Degenerate oligonucleotide primer <scp>MIG</scp>‐seq: an effective <scp>PCR</scp>‐based method for high‐throughput genotyping-Reference-Cited by-同舟云学术

Degenerate oligonucleotide primer MIG‐seq: an effective PCR‐based method for high‐throughput genotyping

Published:2024-03-08 Issue:6 Volume:118 Page:2296-2317
ISSN:0960-7412
Container-title:The Plant Journal
language:en
Short-container-title:The Plant Journal

Author:

Nishimura Kazusa¹²^ORCID,Kokaji Hiroyuki¹,Motoki Ko¹²,Yamazaki Akira³,Nagasaka Kyoka¹,Mori Takashi¹,Takisawa Rihito⁴,Yasui Yasuo¹,Kawai Takashi²,Ushijima Koichiro²^ORCID,Yamasaki Masanori⁵,Saito Hiroki⁶,Nakano Ryohei¹,Nakazaki Tetsuya¹

Affiliation:

1. Graduate School of Agriculture Kyoto University 4‐2‐1, Shiroyamadai Kizugawa City Kyoto 619‐0218 Japan

2. Graduate School of Environmental, Life, Natural Science and Technology Okayama University 1‐1‐1 Tsushima‐naka, Kita‐ku Okayama City 700‐8530 Okayama Japan

3. Faculty of Agriculture Kindai University 3327‐204, Nakamachi Nara City Nara 631‐8505 Japan

4. Faculty of Agriculture Ryukoku University 1‐5 Yokotani, Seta Oe‐cho Otsu City Shiga 520‐2194 Japan

5. Graduate School of Science and Technology Niigata University 8050 Ikarashi 2 no‐cho, Nishi‐ku Niigata City Niigata 950‐2181 Japan

6. Tropical Agriculture Research Front, Japan International Research Center for Agricultural Sciences 1091‐1 Maezato‐Kawarabaru Ishigaki Okinawa 907‐0002 Japan

Abstract

SUMMARYNext‐generation sequencing (NGS) library construction often involves using restriction enzymes to decrease genome complexity, enabling versatile polymorphism detection in plants. However, plant leaves frequently contain impurities, such as polyphenols, necessitating DNA purification before enzymatic reactions. To overcome this problem, we developed a PCR‐based method for expeditious NGS library preparation, offering flexibility in number of detected polymorphisms. By substituting a segment of the simple sequence repeat sequence in the MIG‐seq primer set (MIG‐seq being a PCR method enabling library construction with low‐quality DNA) with degenerate oligonucleotides, we introduced variability in detectable polymorphisms across various crops. This innovation, named degenerate oligonucleotide primer MIG‐seq (dpMIG‐seq), enabled a streamlined protocol for constructing dpMIG‐seq libraries from unpurified DNA, which was implemented stably in several crop species, including fruit trees. Furthermore, dpMIG‐seq facilitated efficient lineage selection in wheat and enabled linkage map construction and quantitative trait loci analysis in tomato, rice, and soybean without necessitating DNA concentration adjustments. These findings underscore the potential of the dpMIG‐seq protocol for advancing genetic analyses across diverse plant species.

Funder

Core Research for Evolutional Science and Technology

Science and Technology Research Partnership for Sustainable Development

Japan Society for the Promotion of Science

Publisher

Wiley

Link

https://onlinelibrary.wiley.com/doi/pdf/10.1111/tpj.16708

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