Comparative genomics of the medicinal plants Lonicera macranthoides and L. japonica provides insight into genus genome evolution and hederagenin‐based saponin biosynthesis

Author:

Yin Xiaojian12ORCID,Xiang Yaping1,Huang Feng‐Qing1,Chen Yahui1,Ding Hengwu3,Du Jinfa1,Chen Xiaojie1,Wang Xiaoxiao1,Wei Xinru1,Cai Yuan‐Yuan1,Gao Wen1,Guo Dongshu4,Alolga Raphael N.1,Kan Xianzhao3,Zhang Baolong4,Alejo‐Jacuinde Gerardo5,Li Ping1,Tran Lam‐Son Phan5,Herrera‐Estrella Luis56,Lu Xu1ORCID,Qi Lian‐Wen1

Affiliation:

1. Clinical Metabolomics Center, School of Traditional Chinese Pharmacy China Pharmaceutical University Nanjing China

2. Key Laboratory of Soybean Molecular Design Breeding Northeast Institute of Geography and Agroecology, Chinese Academy of Sciences Changchun China

3. The Institute of Bioinformatics, College of Life Sciences Anhui Normal University Wuhu China

4. Provincial Key Laboratory of Agrobiology Jiangsu Academy of Agricultural Science Nanjing China

5. Institute of Genomics for Crop Abiotic Stress Tolerance, Department of Plant and Soil Science, Texas Tech University Lubbock TX USA

6. Laboratorio Nacional de Genomica/ Unidad de Genómica Avanzada del Centro de Investigación y de Estudios Avanzados del IPN Irapuato Mexico

Abstract

SummaryLonicera macranthoides (LM) and L. japonica (LJ) are medicinal plants widely used in treating viral diseases, such as COVID‐19. Although the two species are morphologically similar, their secondary metabolite profiles are significantly different. Here, metabolomics analysis showed that LM contained ~86.01 mg/g hederagenin‐based saponins, 2000‐fold higher than LJ. To gain molecular insights into its secondary metabolite production, a chromosome‐level genome of LM was constructed, comprising 9 pseudo‐chromosomes with 40 097 protein‐encoding genes. Genome evolution analysis showed that LM and LJ were diverged 1.30–2.27 million years ago (MYA). The two plant species experienced a common whole‐genome duplication event that occurred ∼53.9–55.2 MYA before speciation. Genes involved in hederagenin‐based saponin biosynthesis were arranged in clusters on the chromosomes of LM and they were more highly expressed in LM than in LJ. Among them, oleanolic acid synthase (OAS) and UDP‐glycosyltransferase 73 (UGT73) families were much more highly expressed in LM than in LJ. Specifically, LmOAS1 was identified to effectively catalyse the C‐28 oxidation of β‐Amyrin to form oleanolic acid, the precursor of hederagenin‐based saponin. LmUGT73P1 was identified to catalyse cauloside A to produce α‐hederin. We further identified the key amino acid residues of LmOAS1 and LmUGT73P1 for their enzymatic activities. Additionally, comparing with collinear genes in LJ, LmOAS1 and LmUGT73P1 had an interesting phenomenon of ‘neighbourhood replication’ in LM genome. Collectively, the genomic resource and candidate genes reported here set the foundation to fully reveal the genome evolution of the Lonicera genus and hederagenin‐based saponin biosynthetic pathway.

Funder

National Natural Science Foundation of China

Publisher

Wiley

Subject

Plant Science,Agronomy and Crop Science,Biotechnology

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