DeepSeq, School of Life Sciences, Queens Medical Centre, University of Nottingham, Nottingham, UK.
Nat Biotechnol. 2021 Apr;39(4):442-450. doi: 10.1038/s41587-020-00746-x. Epub 2020 Nov 30.
Nanopore sequencers can be used to selectively sequence certain DNA molecules in a pool by reversing the voltage across individual nanopores to reject specific sequences, enabling enrichment and depletion to address biological questions. Previously, we achieved this using dynamic time warping to map the signal to a reference genome, but the method required substantial computational resources and did not scale to gigabase-sized references. Here we overcome this limitation by using graphical processing unit (GPU) base-calling. We show enrichment of specific chromosomes from the human genome and of low-abundance organisms in mixed populations without a priori knowledge of sample composition. Finally, we enrich targeted panels comprising 25,600 exons from 10,000 human genes and 717 genes implicated in cancer, identifying PML-RARA fusions in the NB4 cell line in <15 h sequencing. These methods can be used to efficiently screen any target panel of genes without specialized sample preparation using any computer and a suitable GPU. Our toolkit, readfish, is available at https://www.github.com/looselab/readfish .
纳米孔测序仪可以通过反转单个纳米孔的电压来选择性地对池中的某些 DNA 分子进行测序,从而富集和去除特定的序列,以解决生物学问题。以前,我们使用动态时间扭曲将信号映射到参考基因组来实现这一点,但该方法需要大量的计算资源,并且无法扩展到吉字节大小的参考基因组。在这里,我们通过使用图形处理单元 (GPU) 碱基调用克服了这一限制。我们展示了从人类基因组中特定染色体和混合群体中低丰度生物的富集,而无需事先了解样本组成。最后,我们富集了包含 10000 个人类基因和 717 个与癌症相关基因的 25600 个外显子的靶向面板,在不到 15 小时的测序中鉴定了 NB4 细胞系中的 PML-RARA 融合。这些方法可以在不使用特殊样品制备的情况下,使用任何计算机和合适的 GPU 来有效地筛选任何目标基因面板。我们的工具包 readfish 可在 https://www.github.com/looselab/readfish 获得。
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