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271.
Sundaresan NR Marcus Leo MD Subramani J Anish D Sudhagar M Ahmed KA Saxena M Tyagi JS Sastry KV Saxena VK 《Veterinary research communications》2009,33(1):49-56
Melatonin (N-acetyl-5-methoxytryptamine), an indole hormone, regulates various biological functions through three different receptor subtypes
(Mel-1a, Mel-1b, and Mel-1c). However, the distribution of different melatonin receptor subtypes in chicken reproductive tissues
was not known. In the present investigation, the partial sequences of ovarian melatonin receptor subtypes (Mel-1a, Mel-1b,
and Mel-1c) were characterized. Further, the expression profile of melatonin receptor subtypes in the granulosa and theca
layers of different preovulatory and postovulatory follicles (POF) were studied by semi-quantitative RT-PCR. The expression
of all three subtypes of melatonin receptors were observed in the ovary of domestic chicken. Analysis of partial sequences
of ovarian melatonin receptors revealed that the melatonin subtypes were identical to the brain receptors. In small white
ovary follicles, we observed only the expression of mel-1b receptors, but not mel-1a or mel-1c receptors. In yellow follicles,
all the three subtypes of receptors expression were noticed. Interestingly, we observed the expression of mel-1a receptor
only in thecal layer, but not in granulosa layer. In contrast, mel-1b and -1c receptors were expressed in both granulosa and
thecal layer. During the regression of POF, we observed significant upregulation of melatonin receptors (mel-1a and 1c) expression,
that downregulated in the later stages of regression. We assume that the expression of melatonin receptors might have been
influenced by the atresia or apoptosis of different follicular layers in POF. Our findings suggest that the differential distribution
of melatonin receptor subtypes might have distinct downstream cellular functions in the ovarian tissues. 相似文献
272.
Nagarajan S Rajukumar K Tosh C Ramaswamy V Purohit K Saxena G Behera P Pattnaik B Pradhan HK Dubey SC 《Veterinary microbiology》2009,133(1-2):154-163
A total of 1246 faecal and tissue samples collected/received from 119 farms located in various states of India were processed for isolation of avian influenza viruses (AIV) during 2003-2004 as part of a program to monitor AIV infection in Indian poultry population. Avian influenza virus was isolated for the first time in India from poultry farms with history of drop in egg production, respiratory illness and increased mortality in Haryana state. A total of 29 H9N2 AIV isolates were obtained from the states of Punjab, Haryana, Uttar Pradesh, Gujarat, and Orissa and Union Territory Delhi. Subtyping was done by HI, RT-PCR and neuraminidase inhibition assay. Pathotyping of six representative isolates by intravenous pathogenicity index (0.0/3.0) in 6-8 weeks old chicken, trypsin dependency in cell culture and HA cleavage site analysis (335RSSR*GLF341) confirmed that these isolates are low pathogenic. Nucleotide sequence analysis of the HA gene showed that the Indian isolates are very closely related (95.0-99.6%) and shared a homology of 92-96% with H9N2 isolates from Germany and Asian regions other than that of mainland China. Deduced amino acid sequences showed the presence of L226 (234 in H9 numbering) which indicates a preference to binding of alpha (2-6) sialic acid receptors. Two of the six isolates had 7 glycosylation sites in the HA1 cleaved protein and the remaining four had 5 sites. Phylogenetic analysis showed that they share a common ancestor Qa/HK/G1/97 isolate which had contributed internal genes of H5N1 virus circulating in Vietnam. Further characterization of Indian H9N2 isolates is required to understand their nature and evolution. 相似文献