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通过等温分支扩增检测稀有DNA靶点。

Detection of rare DNA targets by isothermal ramification amplification.

作者信息

Zhang D Y, Zhang W, Li X, Konomi Y

机构信息

Department of Pathology, Mount Sinai School of Medicine, New York University, New York, NY 10029, USA.

出版信息

Gene. 2001 Aug 22;274(1-2):209-16. doi: 10.1016/s0378-1119(01)00607-2.

DOI:10.1016/s0378-1119(01)00607-2
PMID:11675013
Abstract

We described previously a novel DNA amplification technique, termed ramification amplification (RAM) (Zhang et al., Gene 211 (1998) 277). This method was designed to utilize a circular probe (C-probe) that is covalently linked by a DNA ligase when it hybridizes to a target. Then, a DNA polymerase extends the bound forward primer along the C-probe and continuously displaces a downstream strand, generating a multimeric single-stranded DNA (ssDNA), analogous to in vivo 'rolling circle' replication of bacteriophage. This multimeric ssDNA then serves as a template for multiple reverse primers to hybridize, extend, and displace downstream DNA, generating a large ramified (branching) DNA complex, and resulting in an exponential amplification. Previously, we were able to achieve a significant amplification using phi29 DNA polymerase that has a high processivity and strong displacement activity. However, due to the intrinsic limitations of the polymerase, we only achieved a sensitivity of 10,000 target molecules, which is insufficient for most practical uses. Therefore, we tested several DNA polymerases and found that exo(-) Bst DNA polymerase meets the requirement for high sensitivity. By further improving the assay condition and format, we are able to detect fewer than ten targets in 1 h and to apply successfully this method for detection of Epstein-Barr virus in human lymphoma specimens.

摘要

我们之前描述了一种新型的DNA扩增技术,称为分支扩增(RAM)(Zhang等人,《基因》211(1998年)277)。该方法旨在利用一种环状探针(C-探针),当它与靶标杂交时,会通过DNA连接酶共价连接。然后,DNA聚合酶沿着C-探针延伸结合的正向引物,并持续置换下游链,产生多聚体单链DNA(ssDNA),类似于噬菌体在体内的“滚环”复制。这种多聚体ssDNA随后作为多个反向引物杂交、延伸和置换下游DNA的模板,产生一个大的分支(分叉)DNA复合物,从而实现指数扩增。之前,我们使用具有高持续合成能力和强置换活性的phi29 DNA聚合酶能够实现显著的扩增。然而,由于该聚合酶的固有局限性,我们仅达到了10000个靶标分子的灵敏度,这对于大多数实际应用来说是不够的。因此,我们测试了几种DNA聚合酶,发现exo(-) Bst DNA聚合酶符合高灵敏度的要求。通过进一步改进检测条件和形式,我们能够在1小时内检测到少于10个靶标,并成功将该方法应用于检测人类淋巴瘤标本中的爱泼斯坦-巴尔病毒。

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Detection of rare DNA targets by isothermal ramification amplification.通过等温分支扩增检测稀有DNA靶点。
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Single cell sequencing: a distinct new field.单细胞测序:一个独特的新领域。
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Quantitative analysis of zeptomole microRNAs based on isothermal ramification amplification.基于等温分支扩增的zeptomole微小RNA定量分析。
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Real-time hybridization chain reaction.
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Isothermal amplification and molecular typing of the obligate intracellular pathogen Mycobacterium leprae isolated from tissues of unknown origins.从来源不明的组织中分离出的专性胞内病原体麻风分枝杆菌的等温扩增及分子分型
J Clin Microbiol. 2006 Apr;44(4):1502-8. doi: 10.1128/JCM.44.4.1502-1508.2006.
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Use of ramification amplification assay for detection of Escherichia coli O157:H7 and other E. coli Shiga toxin-producing strains.使用分支扩增分析法检测大肠杆菌O157:H7及其他产志贺毒素大肠杆菌菌株。
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