected animals with their care-takers in developing countries signify need to initiate progressive control of the disease using one health approach. [ABSTRACT FROM AUTHOR]

Published

2017

6. Evidence of Coxiella burnetii in Punjab province, Pakistan.

Author

Shabbir, Muhammad Zubair, Akram, Sidra, Hassan, Zia ul, Hanif, Kashif, Rabbani, Masood, Muhammad, Javed, Chaudhary, Muhammad Hamid, Abbas, Tariq, Ghori, Muhammad Taslim, Rashid, Haroon, Jamil, Tariq, Islam, Zia-ul-, Rasool, Haisem, Bano, Asghari, Ahmad, Arfan, Ali, Muhammad Asad, Yaqub, Tahir, McVey, Walt, and Jayarao, Bhushan M.

Subjects

*COXIELLA burnetii, *SEROCONVERSION, *BACTERIAL ecology, *POLYMERASE chain reaction, *DISEASE prevalence

Abstract

Coxiella burnetii causes query (Q) fever, an important zoonotic disease with worldwide significance. The role of environment in the ecology of C. burnetti , and its influence on seroconversion in animals has not been elucidated in Pakistan. We carried out a cross-sectional study in Punjab province to (1) determine the prevalence and distribution of C. burnetii in soil using an ISIIII gene-based real time-polymerase chain reaction (RT-PCR) assay, (2) analyze association between the occurrence of C. burnetii in soil and its predictors i.e. soil characteristics (macro- and micro-nutrients) and several likely risk factors including the seroconversion in small ruminants at places where its genome had or had not been detected, and (3) predict homology and genetic diversity of the identified strains using sequences originated from different hosts worldwide. A total of 2425 soil samples from nine districts of Punjab province were processed. C. burnetii DNA was detected in 47 samples (1.94%, 95% CI: ±0.55) originating from 35 villages of studied districts (7.22%, 95% CI: ±2.30). The highest prevalence was found in Attock (7.11%, 95% CI: ±3.36), followed by Lahore (4.83%, 95% CI: ±3.49), Sahiwal (4.70%, 95% CI: ±2.6), Dera Ghazi Khan (2.33%, 95% CI: ±2.02), Faisalabad (1.35%, 95% CI: ±1.18) and Sheikhupura (0.68%, 95% CI: ±0.94). The odds of detecting bacterial DNA in soil was increased with a unit increase in organic matter [2.511 (95% CI: 1.453–4.340), p = 0.001] and sodium [1.013 (95% CI: 1.005–1.022), p = 0.001], whereas, calcium [0.984 (95% CI: 0.975–0.994), p = 0.002] and potassium [0.994 (95% CI: 0.990–0.999), p = 0.011] had protective effect where a unit increase in each analyte decreased odds for its occurrence by 1.0% approximately. Likewise, for categorical variables (risk factors), the odds of detecting C. burnetii were higher at locations >500 m away from a main road [1.95 (95% CI: 1.06–3.78), p = 0.04]. The enzyme-linked immunosorbent assay (ELISA) revealed an increased prevalence of antibodies in sheep (17.9%, 95% CI: ±5.54) compared with goats (16.4%, 95% CI: ±4.34). When determining the association between soil DNA and C. burnetii antibodies in small ruminants, the odds of detecting these antibodies were significant in sheep at the livestock barns [2.81 (95% CI: 1.20–7.37), p = 0.02]. The IS1111 gene-based sequence analysis revealed a clustering of the DNA into two distinct groups with much genetic divergence (0.76–68.70%): the first group that contained sequences from Lahore district clustered with human and buffalo origin isolates, whereas the second group that contained the sequences from the remaining study districts clustered with goat-, rodent- and human-origin isolates. This study provides the first evidence of the presence of C . burnetii in the environment in Punjab province, Pakistan. Future studies are needed to ascertain the bacteria’s molecular epidemiology over a wide geographical area, type the isolates, and evaluates the potential risks to human populations, particularly farmers and veterinarians. [ABSTRACT FROM AUTHOR]

Published

2016

7. Blinded, controlled field trial of two commercially available Mycoplasma bovis bacterin vaccines in veal calves

Author

Soehnlen, Marty K., Aydin, Adnan, Lengerich, Eugene J., Houser, Beth A., Fenton, Ginger D., Lysczek, Hannah R., Burns, Carolyn M., Byler, Louise I., Hattel, Arthur L., Wolfgang, David R., and Jayarao, Bhushan M.

Subjects

*BACTERIAL vaccines, *MYCOPLASMA, *CALVES, *CATTLE diseases, *ANIMAL vaccination, *ETIOLOGY of diseases, *RESPIRATORY infections, *IMMUNOGLOBULINS, *ARTHRITIS

Abstract

Abstract: Mycoplasma bovis is an etiologic agent of pneumonia, arthritis, and otitis in young calves, such as those found in the special-fed veal industry. We conducted a blinded, controlled trial of two commercially available M. bovis bacterin vaccines for the prevention of respiratory disease in calves associated with M. bovis infection. Calves were randomly assigned to a subcutaneous treatment of vaccine A (n =50), adjuvant A (n =50), vaccine B (n =50), or 0.9% sterile saline solution (n =50) beginning at 27 days of age. Upper-respiratory tract colonization was not impacted by vaccination status. Vaccine A significantly reduced the presence of lung lesions (p =0.0325), however there was no significant reduction of M. bovis in lung lesions. Vaccine B did not significantly reduce total lung lesions or M. bovis-specific lung lesions. The relative risk was determined to be 0.56, 1.0, and 1.36 for vaccine A, adjuvant A, and vaccine B, respectively. There was no association between the total specific antibody isotype (IgM, IgG1, IgG2, IgA) concentrations or M. bovis antibodies and the M. bovis-associated morbidity in the veal calves. Under the field conditions of this study, observed vaccine efficacy for vaccine A and vaccine B was 44% and less than 1%, respectively. [Copyright &y& Elsevier]

Published

2011