Hosono Seiyu, Faruqi A Fawad, Dean Frank B, Du Yuefen, Sun Zhenyu, Wu Xiaohong, Du Jing, Kingsmore Stephen F, Egholm Michael, Lasken Roger S
Molecular Staging, Inc., New Haven, Connecticut 06511, USA.
Genome Res. 2003 May;13(5):954-64. doi: 10.1101/gr.816903. Epub 2003 Apr 14.
Preparation of genomic DNA from clinical samples is a bottleneck in genotyping and DNA sequencing analysis and is frequently limited by the amount of specimen available. We use Multiple Displacement Amplification (MDA) to amplify the whole genome 10,000-fold directly from small amounts of whole blood, dried blood, buccal cells, cultured cells, and buffy coats specimens, generating large amounts of DNA for genetic testing. Genomic DNA was evenly amplified with complete coverage and consistent representation of all genes. All 47 loci analyzed from 44 individuals were represented in the amplified DNA at between 0.5- and 3.0-fold of the copy number in the starting genomic DNA template. A high-fidelity DNA polymerase ensures accurate representation of the DNA sequence. The amplified DNA was indistinguishable from the original genomic DNA template in 5 SNP and 10 microsatellite DNA assays on three different clinical sample types for 20 individuals. Amplification of genomic DNA directly from cells is highly reproducible, eliminates the need for DNA template purification, and allows genetic testing from small clinical samples. The low amplification bias of MDA represents a dramatic technical improvement in the ability to amplify a whole genome compared with older, PCR-based methods.
从临床样本中制备基因组DNA是基因分型和DNA测序分析的一个瓶颈,并且常常受到可用样本量的限制。我们使用多重置换扩增(MDA)技术直接从少量全血、干血、颊细胞、培养细胞和血沉棕黄层样本中对全基因组进行10000倍扩增,从而生成大量用于基因检测的DNA。基因组DNA得到了均匀扩增,所有基因均有完整覆盖且代表性一致。从44个个体中分析的所有47个基因座在扩增后的DNA中的拷贝数是起始基因组DNA模板中拷贝数的0.5至3.0倍。一种高保真DNA聚合酶确保了DNA序列的准确呈现。在针对20个个体的三种不同临床样本类型进行的5个单核苷酸多态性(SNP)和10个微卫星DNA检测中,扩增后的DNA与原始基因组DNA模板无法区分。直接从细胞中扩增基因组DNA具有高度可重复性,无需进行DNA模板纯化,并且能够对少量临床样本进行基因检测。与基于聚合酶链反应(PCR)的旧方法相比,MDA的低扩增偏差代表了在全基因组扩增能力方面的一项重大技术进步。
