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2. Evolutionary and bioinformatic analysis of the spike glycoprotein gene of H120 vaccine strain protectotype of infectious bronchitis virus from India

Author

Sataish S Gaikwad, Sohini Dey, Sanjeev Kumar Shukla, C. Madhan Mohan, Sagar A. Khulape, Nitin M. Kamble, and Aravind S. Pillai

Subjects
0301 basic medicine, Serotype, 040301 veterinary sciences, Biomedical Engineering, Bioengineering, Infectious bronchitis virus, Applied Microbiology and Biotechnology, Microbiology, 0403 veterinary science, 03 medical and health sciences, Drug Discovery, Genotype, Genotyping, biology, Process Chemistry and Technology, Outbreak, 04 agricultural and veterinary sciences, General Medicine, Avian infectious bronchitis, biology.organism_classification, Virology, Vaccination, 030104 developmental biology, GenBank, Molecular Medicine, Biotechnology
Abstract

The infectious bronchitis virus is a causative agent of avian infectious bronchitis (AIB), and is is an important disease that produces severe economic losses to the poultry industry worldwide. Recent AIB outbreaks in India have been associated with poor growth in broilers, drop in egg production, and thin egg shells in layers. The complete spike gene of Indian AIB vaccine strain was amplified and sequenced using a conventional reverse transcription polymerase chain reaction and is submitted to the GenBank (accession no KF188436). Phylogenetic analysis revealed that the vaccine strain currently used belongs to H120 genotype, an attenuated strain of Massachusetts (Mass) serotype. Nucleotide and amino acid sequence comparisons have shown that the reported spike gene from Indian isolates have 71.8%-99% and 71.4%-96.9% genetic similarity with the sequenced H120 strain. The study identifies live attenuated IBV vaccine strain, which is routinely used for vaccination, for the first time. Based on nucleotide and amino acid relatedness studies of the vaccine strain with reported IBV sequences from India, it is shown that the current vaccine strain is efficient in controlling the IBV infection. Continuous monitoring of IBV outbreaks by sequencing for genotyping and in vivo cross protection studies for serotyping is not only important for epidemiological investigation but also for evaluation of efficacy of the current vaccine.

Published
2016
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3. Evolutionary and bioinformatic analysis of the spike glycoprotein gene of H120 vaccine strain protectotype of infectious bronchitis virus from India

Author

Nitin Machindra, Kamble, Aravind S, Pillai, Satish S, Gaikwad, Sanjeev Kumar, Shukla, Sagar Aashok, Khulape, Sohini, Dey, and C Madhan, Mohan

Subjects
Genotype, H120, Infectious bronchitis virus, Molecular Sequence Data, Computational Biology, India, Viral Vaccines, Original Articles, spike, Protein Sorting Signals, Vaccines, Attenuated, phylogeny, Poultry, infectious bronchitis, Viral Proteins, Animals, Original Article, Amino Acid Sequence, Coronavirus Infections, Poultry Diseases, Glycoproteins
Abstract

The infectious bronchitis virus is a causative agent of avian infectious bronchitis (AIB), and is is an important disease that produces severe economic losses to the poultry industry worldwide. Recent AIB outbreaks in India have been associated with poor growth in broilers, drop in egg production, and thin egg shells in layers. The complete spike gene of Indian AIB vaccine strain was amplified and sequenced using a conventional reverse transcription polymerase chain reaction and is submitted to the GenBank (accession no KF188436). Phylogenetic analysis revealed that the vaccine strain currently used belongs to H120 genotype, an attenuated strain of Massachusetts (Mass) serotype. Nucleotide and amino acid sequence comparisons have shown that the reported spike gene from Indian isolates have 71.8%–99% and 71.4%–96.9% genetic similarity with the sequenced H120 strain. The study identifies live attenuated IBV vaccine strain, which is routinely used for vaccination, for the first time. Based on nucleotide and amino acid relatedness studies of the vaccine strain with reported IBV sequences from India, it is shown that the current vaccine strain is efficient in controlling the IBV infection. Continuous monitoring of IBV outbreaks by sequencing for genotyping and in vivo cross protection studies for serotyping is not only important for epidemiological investigation but also for evaluation of efficacy of the current vaccine.

Published
2014

4. Diagnosis of leptospirosis by recombinant antigen based single serum dilution ELISA

Author

Sohini, Dey, C Madhan, Mohan, P, Ramadass, and K, Nachimuthu

Subjects
Antigens, Bacterial, Lipoproteins, Humans, Regression Analysis, Enzyme-Linked Immunosorbent Assay, Leptospirosis, Skin Test End-Point Titration, Leptospira interrogans, Sensitivity and Specificity, Bacterial Outer Membrane Proteins
Abstract

Leptospirosis, a zoonosis with a worldwide distribution is an acute febrile illness caused by spirochaetes of the pathogenic Leptospira interrogans. Microscopic agglutination test (MAT), the reference method for diagnosis was successively done to evaluate the modified ELISA which was developed with the recombinant LipL32 antigen for the detection of anti-leptospiral antibodies in human serum samples.The recombinant LipL32 antigen was developed from the serovar Pomona strain Pomona of the pathogenic L. interrogans species. The predicted titre at a single working dilution was plotted against the observed antiserum titre. Subsequently, predicted antibody activity titres were determined directly from the standard curve by solving the regression line equation. The relative sensitivity, specificity and accuracy of the single dilution ELISA for the detection of anti-leptospiral antibodies were determined in comparison to the MAT.A linear relationship was found between the predicted antibody titres at a single working dilution of 1:250 and the corresponding observed serum titres by the standard serial-dilution method. Regression analysis was used to determine a standard curve from which an equation was derived that allowed demonstration of the mentioned correlation. The equation was then used to convert the corrected absorbance readings of the single working dilution directly into the predicted ELISA antibody titres. A high level of sensitivity of 96 per cent and specificity of 91 per cent between ELISA and MAT titres was found. The kappa value was almost 1.0 indicating perfect agreement.The r LipL32 ELISA was proved to be sensitive, specific and accurate as compared to the standard MAT and the test could be efficiently utilized as a screening test for a large number of human serum samples for the detection of leptospiral antibodies.

Published
2008

5. Molecular changes of the fusion protein gene of chicken embryo fibroblast-adapted velogenic Newcastle disease virus: effect on its pathogenicity

Author

K. Kumanan, Sohini Dey, and C. Madhan Mohan

Subjects
animal structures, Sequence analysis, viruses, Molecular Sequence Data, Adaptation, Biological, Newcastle disease virus, Virulence, India, Chick Embryo, Biology, Newcastle disease, Virus, Fusion gene, Food Animals, Animals, Amino Acid Sequence, Cloning, Molecular, Serial Passage, Gene, DNA Primers, General Immunology and Microbiology, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, Embryo, Sequence Analysis, DNA, Fibroblasts, biology.organism_classification, Virology, Molecular biology, Fusion protein, Culture Media, embryonic structures, Animal Science and Zoology, Chickens, Viral Fusion Proteins
Abstract

Molecular changes of cell culture-adapted Newcastle disease virus (NDV) were studied by adapting a velogenic NDV isolated from commercial layer chicken-to-chicken embryo fibroblast (CEF) cells. The isolate was passaged 50 times in CEF cells. At every 10th passage the virus was characterized conventionally by mean death time analysis, intracerebral pathogenicity index, and virus titration. As the passage level increased, a gradual reduction in the virulence of the virus was observed. Molecular characterization of the virus included cloning and sequencing of a portion of the fusion gene (1349 bp) encompassing the fusion protein cleavage site (FPCS), which was previously amplified by reverse transcription-polymerase chain reaction. Sequence analysis revealed a total of 134 nucleotide substitutions, which resulted in the change of 41 amino acids between the parent and the 50th passage virus. Pathogenicity studies conducted in 20-wk-old seronegative chickens revealed gross and histopathologic changes in the chickens injected with the parent virus and absence of the lesions in chickens injected with the adapted virus. The 50th passage cell culture virus was back-passaged five times in susceptible chickens and was subjected to virulence attribute analysis and sequence analysis of the FPCS region, with minor differences between them.

Published
2005

6. Clonidine as an adjuvant in monitored anesthesia care for ENT surgeries: A prospective, randomized, double blind placebo controlled study.

Author

Kumari, Indira, Naithani, Udita, Harsha, Singhal, Yogendra, Meena, Khemraj, and C., Madhan Mohan

Subjects
*CLONIDINE, *ANESTHESIA in otolaryngology, *PAIN measurement, *THERAPEUTICS
Abstract

Objective: Alpha-2 adrenoceptors have recently been used perioperatively for their sedative, analgesic, sympatholytic and cardiovascular stabilizing effects. The efficacy of clonidine as an adjuvant in providing monitored anesthesia care (MAC) for ear, nose and throat (ENT) surgeries has not been much investigated, so we conducted this study. Methodology: In this prospective double blind randomized placebo controlled study, 90 patients posted for elective ENT surgeries under local anesthesia with MAC were included and divided into 3 groups of 30 each. In Group CBI patients received clonidine 3 μg/kg intravenous bolus followed by clonidine infusion at 0.3 μg/kg/hr. Patients of Group CB received clonidine 3 μg/kg bolus followed by placebo infusion and in Group P patients received placebo bolus followed by placebo infusion. All three Groups received similar premedication of intravenous midazolam 0.03 mg/kg and fentanyl 2 μg/kg. Demographic data, intraoperative vital parameters, observer's assessment and alertness scale (OAAS) score for sedation, bleeding score, patient and surgeon satisfaction score, postoperative Aldrete score, visual analogue scale (VAS) score for analgesia, rescue sedative and analgesic consumption and complications were noted. Results: OAAS score (0-noresponse to 5-awake), 10 min after infusion of study drug was significantly lower in Groups CBI (2.06 ± 0.61) and CB (2.83 ± 0.70) signifying superior sedation as compared to placebo Group (4.80 ± 0.40), (p=0.000). Intraoperative rescue sedative and analgesic consumption were significantly lower in Groups CBI and CB, as compared to placebo group (p = 0.000). Mean heart rate (HR) and mean arterial pressure (MAP) were significantly lower in Groups CBI and CB as compared to Group P (p = 0.000). Intraoperative bleeding score (0-Nolbleeding to 4-modearte bleeding) was significantly lower in Group CBI (0.86 ± 0.68) and CB (1.36 ± 0.76) as compared to placebo (3.10 ± 0.54), p = 0.000. Surgeons and patients were more satisfied in clonidine Groups CBI and CB, (p = 0.000). Patients of Group CBI demonstrated better sedation profile, less bleeding score and higher satisfaction scores as compared to Group CB (p<0.05). Conclusion: Being a safe, well tolerated, cheap and effective regime, our study favors the use of clonidine 3 μg/kg IV bolus followed by infusion of 0.3 μg/kg/hr as an adjunct to conventional MAC regime of midazolam and fentanyl in ENT surgeries as it provides effective sedation and bloodless surgical field. [ABSTRACT FROM AUTHOR]

Published
2015

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