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AluScan: a method for genome-wide scanning of sequence and structure variations in the human genome

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机构: [1]Capital Med Univ, Dept Neurosurg, Beijing Tiantan Hosp, Beijing 100050, Peoples R China; [2]Hong Kong Univ Sci & Technol, Div Life Sci, Kowloon, Hong Kong, Peoples R China; [3]Hong Kong Univ Sci & Technol, Appl Genom Ctr, Brain Canc Genome Consortium Hong Kong, Kowloon, Hong Kong, Peoples R China; [4]Beijing Genome Inst Shenzhen, Chinese Canc Genome Consortium, Shenzhen 518083, Peoples R China; [5]Queen Elizabeth Hosp, Dept Neurosurg, Kowloon, Hong Kong, Peoples R China; [6]Chinese Univ Hong Kong, Dept Surg, Prince Wales Hosp, Div Neurosurg, Sha Tin, Hong Kong, Peoples R China; [7]Univ Hong Kong, Queen Mary Hosp, Li Ka Shing Fac Med, Div Neurosurg,Dept Surg, Hong Kong, Hong Kong, Peoples R China; [8]Chinese Univ Hong Kong, Prince Wales Hosp, Dept Anat & Cellular Pathol, Sha Tin, Hong Kong, Peoples R China; [9]Capital Med Univ, Dept Neurosurg, Beijing Tiantan Hosp, 6 Tiantan Xili, Beijing 100050, Peoples R China
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Background: To complement next-generation sequencing technologies, there is a pressing need for efficient pre-sequencing capture methods with reduced costs and DNA requirement. The Alu family of short interspersed nucleotide elements is the most abundant type of transposable elements in the human genome and a recognized source of genome instability. With over one million Alu elements distributed throughout the genome, they are well positioned to facilitate genome-wide sequence amplification and capture of regions likely to harbor genetic variation hotspots of biological relevance. Results: Here we report on the use of inter-Alu PCR with an enhanced range of amplicons in conjunction with next-generation sequencing to generate an Alu-anchored scan, or 'AluScan', of DNA sequences between Alu transposons, where Alu consensus sequence-based 'H-type' PCR primers that elongate outward from the head of an Alu element are combined with 'T-type' primers elongating from the poly-A containing tail to achieve huge amplicon range. To illustrate the method, glioma DNA was compared with white blood cell control DNA of the same patient by means of AluScan. The over 10 Mb sequences obtained, derived from more than 8,000 genes spread over all the chromosomes, revealed a highly reproducible capture of genomic sequences enriched in genic sequences and cancer candidate gene regions. Requiring only sub-micrograms of sample DNA, the power of AluScan as a discovery tool for genetic variations was demonstrated by the identification of 357 instances of loss of heterozygosity, 341 somatic indels, 274 somatic SNVs, and seven potential somatic SNV hotspots between control and glioma DNA. Conclusions: AluScan, implemented with just a small number of H-type and T-type inter-Alu PCR primers, provides an effective capture of a diversity of genome-wide sequences for analysis. The method, by enabling an examination of gene-enriched regions containing exons, introns, and intergenic sequences with modest capture and sequencing costs, computation workload and DNA sample requirement is particularly well suited for accelerating the discovery of somatic mutations, as well as analysis of disease-predisposing germline polymorphisms, by making possible the comparative genome-wide scanning of DNA sequences from large human cohorts.

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出版当年[2010]版:
大类 | 2 区 生物
小类 | 2 区 生物工程与应用微生物 3 区 遗传学
最新[2023]版:
大类 | 2 区 生物学
小类 | 2 区 生物工程与应用微生物 2 区 遗传学
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出版当年[2009]版:
Q1 BIOTECHNOLOGY & APPLIED MICROBIOLOGY Q2 GENETICS & HEREDITY
最新[2023]版:
Q2 GENETICS & HEREDITY Q2 BIOTECHNOLOGY & APPLIED MICROBIOLOGY

影响因子: 最新[2023版] 最新五年平均 出版当年[2009版] 出版当年五年平均 出版前一年[2008版] 出版后一年[2010版]

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第一作者机构: [2]Hong Kong Univ Sci & Technol, Div Life Sci, Kowloon, Hong Kong, Peoples R China;
通讯作者:
通讯机构: [1]Capital Med Univ, Dept Neurosurg, Beijing Tiantan Hosp, Beijing 100050, Peoples R China; [4]Beijing Genome Inst Shenzhen, Chinese Canc Genome Consortium, Shenzhen 518083, Peoples R China; [9]Capital Med Univ, Dept Neurosurg, Beijing Tiantan Hosp, 6 Tiantan Xili, Beijing 100050, Peoples R China
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