Gel purification of gDNA for next-generation sequencing applications

Author:

Utthiya Supanut1,Wonnapinij Passorn123ORCID,Napaumpaiporn Pondpan1,Kittiwongwattana Chokchai4ORCID,Sakulkoo Jenjira1,Suttangkakul Anongpat123ORCID,Vuttipongchaikij Supachai123ORCID

Affiliation:

1. Department of Genetics, Faculty of Science, Kasetsart University, Bangkok, 10900, Thailand

2. Center of Advanced studies for Tropical Natural Resources, Kasetsart University, Bangkok, 10900, Thailand

3. Omics Center for Agriculture, Bioresources, Food & Health, Kasetsart University (OmiKU), Bangkok, 10900, Thailand

4. Department of Biology, Faculty of Science, King Mongkut's Institute of Technology Ladkrabang, Bangkok, 10520, Thailand

Abstract

We demonstrate that gDNA can be conveniently and efficiently isolated and purified using standard agarose gel electrophoresis, band excision and gel purification. This method yields a substantial amount at microgram levels of gDNA per gel cleanup with high purity. An RNase A treatment step can be omitted. The quality of gDNA is suitable for next-generation sequencing, resulting in >10 Mb reads and high-quality read data (Phred score >28 up to 100 of 150 base reads). Furthermore, the gDNA can be kept intact in a gel slice for several days. This method has been tested for dictyostelids, bacteria and plants.

Funder

Faculty of Science, Kasetsart University

The Thailand Science Research and Innovation through the Kasetsart University Reinventing University Program 2021

Kasetsart University Research and Development Institute

National Research Council of Thailand

Publisher

Future Science Ltd

Subject

General Biochemistry, Genetics and Molecular Biology,Biotechnology

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