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自制酶预混物和Illumina测序技术可实现一步法吉布森组装及病毒感染性克隆的验证。

Home-made enzymatic premix and Illumina sequencing allow for one-step Gibson assembly and verification of virus infectious clones.

作者信息

Zhao Mingmin, García Beatriz, Gallo Araiz, Tzanetakis Ioannis E, Simón-Mateo Carmen, García Juan Antonio, Pasin Fabio

机构信息

Centro Nacional de Biotecnología (CNB-CSIC), 28049 Madrid, Spain.

College of Horticulture and Plant Protection, Inner Mongolia Agricultural University, Hohhot 010018, China.

出版信息

Phytopathol Res. 2020;2. doi: 10.1186/s42483-020-00077-4. Epub 2020 Dec 3.

Abstract

An unprecedented number of viruses have been discovered by leveraging advances in high-throughput sequencing. Infectious clone technology is a universal approach that facilitates the study of biology and role in disease of viruses. In recent years homology-based cloning methods such as Gibson assembly have been used to generate virus infectious clones. We detail herein the preparation of home-made cloning materials for Gibson assembly. The home-made materials were used in one-step generation of the infectious cDNA clone of a plant RNA virus into a T-DNA binary vector. The clone was verified by a single Illumina reaction and a de novo read assembly approach that required no primer walking, custom primers or reference sequences. Clone infectivity was finally confirmed by -mediated delivery to host plants. We anticipate that the convenient home-made materials, one-step cloning and Illumina verification strategies described herein will accelerate characterization of viruses and their role in disease development.

摘要

通过利用高通量测序技术的进步,已经发现了数量空前的病毒。感染性克隆技术是一种通用方法,有助于研究病毒的生物学特性及其在疾病中的作用。近年来,基于同源性的克隆方法,如吉布森组装法,已被用于生成病毒感染性克隆。我们在此详细介绍用于吉布森组装的自制克隆材料的制备。这些自制材料用于将植物RNA病毒的感染性cDNA克隆一步法构建到T-DNA二元载体中。该克隆通过单次Illumina反应和从头读取组装方法进行验证,该方法无需引物步移、定制引物或参考序列。最终通过农杆菌介导的方法将克隆导入宿主植物来确认克隆的感染性。我们预计,本文所述的便捷自制材料、一步克隆和Illumina验证策略将加速病毒特性及其在疾病发展中作用的表征。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1e94/7990137/90e839f59c54/nihms-1677486-f0001.jpg

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