Antigenic variation in Trypanosoma brucei: a telomeric expression site for variant-specific surface glycoprotein genes with novel features

doi:10.1093/nar/19.7.1359

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Nucleic Acids Research, 1991, Vol. 19, No. 7 1359-1368
© 1991

MOLECULAR BIOLOGY

Antigenic variation in Trypanosoma brucei: a telomeric expression site for variant-specific surface glycoprotein genes with novel features

Joost C.B.M. Zomerdijk, Rudo Kieft, Monique Duyndam, Paul G. Shiels and Piet Borst^*

Division of Molecular Biology, The Netherlands Cancer Institute Plesmanlaan 121, 1066 CX Amsterdam, The Netherlands

^* To whom correspondence should be addressed

Received February 13, 1991. Accepted March 12, 1991.

African trypanosomes evade the immune response of their hostby periodically changing their variant surface glycoprotein(VSG) coat. Each coat is encoded by a separate VSG gene. Expressedgenes are in a telomeric expression site (ES) and there areseveral sites in each trypanosome. To study the transcriptioncontrol of VSG genes in Trypanosoma brucei we have analyzedan ES, called the dominant ES (DES), that readily switches offand on. The promoter area of the DES is very similar to thatof the 221 ES (Zomerdijk et al., 1990). It can be switched offand on in vivo without detectable DNA alterations in the vicinityof the transcription start and it can drive high transient expressionof a reporter gene in transfection experiments. However, thereare also two major differences between the DES and the 221 ES.First, one version of the DES contains an additional upstreamtranscription unit overlapping the VSG gene ES promoter. Thepresence of this upstream transcription is dispensable, however,for the VSG gene ES promoter is active, even if transcriptionthrough this start from the upstream promoter is blocked usingUV light. Moreover, a second version of the DES present in anothertrypanosome variant does not produce these upstream transcripts.Secondly, we find that the inactivation of DES transcriptionin one trypanosome variant is accompanied by DNA alterationsin the DES upstream (>2 kb) of the transcription start; reactivationof DES transcription is accompanied by another alteration farupstream. Although we cannot exclude that these DNA rearrangementsare incidental, our results raise the possibility that the activityof ES promoters is negatively controlled in cis by far jpstreamsequences not included in transfection constructs and that alterationsin these sequences may lead to (in)activation of the promoter.

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