Myler, P. J. ; Sisk, E. ; McDonagh, P. D. ; Martinez-Calvillo, S. ; Schnaufer, A. ; Sunkin, S. M. ; Yan, S. ; Madhubala, R. ; Ivens, A. ; Stuart, K. (2000) Genomic organization and gene function in Leishmania Biochemical Society Transactions, 28 . pp. 527-531. ISSN 0300-5127
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Official URL: http://www.biochemsoctrans.org/bst/028/bst0280527....
Abstract
Sequencing of the Leishmania major Friedlin genome is well underway with chromosome 1 (Chr1) and Chr3 having been completely sequenced, and Chr4 virtually complete. Sequencing of several other chromosomes is in progress and the complete genome sequence may be available as soon as 2003. A large proportion ( ≈ 70%) of the newly identified genes remains unclassified, with many of these being potentially Leishmania- (or kinetoplastid-) specific. Most interestingly, the genes are organized into large (> 100-300 kb) polycistronic clusters of adjacent genes on the same DNA strand. Chr1 contains two such clusters organized in a 'divergent' manner, i.e. the mRNAs for the two sets of genes are both transcribed towards the telomeres. Chr3 contains two 'convergent' clusters, with a single 'divergent' gene at one telomere, with the two large clusters separated by a tRNA gene. We have characterized several genes from the LD1 (Leishmania DNA 1) region of Chr35. BT1 (formerly ORFG) encodes a biopterin transporter and ORFF encodes a nuclear protein of unknown function. Immunization of mice with recombinant antigens from these genes results in significant reduction in parasite burden following Leishmania challenge. Recombinant ORFF antigen shows promise as a serodiagnostic. We have also developed a tetracycline-regulated promoter system, which allows us to modulate gene expression in Leishmania.
Item Type: | Article |
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Source: | Copyright of this article belongs to Portland Press Limited. |
Keywords: | Genome Sequencing; Regulatable Promoter; Serodiagnosis; Transcription; Vaccine; |
ID Code: | 29843 |
Deposited On: | 23 Dec 2010 04:34 |
Last Modified: | 17 May 2016 12:38 |
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