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The next generation of target capture technologies - large DNA fragment enrichment and sequencing determines regional genomic variation of high complexity

机译:下一代目标捕获技术-大的DNA片段富集和测序确定了高度复杂的区域基因组变异

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Background The ability to capture and sequence large contiguous DNA fragments represents a significant advancement towards the comprehensive characterization of complex genomic regions. While emerging sequencing platforms are capable of producing several kilobases-long reads, the fragment sizes generated by current DNA target enrichment technologies remain a limiting factor, producing DNA fragments generally shorter than 1 kbp. The DNA enrichment methodology described herein, Region-Specific Extraction (RSE), produces DNA segments in excess of 20 kbp in length. Coupling this enrichment method to appropriate sequencing platforms will significantly enhance the ability to generate complete and accurate sequence characterization of any genomic region without the need for reference-based assembly. Results RSE is a long-range DNA target capture methodology that relies on the specific hybridization of short (20-25 base) oligonucleotide primers to selected sequence motifs within the DNA target region. These capture primers are then enzymatically extended on the 3’-end, incorporating biotinylated nucleotides into the DNA. Streptavidin-coated beads are subsequently used to pull-down the original, long DNA template molecules via the newly synthesized, biotinylated DNA that is bound to them. We demonstrate the accuracy, simplicity and utility of the RSE method by capturing and sequencing a 4 Mbp stretch of the major histocompatibility complex (MHC). Our results show an average depth of coverage of 164X for the entire MHC. This depth of coverage contributes significantly to a 99.94?% total coverage of the targeted region and to an accuracy that is over 99.99?%. Conclusions RSE represents a cost-effective target enrichment method capable of producing sequencing templates in excess of 20 kbp in length. The utility of our method has been proven to generate superior coverage across the MHC as compared to other commercially available methodologies, with the added advantage of producing longer sequencing templates amenable to DNA sequencing on recently developed platforms. Although our demonstration of the method does not utilize these DNA sequencing platforms directly, our results indicate that the capture of long DNA fragments produce superior coverage of the targeted region.
机译:背景技术捕获和连续的大型DNA片段的能力代表了对复杂基因组区域进行全面表征的重要进展。虽然新兴的测序平台能够产生几千个碱基长的读数,但当前的DNA靶标富集技术产生的片段大小仍然是一个限制因素,通常会产生小于1 kbp的DNA片段。本文所述的DNA富集方法学(特定区域提取(RSE))可产生长度超过20 kbp的DNA片段。将该富集方法与适当的测序平台结合,将显着增强生成任何基因组区域的完整而准确的序列表征的能力,而无需基于参考的组装。结果RSE是一种远程DNA靶捕获方法,它依赖于短(20-25个碱基)的寡核苷酸引物与DNA靶区域内选定的序列基序的特异性杂交。然后将这些捕获引物在3'端进行酶促延伸,将生物素化的核苷酸整合到DNA中。随后,用抗生蛋白链菌素包被的珠子通过结合到它们上的新合成的生物素化的DNA下拉原始的长DNA模板分子。我们通过捕获和测序主要组织相容性复合体(MHC)的4 Mbp片段来证明RSE方法的准确性,简单性和实用性。我们的结果表明,整个MHC的平均覆盖深度为164倍。这种覆盖深度极大地有助于目标区域的总覆盖率达到99.94%,并且准确性超过99.99%。结论RSE是一种经济高效的靶标富集方法,能够产生长度超过20 kbp的测序模板。与其他市售方法相比,我们方法的实用性已被证明可在整个MHC上产生出色的覆盖率,并具有在最近开发的平台上产生适合DNA测序的更长测序模板的额外优势。尽管我们对该方法的演示并未直接利用这些DNA测序平台,但我们的结果表明,长DNA片段的捕获可产生对靶区域的出色覆盖。

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