Transcriptional factor MdESE3 controls fruit acidity by activating genes regulating malic acid content in apple

Author:

Zheng Litong1,Ma Wenfang12ORCID,Liu Peipei1,Song Shujie1,Wang Liang1,Yang Wei1,Ren Hang1,Wei Xiaoyu1ORCID,Zhu Lingcheng1ORCID,Peng Jiaqing2,Ma Fengwang1ORCID,Li Mingjun1ORCID,Ma Baiquan1ORCID

Affiliation:

1. State Key Laboratory for Crop Stress Resistance and High-Efficiency Production/Shaanxi Key Laboratory of Apple, College of Horticulture, Northwest A&F University , Yangling 712100, Shaanxi , China

2. Institute of Economic Crop Research, Shiyan Academy of Agricultural Sciences , Shiyan 442714, Hubei , China

Abstract

Abstract Acidity is a key factor controlling fruit flavor and quality. In a previous study, combined transcriptome and methylation analyses identified a P3A-type ATPase from apple (Malus domestica), MdMa11, which regulates vacuolar pH when expressed in Nicotiana benthamiana leaves. In this study, the role of MdMa11 in controlling fruit acidity was verified in apple calli, fruits, and plantlets. In addition, we isolated an APETALA2 domain-containing transcription factor, designated MdESE3, based on yeast one-hybrid (Y1H) screening using the MdMa11 promoter as bait. A subcellular localization assay indicated that MdESE3 localized to the nucleus. Analyses of transgenic apple calli, fruits, and plantlets, as well as tomatoes, demonstrated that MdESE3 enhances fruit acidity and organic acid accumulation. Meanwhile, chromatin immunoprecipitation quantitative PCR, luciferase (LUC) transactivation assays, and GUS reporter assays indicated that MdESE3 could bind to the ethylene-responsive element (ERE; 5ʹ-TTTAAAAT-3ʹ) upstream of the MdMa11 transcription start site, thereby activating its expression. Furthermore, MdtDT, MdDTC2, and MdMDH12 expression increased in apple fruits and plantlets overexpressing MdESE3 and decreased in apple fruits and plantlets where MdESE3 was silenced. The ERE was found in MdtDT and MdMDH12 promoters, but not in the MdDTC2 promoter. The Y1H, LUC transactivation assays, and GUS reporter assays indicated that MdESE3 could bind to the MdtDT and MdMDH12 promoters and activate their expression. Our findings provide valuable functional validation of MdESE3 and its role in the transcriptional regulation of MdMa11, MdtDT, and MdMDH12 and malic acid accumulation in apple.

Funder

National Natural Science Foundation of China

Program for National Key Research and Development

China Postdoctoral Science Foundation

Shaanxi Postdoctoral Research Funding Project

Fundamental Research Funds for the Central Universities

Publisher

Oxford University Press (OUP)

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