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J Biol Chem, Vol. 274, Issue 24, 16876-16883, June 11, 1999
The Anatomy and Transcription of a Monocistronic Expression
Site for a Metacyclic Variant Surface Glycoprotein Gene in
Trypanosoma brucei
Mehrdad
Pedram and
John E.
Donelson
From the Department of Biochemistry, University of Iowa,
Iowa City, Iowa 52242
African trypanosomes evade the immune response of
their mammalian hosts by switching the expression of their variant
surface glycoprotein genes (vsg). The bloodstream
trypanosome clone MVAT4 of Trypanosoma brucei rhodesiense
expresses a metacyclic vsg as a monocistronic RNA from a
promoter located 2 kilobases (kb) upstream of its start codon.
Determination of 23 kb of sequence at the metacyclic variant antigen
type 4 (MVAT) vsg expression site (ES) revealed an
ES-associated gene (esag) 1 preceded by an ingi
retroposon and an inverted region containing an unrelated
vsg, short stretches of 70-bp repeats and a pseudo
esag 3. Nuclear run-on experiments indicate that the 18-kb
region upstream of the MVAT4 vsg promoter is
transcriptionally silent. However, multiple members of different esag families are expressed from elsewhere in the genome.
The MVAT4 vsg promoter is highly repressed in the procyclic
stage, in contrast to the known polycistronic vsg ESs which
undergo abortive transcription. Activation of the MVAT4 vsg
ES occurs in situ without nucleotide sequence changes,
although this monocistronic ES undergoes a pattern of base J
modifications similar to that reported for the polycistronic ESs. The
relative simplicity of the MVAT4 vsg ES and the uncoupled
expression of the vsg and esags provide a unique opportunity for investigating the molecular mechanisms responsible for antigenic variation in African trypanosomes.
Copyright © 1999 by The American Society for Biochemistry and Molecular Biology, Inc.

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Copyright © 1999 by the American Society for Biochemistry and Molecular Biology.
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