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논문 기본 정보

자료유형
학술저널
저자정보
Cao Zhengyan (Chongqing University of Arts and Sciences China) Wu Peiyin (Chongqing University of Arts and Sciences China) Gao Hongmei (Chongqing University of Arts and Sciences China) Xia Ning (Chongqing University of Arts and Sciences China) Jiang Ying (Chongqing University of Arts and Sciences China) Tang Ning (Chongqing University of Arts and Sciences China) Liu Guohua (Chongqing University of Arts and Sciences China) Chen Zexiong (Chongqing University of Arts and Sciences China)
저널정보
한국유전학회 Genes & Genomics Genes & Genomics Vol.44 No.2
발행연도
2022.2
수록면
219 - 235 (17page)
DOI
10.1007/s13258-021-01118-8

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Background Lonicera macranthoides is an important woody plant with high medicinal values widely cultivated in southern China. WRKY, one of the largest transcription factor families, participates in plant development, senescence, and stress responses. However, a comprehensive study of the WRKY family in L. macranthoides hasn’t been reported previously. Objective To establish an extensive overview of the WRKY family in L. macranthoides and identify senescence-responsive members of LmWRKYs. Methods RNA-Seq and phylogenetic analysis were employed to identify the LmWRKYs and their evolutionary relationships. Quantitative real-time (qRT-PCR) and transgenic technology was utilized to investigate the roles of LmWRKYs in response to developmental-, cold-, and ethylene-induced senescence. Results A total of 61 LmWRKY genes with a highly conserved motif WRKYGQK were identified. Phylogenetic analysis of LmWRKYs together with their orthologs from Arabidopsis classified them into three groups, with the number of 15, 39, and 7, respectively. 17 LmWRKYs were identified to be differentially expressed between young and aging leaves by RNA-Seq. Further qRT-PCR analysis showed 15 and 5 LmWRKY genes were significantly induced responding to tissue senescence in leaves and stems, respectively. What’s more, five LmWRKYs, including LmWRKY4, LmWRKY5, LmWRKY6, LmWRKY11, and LmWRKY16 were dramatically upregulated under cold and ethylene treatment in both leaves and stems, indicating their involvements commonly in developmental- and stress-induced senescence. In addition, function analysis revealed LmWRKY16, a homolog of AtWRKY75, can accelerate plant senescence, as evidenced by leaf yellowing during reproductive growth in LmWRKY16-overexpressing tobaccos. Conclusion The results lay the foundation for molecular characterization of LmWRKYs in plant senescence.

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