Nucleotide polymorphisms in the bovine lymphotoxin A gene and their distribution among Bos indicus zebu cattle breeds

The present study was undertaken to characterize the genetic variation present in lymphoxin A gene (LTA gene) encoding for the lymphotoxin A protein also known as tumor necrosis factor beta, a cytokine produced by lymphocytes, known to be cytotoxic for a wide range of tumor cells both in vitro and i...

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Bibliographic Details
Published in:Gene 2016-03, Vol.579 (1), p.82-94
Main Authors: Behl, Jyotsna Dhingra, Mishra, Priyanka, Verma, N.K., Niranjan, S.K., Dangi, P.S., Sharma, Rekha, Behl, Rahul
Format: Article
Language:English
Subjects:
Animals
Binding Sites
Bos
Bos indicus
Breeding
Cattle - genetics
Cattle - immunology
Gene Frequency
Genetic variability
Genotype
Haplotypes
INDEL Mutation
Lymphotoxin-alpha - chemistry
Lymphotoxin-alpha - genetics
Lymphotoxin-alpha - metabolism
Paired Box Transcription Factors - metabolism
Polymorphism, Single Nucleotide
Promoter Regions, Genetic
Proto-Oncogene Proteins c-rel - genetics
Proto-Oncogene Proteins c-rel - metabolism
SNPs
Tumour necrosis factor beta gene
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Summary:The present study was undertaken to characterize the genetic variation present in lymphoxin A gene (LTA gene) encoding for the lymphotoxin A protein also known as tumor necrosis factor beta, a cytokine produced by lymphocytes, known to be cytotoxic for a wide range of tumor cells both in vitro and in vivo, and, which is essential for normal immunological development; in 40 animals of 5 diverse Bos indicus Indian zebu cattle breeds. These breeds survive under the harsh and tough tropical climatic conditions of various parts of the Indian subcontinent. The LTA gene in the present study was observed to contain 33 SNPs and 3 small insertion/deletion polymorphisms. Four SNPs occurred in the coding regions of the gene viz. g.1327A>G and g.1400C>T in exon 2 and g.1840C>T and g.1942C>T in exon 3, of which the SNP g.1327A>G in exon 2 resulted in a non-synonymous amino acid change G38D. This amino acid change was however predicted not be affecting the protein function in any manner. The gene contained putative transcription factor binding sites for the c-Re1 and for Pax-4 transcription factors. A putative promoter region was also predicted on the reverse DNA strand from position 894 to 644. Several repeat elements and microsatellite repeats were detected to be occurring across the 3.2kb LTA gene sequence. The study showed the occurrence of 40 genotypes and 48 most probable haplotypes. The genotypes at the observed SNP positions in the LTA gene were in near Hardy–Weinberg equilibrium. A negative Tajima's D value that was not significant statistically at P>0.10 indicated that the neutral mutation hypothesis could not be excluded. The genetic variations observed in the LTA gene in the present study have not been reported earlier and these could possibly be used as molecular markers for further studies involving association of the gene variability with disease resistance/tolerance traits. •Thirty three SNPs and 3 INDELS were deciphered in Bos indicus lymphotoxin A gene.•The SNP g.1327A>G in exon 2 resulted in amino acid change G38D.•Two putative TFBS — c-Re1 and Pax-4, were observed. No SNP was found in the TFBS.•The Tajima's D value indicated that the observed gene variation was neutral.
ISSN:0378-1119
1879-0038
DOI:10.1016/j.gene.2015.12.049