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通过 SNP 微阵列筛选出的犬染色体非整倍体的鉴定。

Identification of aneuploidy in dogs screened by a SNP microarray.

机构信息

Paw Print Genetics, Genetic Veterinary Sciences, Inc, 220 E Rowan, Suite 220, Spokane, WA, 99207, USA.

Center for Reproductive Biology, Washington State University, Pullman, WA, USA.

出版信息

Hum Genet. 2021 Nov;140(11):1619-1624. doi: 10.1007/s00439-021-02318-8. Epub 2021 Jul 21.

Abstract

Microarray analysis is an efficient approach for screening and identifying cytogenetic imbalances in humans. SNP arrays, in particular, are a powerful way to identify copy-number gains and losses representing aneuploidy and aneusomy, but moreover, allow for the direct assessment of individual genotypes in known disease loci. Using these approaches, trisomies, monosomies, and mosaicism of whole chromosomes have been identified in human microarray studies. For canines, this approach is not widely used in clinical laboratory diagnostic practice. In our laboratory, we have implemented the use of a proprietary SNP array that represents approximately 650,000 loci across the domestic dog genome. During the validation of this microarray prior to clinical use, we identified three cases of aneuploidy after screening 2053 dogs of various breeds including monosomy X, trisomy X, and an apparent mosaic trisomy of canine chromosome 38 (CFA38). This study represents the first use of microarrays for copy-number evaluation to identify cytogenetic anomalies in canines. As microarray analysis becomes more routine in canine genetic testing, more cases of chromosome aneuploidy are likely to be uncovered.

摘要

微阵列分析是筛选和识别人类细胞遗传学不平衡的有效方法。SNP 微阵列,特别是,是一种识别代表非整倍体和非整倍体的拷贝数增益和损失的有力方法,但此外,还可以直接评估已知疾病基因座中的个体基因型。使用这些方法,在人类微阵列研究中已经鉴定出整个染色体的三体、单体和嵌合体。对于犬类,这种方法在临床实验室诊断实践中并未广泛使用。在我们的实验室中,我们已经实施了使用一种专有的 SNP 微阵列,该微阵列代表了大约 65 万个犬基因组中的基因座。在临床使用前对该微阵列进行验证时,我们在筛选了包括 X 单体、X 三体和犬 38 号染色体(CFA38)明显的嵌合三体在内的 2053 只不同品种的犬后,发现了三例非整倍体。本研究代表了首次使用微阵列进行拷贝数评估以识别犬科动物的细胞遗传学异常。随着微阵列分析在犬遗传检测中变得更加常规,可能会发现更多的染色体非整倍体病例。

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