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布氏锥虫体外可变表面糖蛋白(VSG)表达位点转换的分析

Analysis of Trypanosoma brucei vsg expression site switching in vitro.

作者信息

Horn D, Cross G A

机构信息

Laboratory of Molecular Parasitology, Rockefeller University, New York, NY 10021-6399, USA.

出版信息

Mol Biochem Parasitol. 1997 Feb;84(2):189-201. doi: 10.1016/s0166-6851(96)02794-6.

Abstract

Trypanosoma brucei can undergo antigenic variation by switching between distinct telomeric variant surface glycoprotein gene (vsg) expression sites (ESs) or by replacing the active vsg. DNA rearrangements have often been associated with ES switching, but it is unclear if such rearrangements are necessary or whether ES inactivation always accompanies ES activation. To explore these issues, we derived ten independent clones, from the same parent, that had undergone a similar vsg activation event. This was achieved in the absence of an immune response, in vitro, using cells with selectable markers integrated into an ES. Nine of the ten clones had undergone ES switching. Such heritable changes in transcription state occurred at a frequency of approximately 6 x 10(-7). Comparison of switched and un-switched clones highlighted the dynamic nature of T. brucei telomeres, but changes in telomere length were not specifically associated with ES switching. Mapping within and beyond the ESs revealed no detectable DNA rearrangements, indicating that rearrangements are not necessary for ES activation/inactivation. Examination of individual cells indicated that ES activation consistently accompanied inactivation of the previously active ES. In some cases, however, we found cells that appeared to have efficiently established the switched state but which subsequently, at a frequency of approximately 2 x 10(-3), generated cells expressing both pre- and post-switch vsgs. These results show that ES activation/inactivation is usually a coupled process but that cells can inherit a propensity to uncouple these events.

摘要

布氏锥虫可通过在不同的端粒可变表面糖蛋白基因(vsg)表达位点(ESs)之间切换或替换活性vsg来进行抗原变异。DNA重排常与ES切换相关,但尚不清楚此类重排是否必要,或者ES失活是否总是伴随着ES激活。为了探究这些问题,我们从同一亲本中获得了十个独立的克隆,它们经历了相似的vsg激活事件。这是在无免疫反应的体外条件下,使用整合有选择标记到一个ES中的细胞实现的。十个克隆中有九个发生了ES切换。这种转录状态的可遗传变化发生频率约为6×10⁻⁷。对切换和未切换克隆的比较突出了布氏锥虫端粒的动态性质,但端粒长度的变化与ES切换并无特异性关联。对ES内部及以外区域的定位分析未发现可检测到的DNA重排,表明重排对于ES激活/失活并非必要。对单个细胞的检测表明,ES激活始终伴随着先前活性ES的失活。然而,在某些情况下,我们发现一些细胞似乎有效地建立了切换状态,但随后以约2×10⁻³的频率产生了同时表达切换前和切换后vsg的细胞。这些结果表明,ES激活/失活通常是一个耦合过程,但细胞可以继承使这些事件解耦的倾向。

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