Transcriptome analyses provide insights into the expression pattern and sequence similarity of several taxol biosynthesis-related genes in three Taxus species

Zhou, Ting; Luo, Xiujun; Yu, Chunna; Zhang, Chengchao; Zhang, Lei; Song, Yue; Dong, Ming; Shen, Chenjia

doi:10.1186/s12870-019-1645-x

Cited by 42 publications

(32 citation statements)

References 44 publications

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“…Transcriptome analysis is currently the most widely used and cost effective way to screen target gene(s) rapidly in functional genomic studies (Ali et al, 2018;Ma et al, 2019;Zhou et al, 2019). In this study, a total of 100,218 unigenes were generated by transtomic sequencing of three chemotypes of C. burmannii.…”

Section: Validation Of Degs Using Quantitative Real-time Pcr (Qrt-pcr)mentioning

confidence: 99%

Mining of candidate genes involved in the biosynthesis of dextrorotatory borneol in Cinnamomum burmannii by transcriptomic analysis on three chemotypes

Yang

Liu

et al. 2020

PeerJ

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Background Dextrorotatory borneol (D-borneol), a cyclic monoterpene, is widely used in traditional Chinese medicine as an efficient topical analgesic drug. Fresh leaves of Cinnamomum trees, e.g., C. burmannii and C. camphor, are the main sources from which D-borneol is extracted by steam distillation, yet with low yields. Insufficient supply of D-borneol has hampered its clinical use and production of patent remedies for a long time. Biological synthesis of D-borneol offers an additional approach; however, mechanisms of D-borneol biosynthesis remain mostly unresolved. Hence, it is important and necessary to elucidate the biosynthetic pathway of D-borneol. Results Comparative analysis on the gene expression patterns of different D-borneol production C. burmannii samples facilitates elucidation on the underlying biosynthetic pathway of D-borneol. Herein, we collected three different chemotypes of C. burmannii, which harbor different contents of D-borneol.A total of 100,218 unigenes with an N50 of 1,128 bp were assembled de novo using Trinity from a total of 21.21 Gb clean bases. We used BLASTx analysis against several public databases to annotate 45,485 unigenes (45.38%) to at least one database, among which 82 unigenes were assigned to terpenoid biosynthesis pathways by KEGG annotation. In addition, we defined 8,860 unigenes as differentially expressed genes (DEGs), among which 13 DEGs were associated with terpenoid biosynthesis pathways. One 1-deoxy-D-xylulose-5-phosphate synthase (DXS) and two monoterpene synthase, designated as CbDXS9, CbTPS2 and CbTPS3, were up-regulated in the high-borneol group compared to the low-borneol and borneol-free groups, and might be vital to biosynthesis of D-borneol in C. burmannii. In addition, we identified one WRKY, two BHLH, one AP2/ERF and three MYB candidate genes, which exhibited the same expression patterns as CbTPS2 and CbTPS3, suggesting that these transcription factors might potentially regulate D-borneol biosynthesis. Finally, quantitative real-time PCR was conducted to detect the actual expression level of those candidate genes related to the D-borneol biosynthesis pathway, and the result showed that the expression patterns of the candidate genes related to D-borneol biosynthesis were basically consistent with those revealed by transcriptome analysis. Conclusions We used transcriptome sequencing to analyze three different chemotypes of C. burmannii, identifying three candidate structural genes (one DXS, two monoterpene synthases) and seven potential transcription factor candidates (one WRKY, two BHLH, one AP2/ERF and three MYB) involved in D-borneol biosynthesis. These results provide new insight into our understanding of the production and accumulation of D-borneol in C. burmannii.

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Section: Validation Of Degs Using Quantitative Real-time Pcr (Qrt-pcr)mentioning

confidence: 99%

Mining of candidate genes involved in the biosynthesis of dextrorotatory borneol in Cinnamomum burmannii by transcriptomic analysis on three chemotypes

Yang

Liu

et al. 2020

PeerJ

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“…We previously performed metabolite analyses as part of a capacity building project for medicinal plants, which also included samples from T. media cell suspension cultures (16). Since these cultures were available to us as a source for candidate genes, we downloaded publicly available whole transcriptome shotgun sequencing (RNA-Seq) data sets acquired with this species (National Center for Biotechnology Information (NCBI) Bioproject numbers PRNJA169654, PRJNA341288, and PRNJA497542) (17,18), with an emphasis on suspension cells treated with the elicitor methyl jasmonate, which is commonly used to upregulate the formation of taxoids (19). We then searched in these publicly available data sets for gene sequences with homology to previously characterized AAEs of varying specificity (for details see Experimental procedures).…”

Section: Cloning and Categorization Of Candidate Aaesmentioning

confidence: 99%

“…First-strand cDNA was prepared from RNA with the SuperScript III First Strand Synthesis kit (Invitrogen, Carlsbad, CA, USA) with random hexamer oligonucleotides. Open reading frames for CoA ligases were amplified using gene-specific primers (Table S3) designed based on AAE sequences identified in publicly available T. media transcriptome data sets (NCBI Bioproject numbers PRNJA169654, PRJNA341288, and PRNJA497542) (17,18). Amplicons were ligated into the pET-32b vector featuring an encoded 6 x histidine tag (EMD Millipore, Burlington, MA, USA) and, following sequence confirmation, transformed into E. coli BL21(DE3) cells (New England Biolabs, Ipswich, MA, USA).…”

Section: Cloning and Heterologous Expression Of Candidate Aae Genesmentioning

confidence: 99%

Biochemical characterization of acyl activating enzymes for side chain moieties of Taxol and its analogs

Srividya

Lange

Hartmann

et al. 2020

Journal of Biological Chemistry

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Taxol (paclitaxel) is a very widely used anticancer drug, but its commercial sources mainly consist of stripped bark or suspension cultures of members of the plant genus Taxus. Taxol accumulates as part of a complex mixture of chemical analogs, termed taxoids, which complicates its production in pure form, highlighting the need for metabolic engineering approaches for high-level Taxol production in cell cultures or microbial hosts. Here, we report on the characterization of acyl-activating enzymes (AAEs) that catalyze the formation of CoA esters of different organic acids relevant for the N-substitution of the 3-phenylisoserine side chain of taxoids. On the basis of similarities to AAE genes of known function from other organisms, we identified candidate genes in publicly available transcriptome data sets obtained with Taxus × media. We cloned 17 AAE genes, expressed them heterologously in Escherichia coli, purified the corresponding recombinant enzymes, and performed in vitro assays with 27 organic acids as potential substrates. We identified TmAAE1 and TmAAE5 as the most efficient enzymes for the activation of butyric acid (Taxol D side chain), TmAAE13 as the best candidate for generating a CoA ester of tiglic acid (Taxol B side chain), TmAAE3 and TmAAE13 as suitable for the activation of 4-methylbutyric acid (N-debenzoyl-N-(2-methylbutyryl)taxol side chain), TmAAE15 as a highly efficient candidate for hexanoic acid activation (Taxol C side chain), and TmAAE4 as suitable candidate for esterification of benzoic acid with CoA (Taxol side chain). This study lays important groundwork for metabolic engineering efforts aimed at improving Taxol production in cell cultures.

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“…In addition, DEGs were mapped to the KEGG database in order to elucidate their biological functions (Liang et al 2019;Miao et al 2019;Zhou et al 2019). The top 20 most enriched pathways are shown in Figure 5B and Table A7.…”

Section: Functional Annotation Of Degsmentioning

confidence: 99%

Comparative analysis of transcriptome and metabolome uncovers the metabolic differences between Dendrobium officinale protocorms and mature stems

Mai

Yang

et al. 2020

All Life

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Dendrobium officinale caulis is the dried mature stems (Mat) of D. officinale Kimura et Migo. D. officinale protocorms (DOPs) are the conical embryonic tissues formed after seed germination. Previous studies suggest that these different plant parts possess similar pharmacological activities. However, the metabolic profiles and gene expression across different growth stages of D. officinale remain unknown. In this study, metabolome analysis based on GC and LC/MS/MS was carried out to assess the metabolic profile of both DOPs and Mat. Transcriptome analysis was used to reveal internal relationships between metabolites and the differing gene regulation. The results indicated that although DOPs and Mat had a similar chemical composition, they exhibited different patterns of content. GO classification and KEGG clustering of the differentially expressed genes (DEGs) between DOPs and Mat demonstrated that gene enrichment was mainly related to flavonoid biosynthetic and metabolic processes, carbohydrate metabolic processes, and polysaccharide catabolic processes. An alteration in gene expression related to specific metabolic pathways offered a probable explanation for the observed differences in metabolites between DOPs and Mat. This work provides a foundation for subsequent studies regarding the biosynthetic pathways of related metabolites from D. officinalis.

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Transcriptome analyses provide insights into the expression pattern and sequence similarity of several taxol biosynthesis-related genes in three Taxus species

Cited by 42 publications

References 44 publications

Mining of candidate genes involved in the biosynthesis of dextrorotatory borneol in Cinnamomum burmannii by transcriptomic analysis on three chemotypes

Mining of candidate genes involved in the biosynthesis of dextrorotatory borneol in Cinnamomum burmannii by transcriptomic analysis on three chemotypes

Biochemical characterization of acyl activating enzymes for side chain moieties of Taxol and its analogs

Comparative analysis of transcriptome and metabolome uncovers the metabolic differences between Dendrobium officinale protocorms and mature stems

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