CHARACTERIZATION OF THE 5' REGION OF THE MOUSE NATURAL KILLER RECOGNITION GENE

dc.contributor.authorSimons-Evelyn, Michelle
dc.contributor.departmentHood College Biology
dc.contributor.programBiomedical and Environmental Science
dc.date.accessioned2025-11-24T14:34:20Z
dc.date.issued1997-01
dc.description.abstractThe mouse Nktr (natural killer tumor recognition) gene was cloned and the 5' region characterized. The Nktr gene was found to be single copy and non-arranging and mapped to the distal end of mouse chromosome 9. This gene encodes for a 150 kilodalton protein homologous to cyclophilin, Nopp 140, and SR-containing proteins. Nktr expression is important for maintaining the lytic activity of natural killer cells. Eight exons and one alternate exon have been identified as well as a conserved intron sequence that may be important in the regulation of Nktr pre-mRNA splicing. Through the use of the Rnase protection assay, the Nktr transcriptional start site was identified and found to be 56 nucleotides upstream from the 5' end of a previously isolated cDNA sequence. The Nktr promoter region has features that are typical of a housekeeping gene, including a high G/C content, potential SP1 binding domains, and lack of TATA and CAAT boxes. Further upstream from the core promoter, there are several additional possible binding sites for CREB, AP-2, and Ets-1 binding proteins. To determine the activity of the Nktr promoter, beta-galactosidase reporter constructs driven by the Nktr promoter were generated. The activity of the constructs was equivalent in lymphocyte and fibroblast cell lines, suggesting that NK-TR protein expression is regulated by post-transcriptional mechanisms and not by the initiation of transcription.
dc.format.extent70 pages
dc.genreThesis (M.S.)
dc.identifierdoi:10.13016/m2marp-srve
dc.identifier.urihttp://hdl.handle.net/11603/41018
dc.language.isoen
dc.titleCHARACTERIZATION OF THE 5' REGION OF THE MOUSE NATURAL KILLER RECOGNITION GENE
dc.typeText

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