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KRAB 锌指蛋白基因在小鼠谱系中活跃的逆转录转座子作用下的扩增。

KRAB-zinc finger protein gene expansion in response to active retrotransposons in the murine lineage.

机构信息

The Eunice Kennedy Shriver National Institute of Child Health and Human Development, The National Institutes of Health, Bethesda, United States.

School of Life Sciences, École Polytechnique Fédérale de Lausanne (EPFL), Lausanne, Switzerland.

出版信息

Elife. 2020 Jun 1;9:e56337. doi: 10.7554/eLife.56337.

Abstract

The Krüppel-associated box zinc finger protein (KRAB-ZFP) family diversified in mammals. The majority of human KRAB-ZFPs bind transposable elements (TEs), however, since most TEs are inactive in humans it is unclear whether KRAB-ZFPs emerged to suppress TEs. We demonstrate that many recently emerged murine KRAB-ZFPs also bind to TEs, including the active ETn, IAP, and L1 families. Using a CRISPR/Cas9-based engineering approach, we genetically deleted five large clusters of KRAB-ZFPs and demonstrate that target TEs are de-repressed, unleashing TE-encoded enhancers. Homozygous knockout mice lacking one of two KRAB-ZFP gene clusters on chromosome 2 and chromosome 4 were nonetheless viable. In pedigrees of chromosome 4 cluster KRAB-ZFP mutants, we identified numerous novel ETn insertions with a modest increase in mutants. Our data strongly support the current model that recent waves of retrotransposon activity drove the expansion of KRAB-ZFP genes in mice and that many KRAB-ZFPs play a redundant role restricting TE activity.

摘要

Krüppel 相关盒锌指蛋白 (KRAB-ZFP) 家族在哺乳动物中多样化。大多数人类 KRAB-ZFPs 结合转座元件 (TEs),然而,由于大多数 TEs 在人类中是不活跃的,因此不清楚 KRAB-ZFPs 是否是为了抑制 TEs 而出现的。我们证明,许多新出现的鼠 KRAB-ZFPs 也与 TEs 结合,包括活跃的 ETn、IAP 和 L1 家族。我们使用基于 CRISPR/Cas9 的工程方法,对五个大的 KRAB-ZFP 簇进行了基因缺失,并证明了靶 TEs 被解除抑制,释放了 TE 编码的增强子。尽管两条 2 号染色体和 4 号染色体上缺失了两个 KRAB-ZFP 基因簇的纯合敲除小鼠仍然具有活力。在 4 号染色体簇 KRAB-ZFP 突变体的家系中,我们发现了许多新的 ETn 插入,突变体中有适度增加。我们的数据强烈支持当前的模型,即最近的逆转座子活动浪潮推动了小鼠 KRAB-ZFP 基因的扩张,并且许多 KRAB-ZFPs 发挥冗余作用限制了 TE 活性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/08dc/7289599/e952acd12dc4/elife-56337-fig1.jpg

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