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Single-Nucleotide Polymorphism Genotyping by Nanoparticle-Enhanced Surface Plasmon Resonance Imaging Measurements of Surface Ligation Reactions

机译:单核苷酸多态性基因分型的纳米粒子表面等离子体共振成像表面连接反应的测量。

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摘要

A sensitive method for the analysis of single nucleotide polymorphisms (SNPs) in genomic DNA that utilizes nanoparticle-enhanced surface plasmon resonance imaging (SPRI) measurements of surface enzymatic ligation reactions on DNA microarrays is demonstrated. SNP identification was achieved by using sequence-specific surface reactions of the enzyme Taq DNA ligase, and the presence of ligation products on the DNA microarray elements was detected using SPRI through the hybridization adsorption of complementary oligonucleotides attached to gold nanoparticles. The use of gold nanoparticles increases the sensitivity of the SPRI so that single bases in oligonucleotides can be successfully identified at a concentration of 1 pM. This sensitivity is amply sufficient for performing multiplexed SNP genotyping by using multiple PCR amplicons and should also allow for the direct detection and identification of SNP sequences from 1 pM unamplified genomic DNA samples with this array-based and label-free SPRI methodology. As a first example of SNP genotyping, three different human genomic DNA samples were screened for a possible point mutation in the BRCA1 gene that is associated with breast cancer.
机译:演示了一种灵敏的分析基因组DNA中单核苷酸多态性(SNP)的方法,该方法利用了DNA微阵列上的表面酶连接反应的纳米粒子增强的表面等离子体共振成像(SPRI)测量。通过使用Taq DNA连接酶的序列特异性表面反应来实现SNP鉴定,并使用SPRI通过吸附附着在金纳米颗粒上的互补寡核苷酸的杂交吸附来检测DNA微阵列元件上连接产物的存在。金纳米颗粒的使用提高了SPRI的灵敏度,因此寡核苷酸中的单个碱基可以成功地以1 pM的浓度被鉴定出来。这种敏感性足以通过使用多个PCR扩增子进行多重SNP基因分型,并且还应允许使用这种基于阵列和无标记的SPRI方法从1 pM未扩增基因组DNA样品中直接检测和鉴定SNP序列。作为SNP基因分型的第一个例子,针对与乳腺癌相关的BRCA1基因,筛选了三种不同的人类基因组DNA样品中可能存在的点突变。

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