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Merck
CN
  • Discovery of transgene insertion sites by high throughput sequencing of mate pair libraries.

Discovery of transgene insertion sites by high throughput sequencing of mate pair libraries.

BMC genomics (2014-06-03)
Anuj Srivastava, Vivek M Philip, Ian Greenstein, Lucy B Rowe, Mary Barter, Cathleen Lutz, Laura G Reinholdt
摘要

Transgenesis by random integration of a transgene into the genome of a zygote has become a reliable and powerful method for the creation of new mouse strains that express exogenous genes, including human disease genes, tissue specific reporter genes or genes that allow for tissue specific recombination. Nearly 6,500 transgenic alleles have been created by random integration in embryos over the last 30 years, but for the vast majority of these strains, the transgene insertion sites remain uncharacterized. To obtain a complete understanding of how insertion sites might contribute to phenotypic outcomes, to more cost effectively manage transgenic strains, and to fully understand mechanisms of instability in transgene expression, we've developed methodology and a scoring scheme for transgene insertion site discovery using high throughput sequencing data. Similar to other molecular approaches to transgene insertion site discovery, high-throughput sequencing of standard paired-end libraries is hindered by low signal to noise ratios. This problem is exacerbated when the transgene consists of sequences that are also present in the host genome. We've found that high throughput sequencing data from mate-pair libraries are more informative when compared to data from standard paired end libraries. We also show examples of the genomic regions that harbor transgenes, which have in common a preponderance of repetitive sequences.

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Roche
切口平移试剂盒, sufficient for 50 labeling reactions, kit of 1 (7 components), suitable for FISH
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货号包装规格是否有货价格数量
25 μL
国内现货,预计发货时间 2025年4月21日
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¥2,199.22
4 x 25 μL
国内现货,预计发货时间 2025年4月21日
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¥4,528.97