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首页> 外文期刊>Scientific reports. >Exploring DNA quality of single cells for genome analysis with simultaneous whole-genome amplification
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Exploring DNA quality of single cells for genome analysis with simultaneous whole-genome amplification

机译:探索同时进行全基因组扩增的基因组分析单细胞的DNA质量

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摘要

Single cell genome analysis methods are powerful tools to define features of single cells and to identify differences between them. Since the DNA amount of a single cell is very limited, cellular DNA usually needs to be amplified by whole-genome amplification before being subjected to further analysis. A single nucleus only contains two haploid genomes. Thus, any DNA damage that prevents amplification results in loss of damaged DNA sites and induces an amplification bias. Therefore, the assessment of single cell DNA quality is urgently required. As of today, there is no simple method to determine the quality of a single cell DNA in a manner that will still retain the entire cellular DNA for amplification and downstream analysis. Here, we describe a method for whole-genome amplification with simultaneous quality control of single cell DNA by using a competitive spike-in DNA template.
机译:单细胞基因组分析方法是定义单细胞特征并识别它们之间差异的强大工具。由于单个细胞的DNA数量非常有限,因此在进行进一步分析之前,通常需要通过全基因组扩增来扩增细胞DNA。单个核仅包含两个单倍体基因组。因此,任何阻止扩增的DNA损伤都会导致受损DNA位点的丢失,并引起扩增偏差。因此,迫切需要评估单细胞DNA的质量。到目前为止,还没有一种简单的方法来确定单个细胞DNA的质量,而该方法仍将保留整个细胞DNA进行扩增和下游分析。在这里,我们描述了一种全基因组扩增方法,同时通过使用竞争性的穗状DNA模板对单细胞DNA进行质量控制。

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