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布氏锥虫中活跃的VSG表达位点缺乏核小体。

Active VSG expression sites in Trypanosoma brucei are depleted of nucleosomes.

作者信息

Stanne Tara M, Rudenko Gloria

机构信息

The Peter Medawar Building for Pathogen Research, University of Oxford, South Parks Road, Oxford OX1 3SY, United Kingdom.

出版信息

Eukaryot Cell. 2010 Jan;9(1):136-47. doi: 10.1128/EC.00281-09. Epub 2009 Nov 13.

Abstract

African trypanosomes regulate transcription differently from other eukaryotes. Most of the trypanosome genome is constitutively transcribed by RNA polymerase II (Pol II) as large polycistronic transcription units while the genes encoding the major surface proteins are transcribed by RNA polymerase I (Pol I). In bloodstream form Trypanosoma brucei, the gene encoding the variant surface glycoprotein (VSG) coat is expressed in a monoallelic fashion from one of about 15 VSG bloodstream form expression sites (BESs). Little is known about the chromatin structure of the trypanosome genome, and the chromatin state of active versus silent VSG BESs remains controversial. Here, we determined histone H3 occupancy within the genome of T. brucei, focusing on active versus silent VSG BESs in the bloodstream form. We found that histone H3 was most enriched in the nontranscribed 50-bp and 177-bp repeats and relatively depleted in Pol I, II, and III transcription units, with particular depletion over promoter regions. Using two isogenic T. brucei lines containing marker genes in different VSG BESs, we determined that histone H3 is 11- to 40-fold depleted from active VSG BESs compared with silent VSG BESs. Quantitative PCR analysis of fractionated micrococcal nuclease-digested chromatin revealed that the active VSG BES is depleted of nucleosomes. Therefore, in contrast to earlier views, nucleosome positioning appears to be involved in the monoalleleic control of VSG BESs in T. brucei. This may provide a level of epigenetic regulation enabling bloodstream form trypanosomes to efficiently pass on the transcriptional state of active and silent BESs to daughter cells.

摘要

非洲锥虫调节转录的方式与其他真核生物不同。锥虫基因组的大部分由RNA聚合酶II(Pol II)组成型转录为大型多顺反子转录单元,而编码主要表面蛋白的基因则由RNA聚合酶I(Pol I)转录。在布氏锥虫的血流形式中,编码可变表面糖蛋白(VSG)外壳的基因以单等位基因方式从约15个VSG血流形式表达位点(BESs)之一表达。关于锥虫基因组的染色质结构知之甚少,活跃与沉默的VSG BESs的染色质状态仍存在争议。在这里,我们确定了布氏锥虫基因组中组蛋白H3的占有率,重点关注血流形式中活跃与沉默的VSG BESs。我们发现组蛋白H3在非转录的50 bp和177 bp重复序列中富集最多,而在Pol I、II和III转录单元中相对减少,在启动子区域尤其减少。使用两个在不同VSG BESs中含有标记基因的同基因布氏锥虫系,我们确定与沉默的VSG BESs相比,活跃的VSG BESs中组蛋白H3减少了11至40倍。对微球菌核酸酶消化的染色质进行分级分离后的定量PCR分析表明,活跃的VSG BESs缺乏核小体。因此,与早期观点相反,核小体定位似乎参与了布氏锥虫中VSG BESs的单等位基因控制。这可能提供了一种表观遗传调控水平,使血流形式的锥虫能够有效地将活跃和沉默BESs的转录状态传递给子细胞。

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