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Gene Coexpression Networks Reveal Key Drivers of Flavonoid Variation in Eleven Tea Cultivars (Camellia sinensis) Chao Zheng, Jian-Qiang Ma, Jie-Dan Chen, Chun-Lei Ma, Wei Chen, Ming-Zhe Yao, and Liang Chen J. Agric. Food Chem., Just Accepted Manuscript • DOI: 10.1021/acs.jafc.9b04422 • Publication Date (Web): 12 Aug 2019 Downloaded from pubs.acs.org on August 13, 2019

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Journal of Agricultural and Food Chemistry

Gene Coexpression Networks Reveal Key Drivers of Flavonoid Variation in Eleven Tea Cultivars (Camellia sinensis) Chao Zheng, Jian-Qiang Ma, Jie-Dan Chen, Chun-Lei Ma, Wei Chen, Ming-Zhe Yao*, Liang Chen* Key Laboratory of Tea Biology and Resources Utilization, Ministry of Agriculture and Rural Affairs, Tea Research Institute of the Chinese Academy of Agricultural Sciences, Hangzhou, China * Correspondence: Liang Chen, [email protected]; Ming-Zhe Yao, [email protected] Tel: +86 571 86652835, Fax: +86 571 86653866

Chao Zheng: [email protected]; Jian-Qiang Ma: [email protected]; Jie-Dan Chen: [email protected] Chun-Lei Ma: [email protected]; Wei Chen: [email protected].

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Abstract

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Following the recent completion of the draft genome sequence of the tea plant, high-throughput

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decoding of gene function, especially for those involved in complex secondary metabolism pathways

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has become a major challenge. Here, we profiled the metabolome and transcriptome of eleven tea

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cultivars, and then illustrated a weighted gene coexpression network analysis (WGCNA) based system

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biology strategy to interpret metabolomic flux, predict gene functions, and mining key regulators

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involved in the flavonoid biosynthesis pathway. We constructed a multilayered regulatory network,

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which integrated gene coexpression relationship with the microRNA target and promoter cis-

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regulatory element information. This allowed revealing new uncharacterized TFs (e.g., MADSs,

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WRKYs, and SBPs) and microRNAs (including 17 conserved and 15 novel microRNAs) that

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potentially implicate in different steps of the catechin biosynthesis. Furthermore, we applied

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metabolic-signature-based association method to capture additional key regulators involved in

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catechin pathway. This provides important clues for the functional characterization of five SCPL1A

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acyltransferase family members, which might implicate in the production balance of anthocyanins,

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galloylated catechins, and proanthocyanins. Application of ‘omics’-based system biology strategy

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should facilitate germplasm utilization and provide valuable resources for tea quality improvement.

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KEYWORDS: Camellia sinensis, catechin biosynthesis, metabolomic flux, weighted gene

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coexpression network (WGCNA), widely targeted metabolomics, functional genomics

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Introduction

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Plants including tea are genetically very diverse groups and present numerous types of species,

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cultivars, genotypes and accessions, occurring worldwide. The food industry is currently searching for

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new functional foods and nutraceuticals to help meet the demand presented by the consumers of natural,

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immunity-boosting and health-promoting plant-based food products.1-2 Tea plant (Camellia sinensis

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(L.) O. Kuntze), an important beverage crop, produces numerous characteristic components such as

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theanine, caffeine, and catechins that are estimated to have various beneficial effects.3 Recently, several

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special albino (e.g., ‘Anji Baicha’ and ‘Huangjinya’) and purple-leaf (e.g., ‘Zijuan’ and ‘Sunrouge’)

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tea cultivars have been discovered and developed in many tea-growing countries.4-5 In comparison to

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green-leaf tea cultivars, the concentration of anthocyanins is significantly higher in the new shoots of

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purple-leaf tea cultivars;4 while the albino tea cultivars accumulate a higher quantity of amino acids

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and lower levels of caffeine and catechins in their new shoots.5 The change in the intricate balance of

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these secondary metabolites will greatly influence the flavor of tea. However, the characterization of

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genes involved in the production of these secondary metabolites is still lagging behind, which

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constitutes a major obstacle for metabolic engineering in tea plants. Most recently, one of the greatest

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achievements of tea plant biology is the completion of the draft genome sequence, which will greatly

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facilitate understanding of tea metabolite pathways and accelerate tea breeding progress.6-7 In tea

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plants, most of the genes were functionally annotated based on sequence similarity analysis against

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the known genes in public databases, with a few of them has been validated with direct experimental

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evidence. Currently, the functional elucidation of unknown genes in tea plants, especially those

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involved in secondary metabolism, is therefore, a critical challenge. Based on the sequence annotation

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of the C. sinensis genome, a substantial number of genes are assigned to large enzyme families,

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including 22 SCPL1A acyltransferases genes, 30 terpene synthase genes, 148 ABC protein genes, 226

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cytochrome P450 genes, and 267 glycosyltransferase genes, which are thought to play vital roles in

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the transport, degradation, synthesis, and modification of particular metabolites in tea plants. 7

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Although extensive efforts have been made to reveal the molecular mechanism of the production of

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three major characteristic secondary metabolites (i.e., flavonoids, caffeine, and theanine) in tea plants

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for germplasm selection and tea quality improvement, the function of the great majority of genes

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involved in these pathways remains to be determined.8-14 Thus, a high-throughput functional genomics

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analysis pipeline is essential.

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Weighted gene coexpression network analysis (WGCNA) is a highly robust method for classifying

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genes via hierarchical clustering of gene coexpression network (GCN).15 GCNs are particularly useful

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for analyzing high-dimensionality expression datasets as they provide an intuitive framework for

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describing changes in expression driven by cellular processes acting within or across multiple

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conditions.15 Consequently, WGCNA is now commonly employed to analyze whole transcriptome,

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proteomic, and metabolomic data to identify coexpression modules that relate either to a trait or

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condition of interest.15-16 In our previous study, we used WGCNA to investigate the potential signaling

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interactions between light quality and other environmental cues (e.g., low temperature, drought, and

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blister blight disease) in tea plants.9 We revealed the molecular events that triggered by blue and green

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light might partly overlap with stress responses, which suggest the possibility of a targeted use of blue

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and green light to induce defense responses in tea plants. The WGCNA can also be extended to

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investigate the gene modules that responsible for the variation of metabolites. Xu et al. (2018) profiled

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metabolome and transcriptome of the tea leaves harvested in different seasons, and by using WGCNA

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based integration strategy, key metabolite–specific modules and regulators involved in monoterpenes

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and sesquiterpenes were successfully delimited.17 MicroRNA (miRNA) target and promoter cis-

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regulatory element (CRE) information can be easily integrated into plant GCNs. This strategy has been

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employed to comprehensively identify target genes of the entire R2R3-MYB family in grape.18

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Enrichment for miRNA targets within GCNs has demonstrated a vital role of four classes of miRNA–

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transcription factor (TF) pairs in regulating terpenoid biosynthesis in tea plants.19 Thus, aggregating

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genome-wide coexpression network and several regulatory networks into a community network can

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be advantageous to provide supportive evidence and effectively reveal discrepancies between

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individual networks.

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To date, challenges in tea plant biology are lack of information on the complicated genetic

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background of various cultivars, and the transformation system has not yet been established. The

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integration of transcriptome and metabolome profiles can provide clues for the characterization of

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functions of key metabolic genes and regulators in tea plants. Here, we employed the WGCNA based

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system biology strategy for dissecting the complexity of 11 excellent tea cultivars’ secondary metabolic

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variation. Special emphasis was placed on the practical application of the bait genes- and metabolites-

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guide coexpression networks to interpret metabolomic flux, predict gene functions, and mining key

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regulators involved in the catechin biosynthesis pathway.

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Materials and Methods

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Plant Materials

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Several studies have shown that there is considerable variability in metabolite composition underlying

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the leaf-color mutations in tea plants.4-5 To obtain a highly informative (variable) dataset for WGCNA

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analysis, we selected 11 tea cultivars with different shoot colors for transcriptome and metabolome

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analysis. This should facilitate the implementation of network construction and module detection, as

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well as module-metabolite association analysis. All tea cultivars (ten-year-old) used in this study were

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grown at the China National Germplasm Tea Repository (Hangzhou, Zhejiang, China; latitude: 30.27°

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N, longitude: 120.13° E). The cultivars ‘Fuding Dabaicha’ (GA), ‘TRI15’ (GB), ‘Longjing 43’ (GC),

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‘Longjing Ziya’ (PA), ‘Liercha’ (PB), ‘Zijuan’ (PC), ‘Jingning Baicha’ (WA), ‘Anji Baicha’ (WB),

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‘Huaye’ (YA), ‘Huangjinya’ (YB), and ‘Zhonghuang 3’ (YC) belongs to Camellia sinensis (Figure 1).

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For each cultivar, first-flush young shoots (two leaves and a bud) in the spring were harvested from 30

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individuals for metabolomics (three biological replications * five individuals for each replicate) and

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transcriptomics (three biological replications * five individuals for each replicate) studies.

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Metabolite Profiling and Statistical Analysis

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The freeze-dried leaf sample was crushed using a mixer mill (MM 400, Retsch) for 1.5 min at 30 Hz

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before extraction, 100 mg dried powder was extracted with 1.0 ml pure methanol spiked with 0.1 mg/L

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lidocaine. Following centrifugation at 10000 g for 10 min, the lipid-solubility extracts were absorbed

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and 0.4 ml of each extract was mixed and filtrated before LC–MS analysis. The quality control samples

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(i.e., a mix of all samples) were injected at regular intervals (every ten samples) throughout the

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analytical run to provide a set of data from which repeatability could be assessed. By comparing the

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retention time, m/z values, and the fragmentation patterns with the standards, 462 metabolites were

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identified (Figure S1). For the metabolites for which no commercial standards are available, peaks in

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the MS2T library were used to query the by comparing the MS/MS spectral data with literature

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references and online metabolite databases (METLIN, HMDB, KNApSAcK, MoTo DB and

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MassBank). Relative quantification was achieved by normalization of integrated extracted ion

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chromatograms (XICs) using LC–ESI–MS/MS system (HPLC, Shim-pack UFLC SHIMADZU

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CBM20A system; MS, Applied Biosystems 4000 Q-TRAP) by a large-scale multiple-reaction

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monitoring (MRM) on a triple quadrupole (QQQ) MS (Figure S2).9,

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detection window of 80 s and a target scan time of 1.5 s, the quadrupole filters the precursor ions

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(parent ions) of the target substance and excludes the ions corresponding to other molecular weights

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to prevent interference. After obtaining metabolite data from the different samples, the peak area of

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the mass spectra of all substances was integrated using MultiQuant (v2.0) software (AB SCIEX). Row-

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wise normalization was performed by the quality control sample, and data were log2-transformed and

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auto-scaled to reduce any systematic bias within metabolite data. Principal component analysis (PCA)

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and sparse Independent PCA (sIPCA) were implemented in R. The intra-cultivar Euclidean distances

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(EDs) were calculated by the average of ED crosswise replicate samples within each cultivar, and inter-

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cultivar EDs were calculated by first computing the average of replicates for each cultivar and then

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computing the average ED of remaining cultivars calculated with this cultivar.

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RNA-Seq and Data Processing

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The total RNA was isolated using the RNeasy plant mini kit (Tiangen Bio, Beijing, China) according

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to the manufacturer’s instructions. The cDNA libraries were sequenced on an Illumina HiSeq Xten

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platform (Illumina, San Diego, CA, USA) to produce 150 bp paired-end reads at Novogene (Novogene,

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Beijing, China). The raw reads were submitted to the BIGD (BIG Data Center, http://bigd.big.ac.cn/)

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In the MRM mode with

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under the accession number PRJCA001447. Low-quality reads and adapters were filtered and trimmed

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using Trimmomatic (v0.36). High-quality clean reads were then mapped to the C. sinensis genome

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(http://tpia.teaplant.org/) using HISAT2 (v.2.1.0)21 and were counted using HTseq (v.0.6.1p1).22 TMM

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normalization method was used to calculate gene expression in Bioconductor edgeR package.23 Gene

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Ontology (GO) enrichment analysis of the differentially expressed genes (DEGs) was performed using

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the GOseq R packages (v1.32.0).24

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Gene and Metabolite Coexpression Network Construction

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Weighted gene coexpression network analysis (WGCNA) was implemented using the WGCNA R

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package (v1.63).15 Network construction and module detection were performed by ‘blockwiseModules’

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function with adjusted parameters for transcriptome and metabolome datasets, which allows automatic

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and unsupervised network construction for the input data. For transcriptome dataset, ‘minModuleSize’

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= 30, ‘minKMEtoStay’ = 0.7, ‘mergeCutHeight’ = 0.05, and ‘minCoreKME’ = 0.8 were applied to

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construct a ‘signed’ weighted correlation network, while ‘minModuleSize’ = 10, ‘minKMEtoStay’ =

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0.6, ‘mergeCutHeight’ = 0.05, and ‘minCoreKME’= 0.7 were chosen for the analysis of metabolomic

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datasets. The pattern of gene expression and metabolite level in a given module was summarized using

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modules eigengene and eigenmetabolite values, respectively, which represent the first principal

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component of the scaled data for genes/metabolites in each module.15 The module membership (kME)

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was then calculated to assess the gene connectivity based on Pearson correlation. The module networks

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were visualized using Cytoscape (v3.7.1).25

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Quantitative Real-Time PCR (qRT-PCR) Validation

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The qRT-PCR analysis was carried out using SYBR Premix Ex Taq II kit (Takara, Japan) with a

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LightCycler 480 Real-Time PCR system (Roche Applied Science) according to the manufacturer’s

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instructions. Three biological replicates were performed for each cultivar, and GAPDH was used as an

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endogenous control. The relative transcript abundance was calculated using the 2−ΔΔCT method.26

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Primers used are shown in Table S1.

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MicroRNA Target and Transcription Factor Binding Sites Prediction

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Conserved and novel tea plant miRNAs were collected from our previous study.14 The psRNATarget

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and psRobot were used to determine whether genes involved in the catechin biosynthesis pathway are

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regulated by miRNAs.27-28 The intersection of psRNATarget and psRobot outputs was selected to

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reduce the false-positive rate. Potential TF binding sites in the promoter region (1 kbp upstream from

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the transcription start site) of the entire genome were identified using the TFBSTools R package and

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JASPAR database (http://jaspar.genereg.net).29-30

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Orthogonality of Regulatory Network

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To compare ‘guilt-by-association’ based GCN with known functional networks of Arabidopsis

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thaliana, structure or TF genes involved in the catechin pathway were subjected to BLASTX searching

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against the Arabidopsis protein (TAIR, Version 11, http://www.arabidopsis.org) with a cutoff E-value

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of 10-5. We then downloaded multiple Arabidopsis functional annotation networks from STRING v11

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(http://string-db.org) database and compared whether edges based on expression similarity were found

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in any known functional network.

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Results and Discussion

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Highly Variable Metabolic Profiles of Eleven Tea Cultivars

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To explore metabolic differences existing in 11 tea cultivars, we used a widely targeted metabolomic

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approach to quantify the metabolite levels in tea leaves in a high-throughput manner. Of the 776

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metabolites detected in tea leaves, 462 were identified by using authentic standards, while 314 were

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putatively annotated by comparing the MS/MS spectral data with literature references and online

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metabolite databases (Table S2). We then calculated the intra- and inter-cultivar EDs to measure the

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“metabolic distance” within and among cultivars using the complete normalized metabolic dataset of

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each sample pair (Figure 2B). As shown in the scatterplot, two purple-leaf cultivars, PB (EDintracultivar

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= 46.3) and PC (EDintracultivar = 46.8) showed highest inter-cultivar variations among the cultivars, while

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replicate samples exhibited relatively low intra-cultivar variations (EDintracultivar = 17.3–24.1). In

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addition, we employed PCA to investigate the variance structure of metabolic composition in an

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unsupervised way (Figure 2A). The first (PC1) and the second (PC2) principal components explained

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19% and 14% of the metabolite variation, respectively. In agreement with the results of ED analysis,

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we observed a large variation exist in the relative metabolic profiles between PB/PC and other cultivars

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analyzed.

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To gain a better clustering and to investigate major differential metabolites of these cultivars, we

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employed a sparse version of Independent PCA (sIPCA), which performs an internal variable selection

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and combines the advantages of both PCA and Independent Component Analysis (ICA) on metabolic

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data (Figure 2C). Several important flavonoids (e.g., delphinidin 3-O-rutinoside, (+)-gallocatechin

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(GC), cyanidin 3-O-glucosyl-malonylglucoside, chrysoeriol O-rhamnosyl-O-glucuronic acid,

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myricetin, and fustin) were identified as key metabolites responsible for cultivar discrimination based

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on sIPCA (Figure 2D). Notably, the accumulation level of two anthocyanins (i.e., cyanidin 3-O-

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glucosyl-malonylglucoside and delphinidin 3-O-rutinoside) in PB and PC was much lower than other

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cultivars (Figure 2D and Table S2). However, the total amount of anthocyanins in PA, PB and PC were

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significantly higher than other tea cultivars, which is consistent with previous studies showing that

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anthocyanin overproduction is responsible for the purple coloration in tea plants (Table S2).13, 31-32 In

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addition, it has been suggested that the main coloration components in the leaves of ‘Zijuan’ were

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delphinidin-3-O-galactoside and cyanidin-3-O-galactoside.32 In another study, delphinidin-3-O-

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coumaroylglucoside and cyanidin-3-O-coumaroylgalactoside were identified as the two most

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abundant anthocyanins in ‘Mooma1’, which may responsible for the bright red coloration of new

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shoots in this novel purple-leaf tea variety.13 Consistent with these studies, we observed that

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anthocyanins in different purple-leaf cultivars might be modified by different anthocyanin

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acyltransferases (ATs) and anthocyanidin 3-O-glycosyltransferases (UGTs) to give differently colored

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anthocyanins (e.g., peonidin and pelargonidin) (Figure S3 and Table S2). Thus, the understanding of

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the modification processes to produce those anthocyanins would help us to elucidate the complex

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metabolic flux within the anthocyanidin pathways.

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To reveal metabolic modules and possible metabolic flux responsible for the biosynthesis of

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secondary metabolites in tea plants, we employed WGCNA on the metabolomic dataset. As shown in

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Figure 3A, the WGCNA allowed identification of 19 metabolic modules. Obvious precursor-product

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relationships were recognized within several modules, such as amino acid and its derivatives (MM11),

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and nucleotide derivates and glycerophospholipids (MM12, MM17, and MM18) (Table S2). By

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calculating the correlation efficiency between eigenmetabolite networks, we found that the

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eigenmetabolites of MM1 were negatively correlated with MM7 (r = -0.95, P = 4 × 10-17) (Figure 3B,

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C, D). In MM1, a number of flavone glycosides (e.g., 6-C-hexosyl-luteolin O-hexoside, selgin 5-O-

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hexoside, C-hexosyl-isorhamnetin O-hexoside, apigenin C-glucoside, and luteolin 3',7-di-O-glucoside)

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and metabolites that located in the downstream flavonoid biosynthesis pathway such as

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proanthocyanidins (e.g., procyanidin A1/A2), anthocyanins (e.g., delphinidin and cyanidin), and

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catechin derivatives (e.g., catechin trimer) showed a significant lower production level in PB (Figure

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3C, E and Table S2). On the other hand, PB accumulated a higher level of flavonols (e.g., kaempferol

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3,7-dirhamnoside, isorhamnetin, quercetin 7-O-malonylhexosyl-hexoside, isorhamnetin O-acetyl-

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hexoside, quercetin O-acetylhexoside, and kaempferol 3-O-rhamnoside) and flavones (e.g., velutin,

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acacetin, and apigenin 4-O-rhamnoside) than other cultivars (MM7; Figure 3D, F and Table S2).

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Metabolites in these two modules are mostly derived from the flavonoid biosynthetic pathway, and the

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competition between these metabolites for the same substrates has also been reported.31, 33 For example,

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the concentration of proanthocyanins could be greatly improved by redirecting anthocyanidins flux

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into the proanthocyanin pathway and direct repression of isoflavone biosynthesis pathway.33

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Furthermore, the significantly higher accumulation level of anthocyanin in the new shoot of purple-

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leaf cultivar ‘Zijuan’ was proposed due to direct repression of biosynthesis of lignin.31 These results

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indicated that the WGCNA protocol can be modified to construct weighted metabolic networks for

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meaningful pathway inferring and biological interpretation. Together, information on the varietal

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differences in the accumulation levels of these characteristic secondary metabolites (e.g., flavonols,

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catechins, and anthocyanins), provides valuable insights to further investigate the sensory qualities and

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nutritional values of tea plants.

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Multilevel Regulation of Catechin Biosynthesis

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As an example of the so-called ‘guilt-by-association’ principle, genes that display similar expression

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pattern across different cultivars have an increased likelihood of being within the same metabolic

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pathway or biological process, as well as under the control of a shared regulatory mechanism. To

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understand the coexpression relationships between genes at a systems level, we performed WGCNA

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on the transcriptome dataset. This unbiased and unsupervised analysis identified 279 distinct

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coexpression modules corresponding to clusters of correlated transcripts (Figure S4 and Table S3).

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Flavonoids such as catechins, anthocyanins, and flavonols are important determinant of tea quality and

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flavor.3 Some of them (e.g., delphinidin 3-O-rutinoside, (+)-gallocatechin (GC), cyanidin 3-O-

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glucosyl-malonylglucoside, myricetin, and fustin) were identified as key metabolites responsible for

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cultivar discrimination (Figure 2D). Characterizing genes involved in the regulation of these

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metabolites is crucial for improving tea quality. Taking catechin pathway as an example, we selected

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74 known genes encoding 15 enzymes involved in catechin biosynthesis as ‘bait-genes’ or ‘guide-

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genes’ to construct a GCN based on the results of WGCNA (Figure 4 and Table S4). Keeping in mind

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that GCN constructed based on the ‘guilt-by-association’ principle is by nature different from the

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physical interactions.34 We then questioned to which extent WGCNA based GCN would provide

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orthogonal and new information compared to existing functional genomic networks. We, therefore,

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compared GCN to the genetic and physical interaction networks of Arabidopsis thaliana that stored in

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the STRING database. We found that WGCNA based GCN could provide highly orthogonal

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information (Figure S5). The maximum overlap in gene interaction was 11%, which was obtained by

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combining all evidences in the STRING database (Figure S5). The accuracy of RNA-seq results and

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coexpression relationships was further verified by qRT-PCR (Figure S6).

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Since miRNA and TF have been known to play a critical role in the regulation of flavonoid

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biosynthesis.7, 10 We therefore also integrated promoter CRE and miRNA target information into GCN.

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Our results reveal a much more complex regulatory network (including 45 enzyme genes, 155 TFs, 17

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conserved and 15 novel miRNAs) for catechin biosynthesis (Figure 4 and Table S4). Promoters of a

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considerable number of enzyme-coding genes (e.g., CHSs, PALs, DFRs, and SCPLs) were enriched

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for CREs such as those for MADS, MYB, NAC, AP2/ERF, bZIP, WRKY, SBP, and bHLH TF binding

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(Figure 4 and Table S4). In particular, the MYB binding motif was present in most of the early

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biosynthesis genes (e.g., C4H, PAL, CHS, CHI, and F3H,) and late biosynthesis genes (e.g., ANS, LAR,

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DFR, and SCPL1A) in the catechin pathway. The potential regulation of these genes by MYB and

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bHLH TFs is supported by the coexpression analysis and several recent studies in tea plants.32, 35-36 For

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example, MYB4 and MYB308 are known to function as transcriptional repressors of C4H, 4CL, LAR,

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CHS and ANR to mediate anthocyanin biosynthesis in A. thaliana, tobacco, and tea plant.32, 36-37

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Ectopic expression of these repressors could result in the loss of flowers pigmentation in tobacco due

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to the decrease of anthocyanin levels.37 In our study, MYB4 (TEA032503.1) and MYB308

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(TEA033191.1)) were shown a higher expression level in PC and coexpressed with PAL

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(TEA003137.1, TEA023243.1, and TEA024587.1), ANS (TEA010322.1), F3H (TEA023790.1), and

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LAR (TEA027582.1) (Figure 4 and Table S4). Hence, these MYB repressors were likely to mediate a

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transcriptional feedback inhibition to prevent the deleterious effects of anthocyanin overproduction on

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photosynthesis and other biological processed in PC. GL3 (TEA008168.1; GM131), a bHLH TF that

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isolated from the ‘Zijuan’ (PC), was coexpressed with CHI (TEA034003.1; GM131), CHS

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(TEA034042.1; GM131) and DFR (TEA032730.1; GM131). In addition, GL3 displayed a higher

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expression level in three purple (PA, PB, and PC) cultivars, suggesting its potential role in the

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regulation of anthocyanin accumulation (Figure 4 and Table S4). This hypothesis is supported by a

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recent study in ‘Zijuan’, demonstrating that GL3 might interact with CsAN1 (MYB TF) and CsTTG1

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(WD repeat protein, WDR) to form the MYB-bHLH-WDR (MBW) transcriptional activation complex,

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thus promoting the accumulation of anthocyanin.32

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To date, the transcriptional control of flavonoid biosynthesis by MYB and bHLH TFs is well

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described in many plant species; however, little is known about the role of other TFs in the regulation

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of flavonoid accumulation.38 The GCN we generated is novel in suggesting the potential regulatory

280

roles by those TF families such as AP2/ERF, SBP, and MADS in catechin biosynthesis (Figure 4 and

281

Table S4). For instance, the presence of MADS CREs in DFRs and PALs coincided with the

282

coregulation of MADS TFs (e.g., TT16, SEP3, and AP3) to these genes. Among them, TT16 has been

283

reported to play a vital role in transcriptional regulation of proanthocyanin biosynthesis.39 Interestingly,

284

we observed a strong coregulation of several TF genes (e.g., 1 bHLH, 3 MYB, 2 NAC, 7 AP2/ERF,

285

and 6 WRKY), to C4H (TEA016772.1); however, no corresponding binding site of NAC, AP2/ERF,

286

and WRKY was found in the promoter region (Figure 4 and Table S4). This might be due to the fact

287

that several TFs, such as NAC, SPL, and WRKY could regulate the flavonoid biosynthesis through

288

interaction with the MBW complex.38 Therefore, cis-regulatory element-driven networks that

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integrated gene coexpression relationship with promoter CRE structure information are powerful tools

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for interfering new uncharacterized regulators that involved in the catechin biosynthesis pathway.

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Recently, scientific endeavors are directed toward understanding the posttranscriptional regulation

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of the flavonoid pathway involving miRNAs.10, 14, 40-41 In the current study, 51 out of 200 catechin

293

biosynthesis-related genes/TFs were potentially targeted by 17 conserved and 15 novel miRNAs in tea

294

plants (Figure 4 and Table S4). Several of conserved miRNA (e.g., miR156, miR172, and miR858)

295

identified in the coexpression network have known to play a pivotal role in flavonoid biosynthesis

296

regulation.40-41 For example, miR858 has been demonstrated to act as a negative regulator to control

297

the anthocyanin accumulation in tomato.41 miRNA156-SPL9 pair influences anthocyanin

298

accumulation by destabilizing MBW complex and/or targeting C4H in Arabidopsis.40 Thus, the

299

enrichment of miRNA targets within GCN indicated an important role of these molecules and revealed

300

an additional layer of control of the expression of "switch" genes involved in the catechin biosynthesis.

301

Finally, our high-confidence GCN can be advantageous to effectively reveal a set of potential key

302

regulators of catechin biosynthesis by aggregating different kinds of regulatory information into a

303

community network.

304

305

Metabolic-Signature-Based Association Captures Additional Key Regulators Involved in the

306

Catechin Pathway

307

Since the prediction of gene function by ‘guilt-by-association’ principle is based on the coregulation

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of a set of genes in the same biological process or pathway, only coregulated genes can be predicted

309

by this approach. However, genes involved in the same biological process or pathway are not

310

necessarily coexpressed when regulation occurs at posttranscriptional (e.g., miRNA and lncRNA

311

regulation) or posttranslational (e.g., ubiquitination and phosphorylation) levels, and some key

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regulators cannot be captured by this approach.34 Thus, we employed metabolic-signature-based

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association method to capture additional key regulators involved in the catechin pathway.

314

To analyze the catechin pathway in more detail, error plots of metabolites within the pathway were

315

generated, and MAD scores were calculated to directly compare the variation level across samples

316

(Figure 5A, B). Our previous study demonstrated that albino cultivars (i.e., ‘Anji Baicha’, ‘Baijiguan’,

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and ‘Huangjinya’) contained higher amounts of amino acids and relatively low levels of GC and EGCG

318

compared to the green-leaf tea cultivars (i.e., ‘Fuding Dabaicha’ and ‘Longjing 43’).4 In accordance

319

with this result, we observed that galloylated catechins had a lower abundance in albino tea cultivars

320

(e.g., WA and WB) than in most green- or purple-leaf tea cultivars, hence green tea processed from the

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albino tea cultivars taste more refreshing and less bitter. We then related 279 modules to 776

322

metabolites using eigengene network methodology. Among them, 37 out of 279 coexpression modules

323

showed catechins biosynthesis-related expression values (r > 0.75, P < 10-3), that is, these modules

324

probably represent core gene networks operating in each catalysis and modification reaction (Figure

325

5C, D). Genes functioning in “protein/nucleotide binding”, “carbohydrate derivative/heterocyclic

326

compound/organic

327

“catalytic/transmembrane transporter activity” were observed to be responsible for most metabolites’

328

concentration variations in catechin pathway (Figure 6A). Genes participating in “chromosome

329

organization/protein localization”, “stress/hormone response”, “macromolecule modification”, “signal

330

transduction”, and “transport” altered catechin biosynthesis and modification most frequently (Figure

331

6B). The GO term association analysis reveals a close association of catechin biosynthesis, signaling,

332

and various abiotic/biotic stress responses, suggesting that catechins might play a pivotal role in plant-

cyclic

compound

binding”,

“hydrolase/transferase

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and

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environment interactions, in agreement with previous studies indicating antioxidant and antiinsect

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activities of these important flavan-3-ol products.8, 42

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Galloylated catechins (ECG and EGCG) are characteristic astringent taste compounds and comprise

336

up to 80% (ranged from 81.2 to 88.9%) of total catechins in tea leaves, and therefore have a large

337

impact on tea quality (Table S2). Epicatechin:1-O-galloyl-β-D-glucose O-galloyltransferase (ECGT),

338

an enzyme that belongs to subclade 1A of SCPL acyltransferase has been proposed to play vital roles

339

in galloylation of catechins.7 Comparative genomic analysis revealed a total of 22 SCPL1A genes in

340

the tea plant genome, and most of them (15) were arose from tandem duplications.7 The duplication of

341

these genes could largely promote the neo- and sub-functionalization to generate new enzymatic

342

activities and drive the evolution of plant metabolic complexity. Thus, additional efforts are necessary

343

to precisely identify whether some or all of these SCPL1A genes are involved in catechin galloylation

344

in tea plants.

345

Four modules (GM111, GM124, GM74, and GM264) are comprised of genes that are significantly

346

correlated the variation of CG, ECG, GCG, and EGCG (r > 0.75, P < 10-3; Figure 5C, D). In GM74,

347

an SCPL1A acyltransferase gene (TEA016463.1) was coexpressed with two WDR genes

348

(TEA026107.1 and TEA032249.1) (Figure 6C and Table S3). Proteins containing WDRs are known

349

to act as a docking platform to interact with MYB and bHLH TFs in regulating the anthocyanin and

350

proanthocyanidin biosynthesis in tea plants, thus highlighting WDRs as a possible key regulator of the

351

production of galloylated catechins.38, 43 Notably, many of the coexpressed genes, such as DFL1

352

(auxin), IAA16 (auxin), STE1 (brassinosteroid), ACS2 (ethylene), GID1C (gibberellin), and RLK

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(salicylic acid), are involved in hormone metabolism and signaling (Figure 6C and Table S3).44 These

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results are consistent with several lines of evidence of crosstalk between hormones and flavonoids in

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the control of various facets of plant developmental processes.45

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In GM124, two SCPL1A acyltransferases (i.e., TEA034027.1 and TEA034034.1) were coexpressed

357

with several key positive regulators of flavonoids biosynthesis such as WDR protein (BUB3.2) and

358

bHLH TF (MYC2) (Figure 6D and Table S3). These regulators may not only be related to anthocyanin

359

or flavonol biosynthesis but also to stressor/stimuli such as MYC2.46 In addition, several stress

360

response genes (e.g., HOS1, GRP7, and PIP1B) and protein kinases (e.g., MPK9, dyrk2, and CRCK2)

361

were found to highly coexpressed with these regulators (Figure 6D and Table S3). Various

362

environmental stress signals, such as low temperature, high light, and UV irradiation could result in

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oxidative stress and lead to flavonoid overproduction through the regulation expression of R2R3-MYBs

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and bHLHs, as well as the activity of MBW complexes.8-9, 38 The activity of MBW complexes can be

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regulated through various posttranslational modifications (e.g., ubiquitination and phosphorylation).38,

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47-48

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PAP1 and PAP2, and thus result in the repression of anthocyanin in Arabidopsis.48 In addition, TTG1

368

(WDR family) and TT8 (bHLH042) are also likely to be degraded by the E3 ubiquitin ligase, which

369

has not yet been identified.47 The E3 ubiquitin ligase HOS1 acts as cold signaling attenuator to

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compromise the harmful effect of extreme cold responses by targeting ICE1 for proteasome

371

degradation.49 It is probable, therefore, that HOS1 (TEA015363.1) could trigger negative regulatory

372

feedback of catechin overproduction by control the expression of bHLH (MYC2, TEA009193.1) and

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WDR (BUB3.2, TEA004851.1) genes.

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For example, COP1/SPA E3 ubiquitin ligase could mediate the degradation of the MYB proteins

To date, a number of metabolic quantitative trait locus (QTL) studies have been conducted in tea

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plants to identify QTL affecting the production of characteristic secondary metabolites (e.g.,

376

theobromine, caffeine, and catechins).12, 50-51 Integration of QTL confidence intervals/markers with

377

expression based functional networks are therefore useful and needed to narrow the pool of candidates

378

and interpret the QTL results. HOS15 (TEA014884.1, GM160), another crucial repressor of cold

379

tolerance induced genes, was found to negatively correlated with the accumulation of dihydroquercetin

380

(precursor of catechins) (Table S3).52 Notably, HOS15 has also been identified as a putative QLT

381

related to catechin production in a recent study.51 Therefore, these repressors might play a key role in

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the crosstalk between cold signaling and anthocyanin/catechin metabolic pathways.

383

Of particular interest is the identification of another two modules (GM77 and GM201) that comprise

384

SCPL1A (TEA010715.1 and TEA027270.1) were negatively correlated to the production of cyanidin

385

(Figure 5C and Table S3). Key regulators involved in the anthocyanin biosynthesis pathway, such as

386

genes encoding MYB75, WDR proteins (DWA1 and AT3G49400) and anthocyanin regulatory C1

387

protein, were found to coexpress with several glycosyltransferase (e.g., UGT92A1 and UGT80B1) and

388

acyltransferase (e.g., PEL3, GNA1, and SCPL1A) genes in these two modules (Figure 6E, F and Table

389

S3). In addition, we observed an inverse accumulation pattern exists between catechins (e.g., GCG,

390

and EGCG) and cyanidin in PB (Figure 5B). Therefore, we propose that anthocyanidins are either

391

reduced to generate catechins by anthocyanidin reductase (ANR) or immediately modified by those

392

glycosyltransferases and acyltransferases to produce anthocyanins in PB (Figure S3). Furthermore, an

393

inverse accumulation pattern was also observed between catechins and proanthocyanins (PAs, e.g.,

394

procyanidin A1/A2) in PB (Figure 5B). Catechins such as (-)-epicatechin and (+)-catechin are the

395

monomers and extension units of PAs. Therefore, the galloylation of catechins by SCPL1A may lead

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to the repression of the PAs biosynthesis. Together, we proposed that at least five SCPL1A

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acyltransferase family members (TEA016463.1, TEA034027.1, TEA034034.1, TEA010715.1, and

398

TEA027270.1) could implicate in the production balance of anthocyanins, galloylated catechins, and

399

proanthocyanins in tea plants.

400

Here, we shown an ‘omics’-based data integration approaches to facilitate the identification of

401

functions of unknown metabolic genes and regulators in tea plants. These results will bring new tools

402

and valuable resources to understand how to improve and modify tea quality. Furthermore, additional

403

efforts are required to further account for features such as chromatin structure, TF combinations, and

404

protein-protein interactions by Chip-seq and ATAC-seq.

405 406

Abbreviations Used

407

GA, ‘Fuding Dabaicha’; GB, ‘TRI15’; GC, ‘Longjing 43’; PA, ‘Longjing Ziya’; PB, ‘Liercha’; PC,

408

‘Zijuan’; WA, ‘Jingning Baicha’; WB, ‘Anji Baicha’; YA, ‘Huaye’; YB, ‘Huangjinya’; YC,

409

‘Zhonghuang 3’; TF, transcription factor; miRNA, microRNA; CRE, cis-regulatory element; GO,

410

Gene Ontology; ED, Euclidean distance; MAD, Median absolute deviation; qRT-PCR, quantitative

411

real-time PCR; WGCNA, weighted gene coexpression network analysis; GCN, gene coexpression

412

network; PCA, principal component analysis; sIPCA, sparse Independent PCA; C, catechin; GC,

413

gallocatechin; EC, epicatechin; EGC, epigallocatechin; CG, catechin gallate; ECG, epicatechin gallate;

414

GCG, gallocatechin gallate; EGCG, epigallocatechin gallate; PAs, proanthocyanidins

415 416

Funding

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This work was supported by the Ministry of Agriculture of China through the Earmarked Fund for

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China Agriculture Research System (CARS-019), and the Chinese Academy of Agricultural Sciences

419

through the Agricultural Science and Technology Innovation Program (CAAS-ASTIP-2017-

420

TRICAAS) to Liang Chen.

421 422

Supporting Information

423

Figure S1. Representative MS/MS spectra for metabolites identification.

424

Figure S2. Extracted ion chromatograms (XICs) for detection of multimodal maps.

425

Figure S3. Relative accumulation levels of anthocyanins across 11 tea cultivars. Variations in relative

426

accumulation levels of anthocyanins (Z-score, scale shown in the right) are indicated in color, where

427

red regions indicate higher accumulation level, and blue regions indicate lower accumulation.

428

Figure S4. Hierarchical clustering dendrogram showing gene coexpression modules identified using

429

WGCNA. Modules correspond to branches and are labeled by colors as indicated by the first color

430

band underneath the tree. Remaining color bands reveal highly correlated (red) or anti-correlated (blue)

431

genes for the particular cultivar.

432

Figure S5. Orthogonality of ‘guilt-by-association’ principle-based gene coexpression network to other

433

molecular data in the STRING database.

434

Figure S6. qRT-PCR validation of the RNA-seq results and coexpression relationships.

435

Table S1. Primers used for the qPCR assay.

436

Table S2. WGCNA results of metabolomic dataset and analysis the levels of catechin, anthocyanins,

437

and procyanidins across samples.

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Table S3. WGCNA results of transcriptome dataset.

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Table S4. Gene coexpression relationship, miRNA target and promoter cis-regulatory element

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information of integrated network for catechin regulation in tea plants.

441 442

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TRANSPARENT TESTA16 locus encodes the ARABIDOPSIS BSISTER MADS domain protein and

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is required for proper development and pigmentation of the seed coat. Plant Cell 2002, 14 (10), 2463-

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79.

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(40)Xing, S.; Salinas, M.; Hohmann, S.; Berndtgen, R.; Huijser, P., miR156-targeted and nontargeted

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SBP-box transcription factors act in concert to secure male fertility in Arabidopsis. Plant Cell 2010,

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22 (12), 3935-50.

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(41)Jia, X.; Shen, J.; Liu, H.; Li, F.; Ding, N.; Gao, C.; Pattanaik, S.; Patra, B.; Li, R.; Yuan, L., Small

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tandem target mimic-mediated blockage of microRNA858 induces anthocyanin accumulation in

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tomato. Planta 2015, 242 (1), 283-93.

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(42)War, A. R.; Paulraj, M. G.; Ahmad, T.; Buhroo, A. A.; Hussain, B.; Ignacimuthu, S.; Sharma, H.

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C., Mechanisms of plant defense against insect herbivores. Plant signaling & behavior 2012, 7 (10),

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1306-20.

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(43)Liu, Y.; Hou, H.; Jiang, X.; Wang, P.; Dai, X.; Chen, W.; Gao, L.; Xia, T., A WD40 Repeat Protein

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from Camellia sinensis Regulates Anthocyanin and Proanthocyanidin Accumulation through the

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Formation of MYB-bHLH-WD40 Ternary Complexes. Int. J. Mol. Sci. 2018, 19 (6).

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(44)Ohri, P.; Bhardwaj, R.; Bali, S.; Kaur, R.; Jasrotia, S.; Khajuria, A.; Parihar, R. D., The common

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molecular players in plant hormone crosstalk and signaling. Curr Protein Pept Sci 2015, 16 (5), 369-

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(45)Falcone Ferreyra, M. L.; Rius, S. P.; Casati, P., Flavonoids: biosynthesis, biological functions, and

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biotechnological applications. Front Plant Sci 2012, 3, 222.

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(46)Abe, H.; Urao, T.; Ito, T.; Seki, M.; Shinozaki, K.; Yamaguchi-Shinozaki, K., Arabidopsis

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AtMYC2 (bHLH) and AtMYB2 (MYB) function as transcriptional activators in abscisic acid signaling.

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Plant Cell 2003, 15 (1), 63-78.

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(47)Patra, B.; Pattanaik, S.; Yuan, L., Proteolytic degradation of the flavonoid regulators,

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TRANSPARENT TESTA8 and TRANSPARENT TESTA GLABRA1, in Arabidopsis is mediated by

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the ubiquitin/26Sproteasome system. Plant signaling & behavior 2013, 8 (10), doi: 10 4161/psb 25901.

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(48)Maier, A.; Schrader, A.; Kokkelink, L.; Falke, C.; Welter, B.; Iniesto, E.; Rubio, V.; Uhrig, J. F.;

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Hulskamp, M.; Hoecker, U., Light and the E3 ubiquitin ligase COP1/SPA control the protein stability

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of the MYB transcription factors PAP1 and PAP2 involved in anthocyanin accumulation in Arabidopsis.

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Plant J. 2013, 74 (4), 638-51.

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a SSR-based genetic map and identification of QTLs for catechins content in tea plant (Camellia

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sinensis). PLoS One 2014, 9 (3), e93131.

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(51)Koech, R. K.; Malebe, P. M.; Nyarukowa, C.; Mose, R.; Kamunya, S. M.; Joubert, F.; Apostolides,

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Z., Functional annotation of putative QTL associated with black tea quality and drought tolerance traits.

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(52)Park, J.; Lim, C. J.; Shen, M.; Park, H. J.; Cha, J. Y.; Iniesto, E.; Rubio, V.; Mengiste, T.; Zhu, J.

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K.; Bressan, R. A.; Lee, S. Y.; Lee, B. H.; Jin, J. B.; Pardo, J. M.; Kim, W. Y.; Yun, D. J., Epigenetic

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switch from repressive to permissive chromatin in response to cold stress. Proc. Natl. Acad. Sci. U. S.

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A. 2018, 115 (23), E5400-E5409.

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Figure Captions

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Figure 1. Leaf phenotypes of 11 tea cultivars. ‘Fuding Dabaicha’ (GA); ‘TRI15’ (GB); ‘Longjing 43’

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(GC); ‘Longjing Ziya’ (PA); ‘Liercha’ (PB); ‘Zijuan’ (PC); ‘Huaye’ (YA); ‘Huangjinya’ (YB);

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‘Zhonghuang 3’ (YC); ‘Jingning Baicha’ (WA); ‘Anji Baicha’ (WB).

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Figure 2. Metabolic distance and variation between cultivars. (A) Principal component analysis (PCA)

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and (C) sparse Independent PCA (sIPCA) sample representation using the first two components. (B)

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Scatterplot of intra- and inter-cultivar Euclidean distances (EDs) using the complete normalized

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metabolic profiles of a sample pair. (D) Heatmap of normalized accumulation level for the top 30

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metabolites that were selected based on ranked sIPCA loading values.

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Figure 3. Metabolite coexpression network analysis. (A) Hierarchical clustering dendrogram showing

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metabolite coexpression modules identified using WGCNA. Modules correspond to branches and are

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labeled by colors as indicated by the first color band underneath the tree. Remaining color bands reveal

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highly correlated (red) or anti-correlated (blue) metabolites for the particular cultivar. (B) Correlation

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analysis of module eigenmetabolite that summarizes the modules identified in the clustering analysis.

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Blue color represents the negative correlation, while red represents the positive correlation.

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Eigenmetabolite accumulation for the (C) MM1 and (D) MM7. Bar plots present module

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eigenmetabolite values. Error bars represent the standard errors among three biological replicates for

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each cultivar. Heatmap of normalized accumulation level for top 20 metabolites in (E) MM1 and (F)

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MM7 that were selected based on the WGCNA measure of intramodular gene connectivity (kME).

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Figure 4. An integrated network for catechin regulation in the tea plant. Octagon, circle, and triangle

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nodes represent enzyme-coding genes, transcription factors (TFs), and microRNAs (miRNAs),

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respectively. Coexpression relationships between different TF family members (colored solid circles)

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and enzyme-coding genes are depicted by corresponding colored edges. Dashed red lines with arrows

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depict predicted miRNA-gene interaction. Pie chart colors represent the presence of selected TF-

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binding sites in promoter regions (1kbp upstream from the transcription start site) of the corresponding

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enzyme-coding genes.

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Figure 5. The variation of metabolite levels and module gene expression involved in the catechin

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pathway. (A) Biosynthetic pathway of the principal catechins. CHS, CHI, F3H, F3′H, F3′5′H, DFR,

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ANS, LAR, ANR, and SCPL1A represent chalcone synthase, chalcone isomerase, flavanone 3-

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hydroxylase, flavonoid 3′-hydroxylase, flavonoid 3′,5′-hydroxylase, dihydroflavonol 4-reductase,

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anthocyanidin synthase, leucoanthocyanidin reductase, anthocyanidin reductase, and type 1A serine

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carboxypeptidase-like acyltransferases, respectively. (B) The relative intensity of metabolites in the

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catechin pathway. Mean expression values of metabolite intensities with their standard error bars from

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three biological replicates are represented. The asterisks indicate significant differences across all

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samples (Kruskal-Wallis, "*", P < 0.05; "**", P < 0.01; "***", P < 0.001). Color stripe represents

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metabolite-specific variation coefficients calculated as the relative median absolute distance (relative

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MAD); the degree of MAD is indicated by the node color from green (low) to red (high). (C) The

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heatmap on the bottom left showing the significant correlation between metabolite variation and

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module eigenmetabolite. Blue color represents negative correlation (r < -0.75, P < 10-3), while red

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represents positive correlation (r > 0.75, P < 10-3). (D) The heatmap on the bottom right showing

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relative expression of genes in 37 catechin pathway-related modules across all samples.

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Figure 6. GO enrichment and network analysis for catechin-related modules. GO (A) molecular

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function and (B) biological processes analysis for catechin-related modules. The color of the dots in

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the scatterplot represents the range of the -log10 (P-value). The correlation network of (C) GM74, (D)

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GM124, (E) GM77, and (F) GM201. Genes with a higher degree are indicated by red. Potential key

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genes and regulators discussed in the Results and Discussion section are indicated by larger circles.

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