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对 H19 启动子或其 ICR1 远端区域的 DNA 甲基化进行筛选,可确保 Russell-Silver 综合征中 11p15 染色体的高效检测。

Screening of DNA methylation at the H19 promoter or the distal region of its ICR1 ensures efficient detection of chromosome 11p15 epimutations in Russell-Silver syndrome.

机构信息

Program in Genetics and Genome Biology, The Hospital for Sick Children, Toronto, Ontario, Canada.

出版信息

Am J Med Genet A. 2009 Nov;149A(11):2415-23. doi: 10.1002/ajmg.a.33065.

Abstract

Over a 10-year period blood samples were collected from 57 individuals with growth restriction and RSS-like features. Our goal was to identify epigenetic abnormalities in this cohort, including uniparental disomy of chromosome 7 (UPD7), methylation changes at chromosome 11p15, as well as new epigenomic alterations. We evaluated the methylation status of 7 imprinting control regions on chromosomes 7, 11, 14, and 15. UPD7 and chromosome 7 structural abnormalities had been previously identified in five patients. Epigenetic alterations on chromosome 11p15 were identified in 11 patients. Of interest, in 3 of these 11 patients, the epigenetic alterations were limited to the H19 promoter and the distal region of its associated imprinting center, ICR1. In addition, in one patient, we detected methylation changes consistent with maternal UPD at all tested imprinted regions. This patient series suggests that epimutations on chromosome 11p15 can be most efficiently detected in RSS patients by screening for DNA methylation defects at the H19 promoter or the distal region of ICR.

摘要

在 10 年期间,从 57 名具有生长受限和 RSS 样特征的个体中采集了血液样本。我们的目标是在这个队列中识别表观遗传异常,包括 7 号染色体单亲二体性(UPD7)、11p15 染色体的甲基化变化,以及新的表观基因组改变。我们评估了染色体 7、11、14 和 15 上 7 个印迹控制区的甲基化状态。之前在 5 名患者中发现了 UPD7 和 7 号染色体结构异常。在 11 名患者中发现了 11p15 染色体的表观遗传改变。有趣的是,在这 11 名患者中的 3 名中,这些表观遗传改变仅限于 H19 启动子及其相关印迹中心 ICR1 的远端区域。此外,在一名患者中,我们在所有检测到的印迹区域检测到与母系 UPD 一致的甲基化变化。这个患者系列表明,通过筛查 H19 启动子或 ICR 的远端区域的 DNA 甲基化缺陷,在 RSS 患者中可以最有效地检测到 11p15 染色体上的 epimutations。

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