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首页> 外文期刊>Electrophoresis: The Official Journal of the International Electrophoresis Society >A novel competitive fluorescent multiplex STR polymorphism assay for rapid, reliable and single-tube screening of 22q11.2 copy-number aberrations.
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A novel competitive fluorescent multiplex STR polymorphism assay for rapid, reliable and single-tube screening of 22q11.2 copy-number aberrations.

机译:一种新颖的竞争性荧光多重STR多态性测定法,用于快速,可靠和单管筛查22q11.2拷贝数像差。

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摘要

Copy-number aberrations of the 22q11.2 region can lead to varied resulting and complex phenotypes. Routine screening for these common constitutional chromosomal abnormalities requires powerful tools. A competitive fluorescent multiplex STR polymorphism assay (CFMSA) was built for detecting these aberrations. With the introduction of an internal reference and distinguishable STR polymorphism markers, this competitive fluorescent multiplex STR polymorphism assay provides complementary information about polymorphism and gene dosage in one tube simultaneously, thereby enhancing the assay sensitivity. It was first tested in 110 normal controls, and was proven to have highly polymorphic and reliable gene dosage information. Then, 476 subjects with congenital heart defect were screened according to the testing strategy of the American Heart Association, and 17 deletions and 1 duplication of 22q11.2 were correctly identified. It is expected that this assay will serve as a cost-effective alternative to existingassays for routine, large-scale screening in all at-risk individuals with either deletion or duplication in 22q11.2.
机译:22q11.2区域的拷贝数畸变可能导致不同的结果表型和复杂的表型。对这些常见的体质染色体异常进行常规筛查需要强大的工具。建立了竞争性荧光多重STR多态性分析(CFMSA)来检测这些像差。通过引入内部参考和可区分的STR多态性标记,这种竞争性荧光多重STR多态性测定可同时在一个试管中提供有关多态性和基因剂量的补充信息,从而提高了测定灵敏度。它首先在110个正常对照中进行了测试,并被证明具有高度多态性和可靠的基因剂量信息。然后,根据美国心脏协会的检测策略,筛查了476名先天性心脏缺陷患者,正确识别出22q11.2的17个缺失和1个重复。预期该方法将替代现有方法,在22q11.2中缺失或重复的所有高风险个体中进行常规,大规模筛查,是一种具有成本效益的替代方法。

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