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通过循环连接和切割(CycLiC)直接在微阵列捕获模板上进行测序。

Sequencing by Cyclic Ligation and Cleavage (CycLiC) directly on a microarray captured template.

作者信息

Mir Kalim U, Qi Hong, Salata Oleg, Scozzafava Giuseppe

机构信息

The Wellcome Trust Centre for Human Genetics, Oxford University, Oxford, UK.

出版信息

Nucleic Acids Res. 2009 Jan;37(1):e5. doi: 10.1093/nar/gkn906. Epub 2008 Nov 16.

Abstract

Next generation sequencing methods that can be applied to both the resequencing of whole genomes and to the selective resequencing of specific parts of genomes are needed. We describe (i) a massively scalable biochemistry, Cyclical Ligation and Cleavage (CycLiC) for contiguous base sequencing and (ii) apply it directly to a template captured on a microarray. CycLiC uses four color-coded DNA/RNA chimeric oligonucleotide libraries (OL) to extend a primer, a base at a time, along a template. The cycles comprise the steps: (i) ligation of OLs, (ii) identification of extended base by label detection, and (iii) cleavage to remove label/terminator and undetermined bases. For proof-of-principle, we show that the method conforms to design and that we can read contiguous bases of sequence correctly from a template captured by hybridization from solution to a microarray probe. The method is amenable to massive scale-up, miniaturization and automation. Implementation on a microarray format offers the potential for both selection and sequencing of a large number of genomic regions on a single platform. Because the method uses commonly available reagents it can be developed further by a community of users.

摘要

需要能够应用于全基因组重测序以及基因组特定部分选择性重测序的下一代测序方法。我们描述了(i)一种用于连续碱基测序的大规模可扩展生物化学方法——循环连接与切割(CycLiC),以及(ii)将其直接应用于微阵列上捕获的模板。CycLiC使用四个颜色编码的DNA/RNA嵌合寡核苷酸文库(OL),每次沿着模板延伸一个碱基来延伸引物。这些循环包括以下步骤:(i)OL的连接,(ii)通过标记检测识别延伸的碱基,以及(iii)切割以去除标记/终止子和未确定的碱基。为了进行原理验证,我们表明该方法符合设计要求,并且我们能够从通过溶液与微阵列探针杂交捕获的模板中正确读取连续的碱基序列。该方法适合大规模扩大、小型化和自动化。在微阵列形式上的实施为在单个平台上对大量基因组区域进行选择和测序提供了潜力。由于该方法使用常见的试剂,用户群体可以进一步开发它。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6bf3/2615607/a79f209effb6/gkn906f1.jpg

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