平衡读取长度和测序深度:优化单子片的纳米孔长读测序,重点是百合

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Applied Bio Materials Pub Date : 2023-06-06 DOI:10.1002/aps3.11524
Gisel Y. De La Cerda, Jacob B. Landis, Evan Eifler, Adriana I. Hernandez, Fay-Wei Li, Jing Zhang, Carrie M. Tribble, Nisa Karimi, Patricia Chan, Thomas Givnish, Susan R. Strickler, Chelsea D. Specht
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引用次数: 2

摘要

我们提出了用于为百合产生长读的纳米孔测序读取的方法,并演示了对标准协议的修改如何直接影响读取长度和总输出。目标是帮助那些对生成长读测序数据感兴趣的人确定哪些步骤可能是优化输出和结果所必需的。方法对百合科四种花椒属植物进行测序。对十二烷基硫酸钠(SDS)的提取和清理方案进行了修改,包括用臼和杵研磨,使用切割或宽孔尖端,氯仿清洗,头清洗,去除短片段,以及使用高度纯化的DNA。结果:最大化读取长度的步骤可能会降低总体输出。值得注意的是,流动池中的孔数与总体输出相关,但我们没有看到孔数与读取长度或产生的读取数之间的关联。许多因素促成了纳米孔测序运行的总体成功。我们展示了对DNA提取和清洗步骤的一些修改对总测序输出、读取大小和生成的读取数量的直接影响。我们展示了读取长度和读取数之间的权衡,在较小程度上,总测序输出,所有这些都是成功的从头基因组组装的重要因素。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

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Balancing read length and sequencing depth: Optimizing Nanopore long-read sequencing for monocots with an emphasis on the Liliales

Premise

We present approaches used to generate long-read Nanopore sequencing reads for the Liliales and demonstrate how modifications to standard protocols directly impact read length and total output. The goal is to help those interested in generating long-read sequencing data determine which steps may be necessary for optimizing output and results.

Methods

Four species of Calochortus (Liliaceae) were sequenced. Modifications made to sodium dodecyl sulfate (SDS) extractions and cleanup protocols included grinding with a mortar and pestle, using cut or wide-bore tips, chloroform cleaning, bead cleaning, eliminating short fragments, and using highly purified DNA.

Results

Steps taken to maximize read length can decrease overall output. Notably, the number of pores in a flow cell is correlated with the overall output, yet we did not see an association between the pore number and the read length or the number of reads produced.

Discussion

Many factors contribute to the overall success of a Nanopore sequencing run. We showed the direct impact that several modifications to the DNA extraction and cleaning steps have on the total sequencing output, read size, and number of reads generated. We show a tradeoff between read length and the number of reads and, to a lesser extent, the total sequencing output, all of which are important factors for successful de novo genome assembly.

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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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