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Kerala Agricultural University, Thrissur

The history of agricultural education in Kerala can be traced back to the year 1896 when a scheme was evolved in the erstwhile Travancore State to train a few young men in scientific agriculture at the Demonstration Farm, Karamana, Thiruvananthapuram, presently, the Cropping Systems Research Centre under Kerala Agricultural University. Agriculture was introduced as an optional subject in the middle school classes in the State in 1922 when an Agricultural Middle School was started at Aluva, Ernakulam District. The popularity and usefulness of this school led to the starting of similar institutions at Kottarakkara and Konni in 1928 and 1931 respectively. Agriculture was later introduced as an optional subject for Intermediate Course in 1953. In 1955, the erstwhile Government of Travancore-Cochin started the Agricultural College and Research Institute at Vellayani, Thiruvananthapuram and the College of Veterinary and Animal Sciences at Mannuthy, Thrissur for imparting higher education in agricultural and veterinary sciences, respectively. These institutions were brought under the direct administrative control of the Department of Agriculture and the Department of Animal Husbandry, respectively. With the formation of Kerala State in 1956, these two colleges were affiliated to the University of Kerala. The post-graduate programmes leading to M.Sc. (Ag), M.V.Sc. and Ph.D. degrees were started in 1961, 1962 and 1965 respectively. On the recommendation of the Second National Education Commission (1964-66) headed by Dr. D.S. Kothari, the then Chairman of the University Grants Commission, one Agricultural University in each State was established. The State Agricultural Universities (SAUs) were established in India as an integral part of the National Agricultural Research System to give the much needed impetus to Agriculture Education and Research in the Country. As a result the Kerala Agricultural University (KAU) was established on 24th February 1971 by virtue of the Act 33 of 1971 and started functioning on 1st February 1972. The Kerala Agricultural University is the 15th in the series of the SAUs. In accordance with the provisions of KAU Act of 1971, the Agricultural College and Research Institute at Vellayani, and the College of Veterinary and Animal Sciences, Mannuthy, were brought under the Kerala Agricultural University. In addition, twenty one agricultural and animal husbandry research stations were also transferred to the KAU for taking up research and extension programmes on various crops, animals, birds, etc. During 2011, Kerala Agricultural University was trifurcated into Kerala Veterinary and Animal Sciences University (KVASU), Kerala University of Fisheries and Ocean Studies (KUFOS) and Kerala Agricultural University (KAU). Now the University has seven colleges (four Agriculture, one Agricultural Engineering, one Forestry, one Co-operation Banking & Management), six RARSs, seven KVKs, 15 Research Stations and 16 Research and Extension Units under the faculties of Agriculture, Agricultural Engineering and Forestry. In addition, one Academy on Climate Change Adaptation and one Institute of Agricultural Technology offering M.Sc. (Integrated) Climate Change Adaptation and Diploma in Agricultural Sciences respectively are also functioning in Kerala Agricultural University.

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19932
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Subject: Veterinary Microbiology × End date: 1993 × Start date: 1993 ×
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    ThesisItemOpen Access
    Assessment of immunity to duck plague virus (duck virus enteritis)
    (Department of Microbiology, College of Veterinary and Animal Sciences, Mannuthy, 1993) Diwakar Dattatrayrao, Kulkarni; KAU; James, P C
    During 1991, six outbreak clinically suspected to be duck plague (DP) with 33 per cent morbidity and 26 per cent mortality were investigated Duck plague virus was isolated from each outbreak. The isolates were able to produce the lesions and death of the duck embryos but failed to kill the chicken embryos during initial passages. One of the strains, named DP-S was partially attenuated by 10 passages in chicken .embryos following 20 passages in duck embryos. Though the attenuated strain did kill ducks, its pathogenicity index was reduced from 1.9 to 1,23. The isolate DP-S under transmission electron microscope revealed virions of herpes virus morphology. Two DP vaccines - commercial vaccine and lab-adapted vaccine having virus titres 0.74 and 3.5 log 10 ELD 50/ml respectively, were separately inoculated into four groups of ducklings respectively, two groups receiving single dose and two receiving double dose of corresponding vaccines at an interval of four weeks. Another group of ducklings was kept as control without vaccination. Three ducks in each group were challenged with virulent DPV at four,eight and 20 weeks post-vaccination. The birds in all the five groups were screened at regular intervals for studying the immune response by virus neutralization (VN), leucocyte migration-inhibition (LMI) and passive haemagglutination (PHA) test The challenged and survived birds were screened for the carrier status of DPV by examination of their rectal swabs for virus isolation. In an organized farm, 180 ducks were given commercial vaccine at one year of age and were screened for VN antibodies, LMI response and PHA titres before and eight weeks post -vaccination. Randomly selected two birds were challenged six weeks post-vaccination. The findings of the study are briefly listed as under: Six duck plague outbreaks were investigated, the virus isolated, and characterized. It was partially attenuated in duck and chicken embryos. The commercial, vaccine could elicit very poor immune response as compared to laboratory adapted vaccine. The immunity could not last long even upto eight weeks in single vaccination and 20 weeks in double vaccination.
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    ThesisItemOpen Access
    Characterization of plasmids of Escherichia coli isolated from mastitis
    (Department of Veterinary Microbiology, College of Veterinary and Animal Science, Mannuthy, 1993) Avinash Ganpatrao, Karpe; KAU; Punnoose, K T
    Escherichia coli. were isolated in 15.33 per cent cases of mastitis. Of the 46 E. coli isolated 43 were resistant to one to nine antibiotics and three were sensitive to all the 13 antibiotics tested. The organisms were resistant to rifampicin (78.26%) followed by oxytetracycline (50%), tetracycline (37.78%), nalidixic acid (19.56%), co-trimoxasole (8.69%) and gentamicin (6.52%). All the organisms were susceptible to kamamycin and norfloxacin. Among the .multiple drug resistance oxytetracycline - rifampicin (OR) resistance was noticed in 76.2% cases. Twenty-six different patterns of antibiotic resistance were noticed among 43 E. coli isolates giving a reliability of 60.46 per cent in differentiating the isolates. Hence, antibiogram could only be used as an adjunct to plasmid profiling in epidemiological studies. The resistograms revealed cent per cent resistance to lead, followed by antimony (32.6%), copper (30.43%), silver(19.56%) and cetrimide (2.17%). All the isolates were sensitive to cadmium and mercury. Among the 46 E. coli isolates, 9 different resistogram patterns were obtained giving reliability of 19.56 per cent in differentiating the strains. A correlation between the antibiotics and heavy metal ac; lead an+-imcny and copper, was observed inresistance such as leaa, descending order. of the forty-six E. coli isolates three (6.52%) were hemolytic on sheep blood agar. Two of the three hemolytic strains were also enterotoxigenic. Thirteen of the 46 (28.26%) E. coli isolates were enterotoxigenic, when tested by rabbit ligated ileal loop assay. Two of the thirteen (15.38%) enterotoxigenic isolates were also hemolytic. Fourteen of the 24 (58.33%) drug resistant E. coli transferred drug resistance against one or more antibiotics to the recipient organism. In none of the cases the furazolidone resistance was transferred. All the three hemolytic E. coli isolates transferred the hemolytic character by conjugation indicating the plasmid borne nature of hemolysin production. None of the enterotoxin producing E. coli could transfer the character to recipient by conjugation.