Combinatorial Biosynthesis of Sulfated Benzenediol Lactones with a Phenolic Sulfotransferase from Fusarium graminearum PH-1

Xie, Linan; Xiao, Dongliang; Wang, Xiaojing; Wang, Chen; Bai, Jing; Yue, Qiulin; Yue, Haitao; Li, Ye; Molnár, István; Xu, Yuquan; Zhang, Liwen

doi:10.1128/msphere.00949-20

Cited by 18 publications

(20 citation statements)

References 68 publications

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“…Results obtained from this study showed that A. coerulea is capable of sulfation of chalcones and exhibits parallels between microbial and mammalian metabolism not only in phase I but also in phase II metabolism [21,31]. It is widely known that the phase II sulfation reactions are mediated by the enzyme sulfotransferases, which catalyze the transfer of sulfonate group from the active sulfate to the substrates containing hydroxyl groups [45]. Thus, the sulfate metabolites of licochalcones and xanthohumol were supposed to be produced by the enzyme sulfotransferase from A. coeralea.…”

Section: Microbial Transformation Of Licochalcones a B C H And Xanthohumol By A Coeruleamentioning

confidence: 74%

Microbial Conjugation Studies of Licochalcones and Xanthohumol

Han

Xiao

Lee

2021

IJMS

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Microbial conjugation studies of licochalcones (1–4) and xanthohumol (5) were performed by using the fungi Mucor hiemalis and Absidia coerulea. As a result, one new glucosylated metabolite was produced by M. hiemalis whereas four new and three known sulfated metabolites were obtained by transformation with A. coerulea. Chemical structures of all the metabolites were elucidated on the basis of 1D-, 2D-NMR and mass spectroscopic data analyses. These results could contribute to a better understanding of the metabolic fates of licochalcones and xanthohumol in mammalian systems. Although licochalcone A 4′-sulfate (7) showed less cytotoxic activity against human cancer cell lines compared to its substrate licochalcone A, its activity was fairly retained with the IC50 values in the range of 27.35–43.07 μM.

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Section: Microbial Transformation Of Licochalcones a B C H And Xanthohumol By A Coeruleamentioning

confidence: 74%

Microbial Conjugation Studies of Licochalcones and Xanthohumol

Han

Xiao

Lee

2021

IJMS

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“…Like other plant SOTs, LGS1 is predicted to be localized in cytoplasm. Cytosolic SOTs contain several conserved PAPS-binding motifs, including the one interacts with 5′-phosphate of PAPS (TYPKSGT), 3′-phosphate of PAPS (YxxRNxxDxxVS), and nucleotide of PAPS (GxxGxxK/R) ( Xie et al, 2020 ). Multiple sequence alignment indicates that LGS1 contains these motifs, but with some variations (SLPKSGT and YxxRExxDxxVS, respectively) ( Supplementary Figure 10 ).…”

Section: Resultsmentioning

confidence: 99%

“…LGS1 contains the highly conserved histidine residues (H216) ( Landi and Esposito, 2020 ) and moderately conserved histidine residues (H317A) ( Supplementary Figure 10 ), which likely act as a base to remove the proton from the substrate hydroxyl group, thereby forming an oxygen anion, and then attacking the sulfo group of PAPS to complete the transfer of the sulfo group. To determine whether these residues play a key role in catalysis, we conducted site-directed mutagenesis on residues likely act as a catalytic base (H216A, H317A) or crucial for PAPS binding (K148A, Y247F) ( Xie et al, 2020 ). While LGS1 H 216 A (resulting strain: YSL8f, Supplementary Table 3 ) exhibited same activity as wild type LGS1, replacing LGS1 with LGS1 K 148 A , LGS1 Y 247 F , and LGS1 H 317 A in ECL/YSL8a (resulting strain: YSL8g-i, Supplementary Table 3 ) completely abolished the synthesis of 4DO and 5DS ( Supplementary Figure 11 ), implying that these residues are critical to the catalytic activity of LGS1 ( Supplementary Figure 11 ).…”

Section: Resultsmentioning

confidence: 99%

A Unique Sulfotransferase-Involving Strigolactone Biosynthetic Route in Sorghum

2021

Front. Plant Sci.

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LOW GERMINATION STIMULANT 1 (LGS1) plays an important role in strigolactones (SLs) biosynthesis and Striga resistance in sorghum, but the catalytic function remains unclear. Using the recently developed SL-producing microbial consortia, we examined the activities of sorghum MORE AXILLARY GROWTH1 (MAX1) analogs and LGS1. Surprisingly, SbMAX1a (cytochrome P450 711A enzyme in sorghum) synthesized 18-hydroxy-carlactonoic acid (18-hydroxy-CLA) directly from carlactone (CL) through four-step oxidations. The further oxidated product orobanchol (OB) was also detected in the microbial consortium. Further addition of LGS1 led to the synthesis of both 5-deoxystrigol (5DS) and 4-deoxyorobanchol (4DO). Further biochemical characterization found that LGS1 functions after SbMAX1a by converting 18-hydroxy-CLA to 5DS and 4DO possibly through a sulfonation-mediated pathway. The unique functions of SbMAX1 and LGS1 imply a previously unknown synthetic route toward SLs.

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“…Similar to other plant SOTs, LGS1 is predicted to be localized in cytoplasm. Cytosolic SOTs contain several conserved PAPS-binding motifs, including the one interacts with 5′-phosphate of PAPS (TYPKSGT), 3’-phosphate of PAPS (YxxRNxxDxxVS), and nucleotide of PAPS (GxxGxxK/R) 26 . Multiple sequence alignment indicates that LGS1 contains these motifs, but with some variations ( SL PKSGT and YxxR E xxDxxVS, respectively) (Figure S10).…”

Section: Resultsmentioning

confidence: 99%

“…LGS1 contains the highly conserved histidine residues (H216) 27 and moderately conserved histidine residues (H317A) (Figure S10) which likely act as a base to remove the proton from the substrate hydroxyl group, thereby forming an oxygen anion, and then attacking the sulfo group of PAPS to complete the transfer of the sulfo group. To determine whether these residues play a key role in catalysis, we conducted site directed mutagenesis on residues likely act as a catalytic base (H216A, H317A) or crucial for PAPS binding (K148A, Y247F) 26 . While LGS1 H216A (resulting strain: YSL8f , Table S2) exhibited same activity as wildtype LGS1, replacing LGS1 with LGS1 K148A , LGS1 Y247F , and LGS1 H317A in ECL/YSL8a (resulting strain: YSL8g-i , Table S2) completely abolished the synthesis of 4DO and 5DS (Figure S11), implying that these residues are critical to the catalytic activity of LGS1 (Figure S11).…”

Section: Resultsmentioning

confidence: 99%

A unique sulfotransferase-involving strigolactone biosynthetic route in Sorghum

2021

Preprint

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LOW GERMINATION STIMULANT 1 (LGS1) plays an important role in strigolactones (SLs) biosynthesis and Striga resistance in sorghum but the catalytic function remains unclear. Using the recently developed SL-producing microbial consortia, we examined the activities of sorghum MAX1 analogs and LGS1. Surprisingly, SbMAX1d (accession # XP_002458367) synthesized 18-hydroxy-carlactonoic acid (18-hydroxy-CLA) directly from carlactone (CL) through four-step oxidations, and addition of LGS1 led to the synthesis of both 5-deoxystrigol (5DS) and 4-deoxyorobanchol (4DO). Further biochemical characterization found that LGS1 functions after SbMAX1d by converting 18-hydroxy-CLA to 18-sulphate-CLA to provide an easier leaving group to afford a spontaneous formation of 5DS and 4DO. The unique functions of SbMAX1 and LGS1 imply a previously unknown synthetic route towards strigolactones.

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Combinatorial Biosynthesis of Sulfated Benzenediol Lactones with a Phenolic Sulfotransferase from Fusarium graminearum PH-1

Cited by 18 publications

References 68 publications

Microbial Conjugation Studies of Licochalcones and Xanthohumol

Microbial Conjugation Studies of Licochalcones and Xanthohumol

A Unique Sulfotransferase-Involving Strigolactone Biosynthetic Route in Sorghum

A unique sulfotransferase-involving strigolactone biosynthetic route in Sorghum

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