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(Received for publication, April 21, 1995; and in revised form, July 12, 1995) The genome of Trypanosoma cruzi contains tandemly
arrayed copies of the gene encoding amastin, an abundant protein on the
surface of the amastigote stage of the parasite. The transcription rate
of the amastin genes is the same in the different developmental stages,
but the steady state level of the 1.4-kilobase amastin mRNA is
50-85 times higher in amastigotes than in epimastigotes or
trypomastigotes(1) . Here we show that the amastin genes
alternate with genes encoding another protein, called tuzin, whose
1.7-kilobase mRNA is much less abundant in amastigotes. The
3`-untranslated region (UTR) of tuzin mRNA is only a few nucleotides in
length or even nonexistent, in contrast with the 630-nucleotide 3`-UTR
of amastin mRNA. No promoter elements were found upstream or within the
amastin/tuzin gene cluster. However, in amastigotes, the protein
synthesis inhibitor cycloheximide caused a 3-fold decrease in amastin
mRNA and a 7-fold increase in tuzin mRNA. Furthermore, when the amastin
3`-UTR plus its downstream intergenic region were fused behind the
luciferase coding region in a chimeric plasmid for transient
transfections, luciferase activity increased 7-fold in amastigotes and
decreased 5-fold in epimastigotes. Thus, developmental expression of
these alternating genes is regulated by different mechanisms.
Volume 270,
Number 38,
Issue of September 22, pp. 22586-22594, 1995
©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
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