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Gapfilled nuclear genome assemblies of black-tailed dusky antechinus (Antechinus arktos), silver-headed antechinus (Antechinus argentus), and black-tailed dasyure (Murexia melanurus)

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NIAID Data Ecosystem2026-03-12 收录
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https://zenodo.org/record/3735685
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Paired-end (100 bp) DNA libraries were sequenced by BGI (Hong Kong) using a BGISEQ-500 instrument to generate ~30× genome coverage. Raw data (mean 948,503,285±3,100,231 reads) was filtered using Flexbar v3.4.0 [1,2] (to remove adapters and low-quality reads) with default settings. Paired-end sequence reads from whole-genome sequencing of the three dasyurid species to the repeat-masked reference genome assemblies of the dasyurids yellow-footed antechinus [Antechinus flavipes; assembly AdamAnt) and Tasmanian devil (Sarcophilus harrisii; assembly Devil_ref v7.0, also known as sarHar1 [3])].  Please see https://github.com/sciseim/semelparity for associated scripts.  References 1    Roehr, J. T., Dieterich, C. & Reinert, K. Flexbar 3.0 - SIMD and multicore parallelization. Bioinformatics 33, 2941-2942, doi:10.1093/bioinformatics/btx330 (2017). 2    Dodt, M., Roehr, J. T., Ahmed, R. & Dieterich, C. FLEXBAR-Flexible Barcode and Adapter Processing for Next-Generation Sequencing Platforms. Biology (Basel) 1, 895-905, doi:10.3390/biology1030895 (2012). 3    Murchison, E. P. et al. Genome sequencing and analysis of the Tasmanian devil and its transmissible cancer. Cell 148, 780-791, doi:10.1016/j.cell.2011.11.065 (2012).
创建时间:
2021-05-25
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