Your search keyword '"deglycosylation"' showing total 1,030 results

1. Rat small intestine extract as a source of mammalian α- and β-glycosidases to study polyphenol bioaccessibility and deglycosylation in vitro: A case study with matrix-devoid and matrix-defined apple fractions

Author

Gallego-Lobillo, Pablo, Lopez-Rodulfo, Ivan M., and Martinez, Mario M.

Published

2025

2. Gamma-irradiated hydroxyapatite based electrochemical sensor for simultaneous detection of rutin and quercetin flavonoids

Author

Mayil Vealan, S.B., Ramcharan, Meena, Asokan, K., and Sekar, C.

Published

2024

3. Simultaneous extraction and deglycosylation for flavonoid analysis in Ginkgo biloba products using a two-phase deep eutectic solvent system

Author

Wu, Rong, Song, Yiting, Shi, Manman, Dong, Qihui, Cao, Jun, Yu, Pengfei, Cao, Fuliang, and Su, Erzheng

Published

2024

4. Designing a cost-effective and scalable expression platform for highly efficient recombinant endo-β-N-acetylglucosaminidase H using fed-batch strategy in E. coli

Author

Mohanty, Shilpa, Babbal, Talwar, Mohini, Chauhan, Shivani, Sinha, Priya, Sharma, Shubham, and Khasa, Yogender Pal

Published

2025

5. Functional prediction of the potential NGLY1 mutations associated with rare disease CDG

Author

Yuan, Shuying, Chen, Yanwen, Zou, Lin, Lu, Xinrong, Liu, Ruijie, Zhang, Shaoxing, Zhang, Yuxin, Chen, Cuiying, Cheng, Dongqing, Chen, Li, and Sun, Guiqin

Published

2024

6. N-Glycosidase Rudaea cellulosilytica (PNGase Rc) Column for the Characterization of Glycoprotein Conformational Epitopes by Hydrogen/Deuterium Exchange Mass Spectrometry (HDX-MS).

Author

Deng, Ying, Yang, Dongyuan, Zheng, Wen, Qi, Ao, Yang, Yulin, Shu, Zhulin, Zhang, Fengyi, Han, Hongbo, Chen, Jin, and Zheng, Jie

Subjects

*PEPTIDES, *MASS spectrometry, *GLYCOPROTEINS, *MOLECULAR dynamics, *DEGLYCOSYLATION

Abstract

Hydrogen/deuterium exchange mass spectrometry (HDX-MS) is a sensitive technique used to study the conformational dynamics of proteins in solution. However, performing HDX-MS with N-linked glycoproteins is challenging. Analyzing glycoproteins through HDX-MS requires the use of N-glycoprotein deglycosylation enzyme (peptide: N-glycanase, abbreviated as PNGase) to deglycosylate glycoproteins. Traditional PNGases are inactive or have low activity under HDX-MS operating conditions. Here, we recommend the use of ultra-acidic N-glycopeptidase from PNGase Rc, which exhibits optimal enzymatic activity compared to other PNGases at pH 2.2. We covalently fixed PNGase Rc onto POROS resin for HDX-MS online deglycosylation. The results show that the immobilized PNGase Rc combined with pepsin column has good stability under various quenching conditions. Its online deglycosylation efficiency is better than other PNGases. Meanwhile, we used AlphaFold 2 and molecular dynamics (MD) to characterize the structure and stability of PNGase Rc and other PNGases, and demonstrated that PNGase Rc is the most stable. [ABSTRACT FROM AUTHOR]

Published

2025

7. Non-glycanated ΔDCN isoform in muscle invasive bladder cancer mediates cancer stemness and gemcitabine resistance.

Author

Wu, Nisha, Wang, Jinxiang, Fan, Mingming, Liang, Yanling, wei Qi, Xiao, Deng, Fan, and Zeng, Fangyin

Abstract

Background: The small leucine-rich proteoglycan decorin (DCN) is recognized for its diverse roles in tissue homeostasis and malignant progression. Nevertheless, the regulatory effects of DCN on bladder cancer stem cells (BCSCs) and the underlying mechanisms in muscle-invasive bladder cancer (MIBC) remain to be elucidated. Methods: The study obtained data (including scRNA-seq, clinicopathological characteristics, and survival) were acquired from TCGA and GEO. The BCSCs were cultured by enriching the suspension culture in a serum-free medium, followed by flow cytometry sorting. Overexpression/knockdown was constructed by utilizing lentivirus. The surface biomarkers of cancer stem cells were identified via flow cytometry. Cell proliferation and self-renewal were evaluated by CCK8 and Sphere formation assays, and in vivo tumor growth was evaluated with subcutaneous xenografts. Results: Total DCN expression was significantly elevated in muscle-invasive bladder cancer (MIBC) and was associated with poor prognosis. The ΔDCN isoform, which lacks glycosylation sites, was identified in bladder cancer stem cells (BCSCs) derived from clinical tissue samples and bladder cancer cell lines. Suppression of ΔDCN expression resulted in a reduction of BCSC stemness. Both in vitro and in vivo experiments indicated that overexpression of full-length DCN inhibited stemness within the extracellular matrix. Conversely, overexpression of ΔDCN and the introduction of exogenous recombinant decorin protein in ΔDCN-knockdown BCSC-SW780 cell lines enhanced stemness within the cytoplasm. The ΔDCN isoform exhibited resistance to gemcitabine chemotherapy in vitro. Conclusion: Non-glycanated ΔDCN isoforms were identified in bladder cancer stem cells (BCSCs), where they exhibited differential cytoplasmic localization and promoted oncogenic effects by inducing a stemness phenotype and conferring resistance to gemcitabine chemotherapy. These oncogenic effects are in stark contrast to the anti-tumor functions of glycosylated DCN in the extracellular matrix. The ratio of ΔDCN isoforms to glycosylated DCN is pivotal in predicting tumor progression and therapeutic resistance. [ABSTRACT FROM AUTHOR]

Published

2024

8. Targeted protein editing technique in living mammalian cells by peptide-fused PNGase

Author

Min Wu, Guijie Bai, Ziyi Zhang, Haixia Xiao, Wenliang Sun, and Chaoguang Tian

Subjects

N-glycosylated proteins, peptide:N-glycanase (PNGase), protein-targeting peptides, deglycosylation, protein sequence editing, protein degradation, Medicine

Abstract

Various precise gene editing techniques at the DNA/RNA level, driven by clustered regularly interspaced short palindrome repeats (CRISPR)/CRISPR-associated protein 9 (Cas9) technology, have gained significant prominence. Yet, research on targeted protein editing techniques remains limited. Only a few attempts have been made, including the use of specific proteases and de-O-glycosylating enzymes as editing enzymes. Here, we propose direct editing of N-glycosylated proteins using de-N-glycosylating enzymes to modify N-glycosylation and simultaneously alter the relevant asparagine residue to aspartate in living cells. Selective protein deglycosylation editors were developed by fusing high-affinity protein-targeting peptides with active peptide:N-glycanases (PNGases). Three crucial cell membrane proteins, programmed cell death protein-1 (PD-1), programmed cell death-1 ligand 1 (PD-L1), and severe acute respiratory syndrome coronavirus-2 (SARS-CoV-2) spike protein, were chosen to be tested as a proof of concept. N-linked glycans were removed, and the relevant sites were converted from Asn to Asp in living mammalian cells, destabilizing target proteins and accelerating their degradation. Further investigation focused on SARS-CoV-2 spike protein deglycosylation editing. The collaboration of LCB1-PNGase F (PNGF) effectively reduced syncytia formation, inhibited pseudovirus packaging, and significantly hindered virus entry into host cells, which provides insights for coronavirus disease 2019 (COVID-19) treatment. This tool enables editing protein sequences post-de-N-glycosylation in living human cells, shedding light on protein N-glycosylation functions, and Asn to Asp editing in organisms. It also offers the potential for developing protein degradation technologies.

Published

2024

9. N-glycosylation of the envelope glycoprotein I is essential for the proliferation and virulence of the duck plague virus.

Author

Ning, Yaru, Wang, Mingshu, Cheng, Anchun, Yang, Qiao, Tian, Bin, Ou, Xumin, Sun, Di, He, Yu, Wu, Zhen, Zhao, Xinxin, Zhang, Shaqiu, Wu, Ying, Huang, Juan, Yu, Yanling, Zhang, Ling, Jia, Renyong, Liu, Mafeng, Zhu, Dekang, and Chen, Shun

Subjects

WESTERN immunoblotting, REVERSE genetics, GOLGI apparatus, ENDOPLASMIC reticulum, DEGLYCOSYLATION

Abstract

Duck plague virus (DPV) causes the highly pathogenic duck plague, and the envelope glycoprotein I (gI), as one of the key virulence genes, has not yet had its critical virulence sites identified through screening. This study used reverse genetics technology to target the gI, specifically within the DPV genome. Four DPV mutants with gI N-glycosylation site mutations were designed and constructed, and these mutant strains were successfully rescued. Our results confirmed that three asparagine residues of gI (N69, N78, and N265) are N-glycosylation sites, and western blot analysis substantiated that glycosylation at each predicted N-glycosylation site was compromised. The deglycosylation of gI leads to the protein misfolding and subsequent retention in the endoplasmic reticulum (ER). The subsequent deglycosylated gI is carried into the Golgi apparatus (GM130) in the interaction of gE. Compared to the parental virus, the mutated virus shows a 66.3% reduction in intercellular transmission capability. In ducks, the deglycosylation of gI significantly reduces DPV replication in vivo, thereby weakening the virulence of DPV. This study represents the first successful creation of a weak DPV virus strain by specific mutation at the N-glycosylation site. The findings provide a foundational understanding of DPV pathogenesis and form the basis for developing live attenuated vaccines against the disease. [ABSTRACT FROM AUTHOR]

Published

2024

10. Leishmania major-induced alteration of host cellular and systemic copper homeostasis drives the fate of infection.

Author

Paul, Rupam, Chakrabarty, Adrija, Samanta, Suman, Dey, Swastika, Pandey, Raviranjan, Maji, Saptarshi, Pezacki, Aidan T., Chang, Christopher J., Datta, Rupak, and Gupta, Arnab

Subjects

*COPPER, *LEISHMANIA major, *LABORATORY mice, *ANIMAL disease models, *DEGLYCOSYLATION, *HOMEOSTASIS

Abstract

Copper plays a key role in host-pathogen interaction. We find that during Leishmania major infection, the parasite-harboring macrophage regulates its copper homeostasis pathway in a way to facilitate copper-mediated neutralization of the pathogen. Copper-ATPase ATP7A transports copper to amastigote-harboring phagolysosomes to induce stress on parasites. Leishmania in order to evade the copper stress, utilizes a variety of manipulative measures to lower the host-induced copper stress. It induces deglycosylation and degradation of host-ATP7A and downregulation of copper importer, CTR1 by cysteine oxidation. Additionally, Leishmania induces CTR1 endocytosis that arrests copper uptake. In mouse model of infection, we report an increase in systemic bioavailable copper in infected animals. Heart acts as the major organ for diverting its copper reserves to systemic circulation to fight-off infection by downregulating its CTR1. Our study explores reciprocal mechanism of manipulation of host copper homeostasis pathway by macrophage and Leishmania to gain respective advantages in host-pathogen interaction. Leishmania major alters host copper dynamics. Macrophages utilize copper via ATP7A to stress the pathogen, countered by Leishmania that reduces ATP7A and the copper importer CTR1. Infection elevates mouse systemic copper that aids in its defense. [ABSTRACT FROM AUTHOR]

Published

2024

11. Renoprotective Effects of Daprodustat in Patients with Chronic Kidney Disease and Renal Anemia.

Author

Shimada, Yoshitaka, Izumi, Yuichiro, Yasuoka, Yukiko, Oshima, Tomomi, Nagaba, Yasushi, Nanami, Masayoshi, Sands, Jeff M., Takahashi, Noriko, Kawahara, Katsumasa, and Nonoguchi, Hiroshi

Subjects

*PROXIMAL kidney tubules, *CHRONIC kidney failure, *KIDNEY physiology, *GLOMERULAR filtration rate, *INTERSTITIAL cells

Abstract

Many large-scale studies revealed that exogenous erythropoietin, erythropoiesis-stimulating agents, have no renoprotective effects. We reported the renoprotective effects of endogenous erythropoietin production on renal function in ischemic reperfusion injury (IRI) of the kidney using the prolyl hydroxylase domain (PHD) inhibitor, Roxadustat. The purpose of this study was to investigate the effects of daprodustat on the progression of chronic renal failure. We retrospectively investigated the effects of daprodustat on the progression of chronic renal failure and renal anemia in patients with stages 3a-5 chronic kidney diseases (estimated glomerular filtration rate, eGFR < 60 mL/min/1.73 m2). The results show that daprodustat largely slowed the reduction in eGFR. The recovery of renal function was observed in some patients. Daprodustat is useful not only for renal anemia but also for the preservation of renal function. The renoprotective effect of daprodustat was small in patients with serum creatinine larger than 3–4 mg/dL because of low residual renal function. The appearance of renal anemia would be a sign of the time to start using daprodustat. [ABSTRACT FROM AUTHOR]

Published

2024

12. PD-L1 deglycosylation promotes its nuclear translocation and accelerates DNA double-strand-break repair in cancer.

Author

Shu, Zhen, Dwivedi, Bhakti, Switchenko, Jeffrey M., Yu, David S., and Deng, Xingming

Subjects

DOUBLE-strand DNA breaks, PROGRAMMED death-ligand 1, LUNG cancer, MEDICAL screening, DEGLYCOSYLATION, IONIZING radiation, DNA repair

Abstract

Resistance to radiotherapy is a major barrier during cancer treatment. Here using genome-scale CRISPR/Cas9 screening, we identify CD274 gene, which encodes PD-L1, to confer lung cancer cell resistance to ionizing radiation (IR). Depletion of endogenous PD-L1 delays the repair of IR-induced DNA double-strand breaks (DSBs) and PD-L1 loss downregulates non-homologous end joining (NHEJ) while overexpression of PD-L1 upregulates NHEJ. IR induces translocation of PD-L1 from the membrane into nucleus dependent on deglycosylation of PD-L1 at N219 and CMTM6 and leads to PD-L1 recruitment to DSBs foci. PD-L1 interacts with Ku in the nucleus and enhances Ku binding to DSB DNA. The interaction between the IgC domain of PD-L1 and the core domain of Ku is required for PD-L1 to accelerate NHEJ-mediated DSB repair and produce radioresistance. Thus, PD-L1, in addition to its immune inhibitory activity, acts as mechanistic driver for NHEJ-mediated DSB repair in cancer. Resistance to radiotherapy is a major barrier during cancer treatment. Here the authors find that radiation-induced DNA double-strand-breaks (DSBs) facilitate PD-L1 deglycosylation and translocation into the nucleus, leading to promotion of NHEJ-mediated DSB repair and lung cancer radioresistance. [ABSTRACT FROM AUTHOR]

Published

2024

13. Anything you can do, glycans do better: deglycosylation and noncanonical ubiquitination vie to rule the proteasome.

Author

Lehrbach, Nicolas

Subjects

*TRANSCRIPTION factors, *UBIQUITINATION, *UBIQUITIN, *DEGLYCOSYLATION, *GLYCANS

Abstract

The Nrf1/Nfe2L1 transcription factor is a master regulator of proteasome biogenesis. New work by Yoshida and colleagues reveals a surprising mechanism by which ubiquitination of N -glycosylated Nrf1 controls its function. [ABSTRACT FROM AUTHOR]

Published

2024

14. Different Effects of Deglycosylation on the Lactose Sensing Ability of Mesophilic and Thermophilic Cellobiose Dehydrogenases

Author

Ma, Yaohong, Xue, Yunlong, Wang, Xingbao, Shao, Yue, Huang, Xiaozhen, Zhang, Zhenyu, Zhu, Sirong, and Gong, Weili

Published

2024

15. Doxorubicin induces deglycosylation of cancer cell-intrinsic PD-1 by NGLY1.

Author

Dexuan Wu, Zhen Wu, Han Yao, Xiaojun Yan, Zishan Jiao, Yajing Liu, Meng Zhang, and Donglai Wang

Subjects

*IMMUNE checkpoint proteins, *PROGRAMMED cell death 1 receptors, *TUMOR proteins, *DOXORUBICIN, *DEGLYCOSYLATION

Abstract

Tumor cells can express the immune checkpoint protein programmed death-1 (PD-1), but how cancer cell-intrinsic PD-1 is regulated in response to cellular stresses remains largely unknown. Here, we uncover a unique mechanism by which the chemotherapy drug doxorubicin (Dox) regulates cancer cell-intrinsic PD-1. Dox upregulates PD-1 mRNA while reducing PD-1 protein levels in tumor cells. Although Dox shortens the PD-1 half-life, it fails to directly induce PD-1 degradation. Instead, we observe that Dox promotes the interaction between peptide-N(4)-(N-acetyl-beta-glucosaminyl)asparagine amidase (NGLY1) and PD-1, facilitating NGLY1-mediated PD-1 deglycosylation and destabilization. The maintenance of PD-1 sensitizes tumor cells to Dox-mediated antiproliferative effects. Our study unveils a regulatory mechanism of PD-1 in response to Dox and highlights a potential role of cancer cell-intrinsic PD-1 in Dox-mediated antitumor effects. [ABSTRACT FROM AUTHOR]

Published

2024

16. OGA mutant aberrantly hydrolyzes O-GlcNAc modification from PDLIM7 to modulate p53 and cytoskeleton in promoting cancer cell malignancy.

Author

Chia-Wei Hu, Ao Wang, Dacheng Fan, Worth, Matthew, Zhengwei Chen, Junfeng Huang, Jinshan Xie, Macdonald, John, Lingjun Li, and Jiaoyang Jiang

Subjects

*CANCER cell motility, *CANCER cells, *BIOCHEMICAL substrates, *P53 antioncogene, *PROTEIN domains

Abstract

O-GlcNAcase (OGA) is the only human enzyme that catalyzes the hydrolysis (deglycosylation) of O-linked beta-N-acetylglucosaminylation (O-GlcNAcylation) from numerous protein substrates. OGA has broad implications in many challenging diseases including cancer. However, its role in cell malignancy remains mostly unclear. Here, we report that a cancer-derived point mutation on the OGA's noncatalytic stalk domain aberrantly modulates OGA interactome and substrate deglycosylation toward a specific set of proteins. Interestingly, our quantitative proteomic studies uncovered that the OGA stalk domain mutant preferentially deglycosylated protein substrates with +2 proline in the sequence relative to the O-GlcNAcylation site. One of the most dysregulated substrates is PDZ and LIM domain protein 7 (PDLIM7), which is associated with the tumor suppressor p53. We found that the aberrantly deglycosylated PDLIM7 suppressed p53 gene expression and accelerated p53 protein degradation by promoting the complex formation with E3 ubiquitin ligase MDM2. Moreover, deglycosylated PDLIM7 significantly up-regulated the actin-rich membrane protrusions on the cell surface, augmenting the cancer cell motility and aggressiveness. These findings revealed an important but previously unappreciated role of OGA's stalk domain in protein substrate recognition and functional modulation during malignant cell progression. [ABSTRACT FROM AUTHOR]

Published

2024

17. Functional studies with IgM and IgA immunoglobulins: binding to pIgR, FcαμR, FcμR, and CDC activities.

Author

Beyer, Hanna, Sommerfeld, Mark, Grandien, Kaj, Faust, Christine, Tillmann, Bodo, Leuschner, Wulf Dirk, Régnier‐Vigouroux, Anne, Weil, Sandra, Rao, Ercole, and Langer, Thomas

Subjects

*IMMUNOGLOBULIN A, *IMMUNOGLOBULINS, *IMMUNOGLOBULIN M, *IMMUNOGLOBULIN receptors, *IMMUNE system, *IMMUNE response, *IMMUNOGLOBULIN G

Abstract

IgMs are the first antibodies produced by the immune system upon encounter of a possible pathogen and are one of five antibody subclasses in humans. For IgG, the most intensively studied antibody class, the N‐linked glycosylation site located in the Fc‐domain is directly involved in high affinity binding to the respective receptors and initiation of corresponding immune response. IgM molecules have five N‐glycosylation sites and one N‐glycosylation site in the J‐chain, which can be incorporated in IgM or IgA molecules. There is only limited knowledge available concerning the function of these N‐glycosylations in IgMs. To address this question, we produced IgM molecules lacking a particular N‐glycosylation site and tested these variants as well as IgA molecules for binding to the known receptors: the polymeric immunoglobulin receptor (pIgR), the dual receptor for IgA and IgM, FcαμR, and the specific receptor for IgM, FcμR. The single glycosylation sites did not show an impact on expression and multimerization, except for variant N402Q, which could not be expressed. In SPR measurements, no major impact on the binding to the receptors by particular glycosylation sites could be detected. In cellular assays, deglycosylated variants showed some alterations in induction of CDC activity. Most strikingly, we observed also binding of IgA to the FcμR in the same affinity range as IgM, suggesting that this might have a physiological role. To further substantiate the binding of IgA to FcμR we used IgA from different origins and were able to confirm binding of IgA preparations to the FcμR. [ABSTRACT FROM AUTHOR]

Published

2024

18. Biotransformation approach to produce rare ginsenosides F1, compound Mc1, and Rd2 from major ginsenosides.

Author

Diao, Mengxue, Chen, Yanchi, Meng, Lijun, Li, Jianxiu, and Xie, Nengzhong

Abstract

The stems and leaves of Panax notoginseng contain high saponins, but they are often discarded as agricultural waste. In this study, the predominant ginsenosides Rg1, Rc, and Rb2, presented in the stems and leaves of ginseng plants, were biotransformed into value-added rare ginsenosides F1, compound Mc1 (C-Mc1), and Rd2, respectively. A fungal strain YMS6 (Penicillium sp.) was screened from the soil as a biocatalyst with high selectivity for the deglycosylation of major ginsenosides. Under the optimal fermentation conditions, the yields of F1, C-Mc1, and Rd2 were 97.95, 68.64, and 79.58%, respectively. This study provides a new microbial resource for the selective conversion of protopanaxadiol-type and protopanaxatriol-type major saponins into rare ginsenosides via the whole-cell biotransformation and offers a solution for the better utilization of P. notoginseng waste. [ABSTRACT FROM AUTHOR]

Published

2024

19. Glycoside-metabolizing oxidoreductase D3dgpA from human gut bacterium

Author

Heji Kim, Huynh Thi Ngoc Mi, Joong-Hoon Ahn, Jong Suk Lee, Bekir Engin Eser, Jongkeun Choi, and Jaehong Han

Subjects

deglycosylation, D3dgpA, Gfo/Idh/MocA family, glycosides, NAD+, oxidoreductase, Biotechnology, TP248.13-248.65

Abstract

The Gfo/Idh/MocA family enzyme DgpA was known to catalyze the regiospecific oxidation of puerarin to 3”-oxo-puerarin in the presence of 3-oxo-glucose. Here, we discovered that D3dgpA, dgpA cloned from the human gut bacterium Dorea sp. MRG-IFC3, catalyzed the regiospecific oxidation of various C-/O-glycosides, including puerarin, in the presence of methyl β-D-3-oxo-glucopyranoside. While C-glycosides were converted to 3”- and 2”-oxo-products by D3dgpA, O-glycosides resulted in the formation of aglycones and hexose enediolone from the 3”-oxo-products. From DFT calculations, it was found that isomerization of 3”-oxo-puerarin to 2”-oxo-puerarin required a small activation energy of 9.86 kcal/mol, and the O-glycosidic bond cleavage of 3”-oxo-products was also thermodynamically favored with a small activation energy of 3.49 kcal/mol. In addition, the reaction mechanism of D3dgpA was discussed in comparison to those of Gfo/Idh/MocA and GMC family enzymes. The robust reactivity of D3dgpA was proposed as a new general route for derivatization of glycosides.

Published

2024

20. Tubular Endogenous Erythropoietin Protects Renal Function against Ischemic Reperfusion Injury.

Author

Yasuoka, Yukiko, Izumi, Yuichiro, Fukuyama, Takashi, Oshima, Tomomi, Yamazaki, Taiga, Uematsu, Takayuki, Kobayashi, Noritada, Nanami, Masayoshi, Shimada, Yoshitaka, Nagaba, Yasushi, Mukoyama, Masashi, Sands, Jeff M., Takahashi, Noriko, Kawahara, Katsumasa, and Nonoguchi, Hiroshi

Subjects

*REPERFUSION injury, *KIDNEY physiology, *ERYTHROPOIETIN, *ERYTHROPOIETIN receptors, *INTERSTITIAL cells

Abstract

Many large-scale studies show that exogenous erythropoietin, erythropoiesis-stimulating agents, lack any renoprotective effects. We investigated the effects of endogenous erythropoietin on renal function in kidney ischemic reperfusion injury (IRI) using the prolyl hydroxylase domain (PHD) inhibitor, Roxadustat (ROX). Four h of hypoxia (7% O2) and 4 h treatment by ROX prior to IRI did not improve renal function. In contrast, 24–72 h pretreatment by ROX significantly improved the decline of renal function caused by IRI. Hypoxia and 4 h ROX increased interstitial cells-derived Epo production by 75- and 6-fold, respectively, before IRI, and worked similarly to exogenous Epo. ROX treatment for 24–72 h increased Epo production during IRI by 9-fold. Immunohistochemistry revealed that 24 h ROX treatment induced Epo production in proximal and distal tubules and worked similarly to endogenous Epo. Our data show that tubular endogenous Epo production induced by 24–72 h ROX treatment results in renoprotection but peritubular exogenous Epo production by interstitial cells induced by hypoxia and 4 h ROX treatment did not. Stimulation of tubular, but not peritubular, Epo production may link to renoprotection. [ABSTRACT FROM AUTHOR]

Published

2024

21. Biorefinery of flavonoid aglycones using acidic natural deep eutectic solvents: Role of Bronsted acids and application in valorization of Sophora japonica buds waste.

Author

Yishu Ni, Lin Zhu, Shuhui Ye, Xiafeng Xu, Xianrui Liang, and Sheng Fang

Subjects

*FLAVONOIDS, *CHOLINE chloride, *SOPHORA, *AGLYCONES, *CITRIC acid, *EUTECTICS, *FLAVONOID glycosides, *CYTOTOXINS, *SOLVENTS

Abstract

Biorefinery of flavonoid aglycones by natural deep eutectic solvents (NADESs) is a green approach for the valorization of agro-food wastes. Using rutin/quercetin as a model system, this work studies the role of Bronsted acids in deglycosylation of flavonoid glycosides and the sustainable approach to producing aglycone-rich extracts by acidic NADESs. Different NADESs were tested, and the effects of Bronsted acids in catalysis and Hammett acidities were determined. The deglycosylation kinetics of rutin in the choline chloride-citric acid was measured and followed a first-order model with a half-life time (t1/2) of 0.16 h at 90 °C and an activation energy (Ea) of 140.3 kJ mol-1. A two-step one-pot approach was valid to produce quercetin-rich extracts from Sophora japonica buds waste. The quercetin-to-rutin ratio in the acidic NADES extracts was adjustable by changing the heating time. The acidic NADES of ChCl-Citric and quercetin-rich extracts showed low cytotoxicity to Caco-2 cells with EC50 greater than 2000 mg L-1, and the cytotoxicity was mainly determined by citric acid. The study provides a new perspective for the valorization of bioproducts into ready-to-use flavonoid aglycone-rich extracts using acidic NADES. [ABSTRACT FROM AUTHOR]

Published

2024

22. Deglycosylated RBD produced in Pichia pastoris as a low-cost sera COVID-19 diagnosis tool and a vaccine candidate.

Author

Idrovo-Hidalgo, Tommy, Pignataro, María F, Bredeston, Luis M, Elias, Fernanda, Herrera, María G, Pavan, María F, Foscaldi, Sabrina, Suireszcz, Mayra, Fernández, Natalia B, Wetzler, Diana E, Paván, Carlos H, Craig, Patricio O, Roman, Ernesto A, Ruberto, Lucas A M, Noseda, Diego G, Ibañez, Lorena I, Czibener, Cecilia, Consortium, Argentinian AntiCovid, Ugalde, Juan E, and Nadra, Alejandro D

Subjects

*PICHIA pastoris, *PROTEIN expression, *COVID-19 testing, *COVID-19 pandemic, *EUKARYOTIC cells, *SECRETION, *SERUM, *GLYCANS

Abstract

During the COVID-19 outbreak, numerous tools including protein-based vaccines have been developed. The methylotrophic yeast Pichia pastoris (synonymous to Komagataella phaffii) is an eukaryotic cost-effective and scalable system for recombinant protein production, with the advantages of an efficient secretion system and the protein folding assistance of the secretory pathway of eukaryotic cells. In a previous work, we compared the expression of SARS-CoV-2 Spike Receptor Binding Domain in P. pastoris with that in human cells. Although the size and glycosylation pattern was different between them, their protein structural and conformational features were indistinguishable. Nevertheless, since high mannose glycan extensions in proteins expressed by yeast may be the cause of a nonspecific immune recognition, we deglycosylated RBD in native conditions. This resulted in a highly pure, homogenous, properly folded and monomeric stable protein. This was confirmed by circular dichroism and tryptophan fluorescence spectra and by SEC-HPLC, which were similar to those of RBD proteins produced in yeast or human cells. Deglycosylated RBD was obtained at high yields in a single step, and it was efficient in distinguishing between SARS-CoV-2-negative and positive sera from patients. Moreover, when the deglycosylated variant was used as an immunogen, it elicited a humoral immune response ten times greater than the glycosylated form, producing antibodies with enhanced neutralizing power and eliciting a more robust cellular response. The proposed approach may be used to produce at a low cost, many antigens that require glycosylation to fold and express, but do not require glycans for recognition purposes. [ABSTRACT FROM AUTHOR]

Published

2024

23. Enzymatic β-elimination in natural product O- and C-glycoside deglycosylation.

Author

Bitter, Johannes, Pfeiffer, Martin, Borg, Annika J. E., Kuhlmann, Kirill, Pavkov-Keller, Tea, Sánchez-Murcia, Pedro A., and Nidetzky, Bernd

Subjects

NATURAL products, AGROBACTERIUM tumefaciens, PRODUCT elimination, DEGLYCOSYLATION, CONVERGENT evolution

Abstract

Biological degradation of natural product glycosides involves, alongside hydrolysis, β-elimination for glycosidic bond cleavage. Here, we discover an O-glycoside β-eliminase (OGE) from Agrobacterium tumefaciens that converts the C3-oxidized O-β-d-glucoside of phloretin (a plant-derived flavonoid) into the aglycone and the 2-hydroxy-3-keto-glycal elimination product. While unrelated in sequence, OGE is structurally homologous to, and shows effectively the same Mn2+ active site as, the C-glycoside deglycosylating enzyme (CGE) from a human intestinal bacterium implicated in β-elimination of 3-keto C-β-d-glucosides. We show that CGE catalyzes β-elimination of 3-keto O- and C-β-d-glucosides while OGE is specific for the O-glycoside substrate. Substrate comparisons and mutagenesis for CGE uncover positioning of aglycone for protonic assistance by the enzyme as critically important for C-glycoside cleavage. Collectively, our study suggests convergent evolution of active site for β-elimination of 3-keto O-β-d-glucosides. C-Glycoside cleavage is a specialized feature of this active site which is elicited by substrate through finely tuned enzyme-aglycone interactions. Biological degradation of glycosides involves, alongside hydrolysis, β-elimination for glycosidic bond cleavage. Here, the authors report an O-glycoside β-eliminase from Agrobacterium tumefaciens that converts the C3-oxidized O-β-d-glucoside of phloretin into the aglycone and the 2-hydroxy-3-keto-d-glycal elimination product, and suggest convergent evolution of β-eliminase active sites for the cleavage of natural product 3-keto-O-glycosides. [ABSTRACT FROM AUTHOR]

Published

2023

24. Deglycosylation of eukaryotic-expressed flagellin restores adjuvanticity.

Author

Khim, Koemchhoy, Puth, Sao, Radhakrishnan, Kamalakannan, Nguyen, Tien Duc, Lee, Youn Suhk, Jung, Che-Hun, Lee, Shee Eun, and Rhee, Joon Haeng

Subjects

FLAGELLIN, DEGLYCOSYLATION, VIBRIO vulnificus, SITE-specific mutagenesis, NUCLEIC acids

Abstract

Flagellin, the TLR5 agonist, shows potent adjuvant activities in diverse vaccines and immunotherapies. Vibrio vulnificus flagellin B expressed in eukaryotic cells (eFlaB) could not stimulate TLR5 signaling. Enzymatic deglycosylation restored eFlaB's TLR5 stimulating functionality, suggesting that glycosylation interferes with eFlaB binding to TLR5. Site-directed mutagenesis of N-glycosylation residues restored TLR5 stimulation and adjuvanticity. Collectively, deglycosylated eFlaB may provide a built-in adjuvant platform for eukaryotic-expressed antigens and nucleic acid vaccines. [ABSTRACT FROM AUTHOR]

Published

2023

25. In vivo deglycosylation of recombinant glycoproteins in tobacco BY‐2 cells.

Author

Herman, Xavier, Far, Johann, Peeters, Marie, Quinton, Loïc, Chaumont, François, and Navarre, Catherine

Subjects

*GLYCOPROTEINS, *DEGLYCOSYLATION, *PROTEIN stability, *CELL lines, *TOBACCO, *HUMAN cytomegalovirus, *IMMUNOGLOBULIN G

Abstract

Summary: Production of recombinant pharmaceutical glycoproteins has been carried out in multiple expression systems. However, N‐glycosylation, which increases heterogeneity and raises safety concerns due to the presence of non‐human residues, is usually not controlled. The presence and composition of N‐glycans are also susceptible to affect protein stability, function and immunogenicity. To tackle these issues, we are developing glycoengineered Nicotiana tabacum Bright Yellow‐2 (BY‐2) cell lines through knock out and ectopic expression of genes involved in the N‐glycosylation pathway. Here, we report on the generation of BY‐2 cell lines producing deglycosylated proteins. To this end, endoglycosidase T was co‐expressed with an immunoglobulin G or glycoprotein B of human cytomegalovirus in BY‐2 cell lines producing only high mannose N‐glycans. Endoglycosidase T cleaves high mannose N‐glycans to generate single, asparagine‐linked, N‐acetylglucosamine residues. The N‐glycosylation profile of the secreted antibody was determined by mass spectrometry analysis. More than 90% of the N‐glycans at the conserved Asn297 site were deglycosylated. Likewise, extensive deglycosylation of glycoprotein B, which possesses 18 N‐glycosylation sites, was observed. N‐glycan composition of gB glycovariants was assessed by in vitro enzymatic mobility shift assay and proven to be consistent with the expected glycoforms. Comparison of IgG glycovariants by differential scanning fluorimetry revealed a significant impact of the N‐glycosylation pattern on the thermal stability. Production of deglycosylated pharmaceutical proteins in BY‐2 cells expands the set of glycoengineered BY‐2 cell lines. [ABSTRACT FROM AUTHOR]

Published

2023

26. Cholangiocytes express an isoform of soluble adenylyl cyclase that is N‐linked glycosylated and secreted in extracellular vesicles.

Author

Go, Simei, Li, Hang Lam, Chang, Jung‐Chin, Verhoeven, Arthur J., and Elferink, Ronald P. J. Oude

Subjects

*EXTRACELLULAR vesicles, *ADENYLATE cyclase, *CARRIER proteins, *DEGLYCOSYLATION, *PROTEIN transport

Abstract

Soluble adenylyl cyclase (sAC)‐derived cAMP regulates various cellular processes; however, the regulatory landscape mediating sAC protein levels remains underexplored. We consistently observed a 85 kD (sAC85) or 75 kD (sAC75) sAC protein band under glucose‐sufficient or glucose‐deprived states, respectively, in H69 cholangiocytes by immunoblotting. Deglycosylation by PNGase‐F demonstrated that both sAC75 and sAC85 are N‐linked glycosylated proteins with the same polypeptide backbone. Deglycosylation with Endo‐H further revealed that sAC75 and sAC85 carry distinct sugar chains. We observed release of N‐linked glycosylated sAC (sACEV) in extracellular vesicles under conditions that support intracellular sAC85 (glucose‐sufficient) as opposed to sAC75 (glucose‐deprived) conditions. Consistently, disrupting the vesicular machinery affects the maturation of intracellular sAC and inhibits the release of sACEV into extracellular vesicles. The intracellular turnover of sAC85 is extremely short (t1/2 ~30 min) and release of sACEV in the medium was detected within 3 h. Our observations support the maturation and trafficking in cholangiocytes of an N‐linked glycosylated sAC isoform that is rapidly released into extracellular vesicles. [ABSTRACT FROM AUTHOR]

Published

2023

27. A Widespread Glycosidase Confers Lobophorin Resistance and Host‐Dependent Structural Diversity.

Author

Tan, Bin, Zhang, Liping, Zhang, Qingbo, Chen, Siqiang, Xiong, Weiliang, Zhu, Yiguang, and Zhang, Changsheng

Subjects

*GLYCOSIDASES, *DRUG resistance in bacteria, *NATURAL products, *DEGLYCOSYLATION, *CRYSTAL structure, *ACTINOBACTERIA

Abstract

Identifying new environmental resistance determinants is significant to combat rising antibiotic resistance. Herein we report the unexpected correlation of a lobophorin (LOB) resistance‐related glycosidase KijX with the host‐dependent chemical diversity of LOBs, by a process of glycosylation, deglycosylation and reglycosylation. KijX homologues are widespread among bacteria, archaea and fungi, and encode the same glycohydrolytic activity on LOBs. The crystal structure of AcvX (a KijX homologue) shows a similar fold to that of the glycoside hydrolase family 113 and a special negatively charged groove to accommodate and deglycosylate LOBs. Antagonistic assays indicate kijX as a defense weapon of actinomycetes to combat LOB producers in environment, reflecting an elegant coevolution relationship. Our study provides insight into the KijX‐related glycosidases as preexisting resistance determinants and represents an example of resistance genes accidentally integrated into natural product assembly. [ABSTRACT FROM AUTHOR]

Published

2023

28. Progress in the Detection of Erythropoietin in Blood, Urine, and Tissue.

Author

Yasuoka, Yukiko, Izumi, Yuichiro, Sands, Jeff M., Kawahara, Katsumasa, and Nonoguchi, Hiroshi

Subjects

*ERYTHROPOIETIN, *ISOELECTRIC focusing, *WESTERN immunoblotting, *MASS spectrometry, *URINE, *IMMUNOGLOBULINS

Abstract

Detection of erythropoietin (Epo) was difficult until a method was developed by the World Anti-Doping Agency (WADA). WADA recommended the Western blot technique using isoelectric focusing (IEF)-PAGE to show that natural Epo and injected erythropoiesis-stimulating agents (ESAs) appear in different pH areas. Next, they used sodium N-lauroylsarcosinate (SAR)-PAGE for better differentiation of pegylated proteins, such as epoetin β pegol. Although WADA has recommended the use of pre-purification of samples, we developed a simple Western blotting method without pre-purification of samples. Instead of pre-purification, we used deglycosylation of samples before SDS-PAGE. The double detection of glycosylated and deglycosylated Epo bands increases the reliability of the detection of Epo protein. All of the endogenous Epo and exogenous ESAs shift to 22 kDa, except for Peg-bound epoetin β pegol. All endogenous Epo and exogenous ESAs were detected as 22 kDa deglycosylated Epo by liquid chromatography/mass spectrum (LC/MS) analysis. The most important factor for the detection of Epo is the selection of the antibody against Epo. WADA recommended clone AE7A5, and we used sc-9620. Both antibodies are useful for the detection of Epo protein by Western blotting. [ABSTRACT FROM AUTHOR]

Published

2023

29. The Clinical Significance of Deglycosylated PD-L1 Level Detection Using 28-8 Monoclonal Antibody in Lung Adenocarcinoma

Author

Wang H, Gu D, Chen D, Mei J, Yang X, Ding J, Xu J, Wang M, Liu C, and Hua D

Subjects

programmed death ligand 1, deglycosylation, lung adenocarcinoma, mutation, survival, Medicine (General), R5-920

Abstract

Huiyu Wang,1,&ast; Dingyi Gu,1,&ast; Datian Chen,2,&ast; Jie Mei,1 Xuejing Yang,1 Junli Ding,1 Junying Xu,1 Meilin Wang,3 Chaoying Liu,1 Dong Hua1 1Comprehensive Cancer Center, The Affiliated Wuxi People’s Hospital of Nanjing Medical University, Wuxi, 214023, People’s Republic of China; 2Department of Oncology, Haimen People’s Hospital Affiliated to Nantong University, Haimen, 226100, People’s Republic of China; 3The School of Public Health, Nanjing Medical University, Nanjing, 210000, People’s Republic of China&ast;These authors contributed equally to this workCorrespondence: Meilin Wang; Chaoying Liu, Email meilin_wang210@126.com; liuchaoying666@163.comPurpose: The aim of this study was to explore the clinical significance of deglycosylated PD-L1 level and its correlation with EGFR and ALK mutation in lung adenocarcinoma.Materials and Methods: We estimated the intensity of both native and deglycosylated PD-L1 signals using a 28– 8 antibody on lung adenocarcinoma tissue microarray sections. We analyzed the difference in the H-score between tumor and paratumor tissues, as well as that before and after deglycosylation. Correlations between EGFR or ALK status and PD-L1 expression were analyzed. We also evaluated the differences among survival curves.Results: The expression level of PD-L1 in lung adenocarcinoma tissues was significantly higher than that in paratumor tissues (P< 0.0001). Deglycosylation significantly enhanced the detection of PD-L1 in tumor tissues (P< 0.0001). There was no statistical significance between the signal intensity of deglycosylated PD-L1 and the survival of patients (P=0.9099). However, the response to deglycosylation of PD-L1 was significantly correlated with the survival of patients with stage N1-N3 (P=0.0435) and stage T3-T4 (P=0.0366) and male patients (P=0.0258). A statistical trend was found in the correlation between the response to deglycosylation of PD-L1 and the survival of patients with grade II–III plus grade III (P=0.0973). Correlation between EGFR or ALK status and the expression of PD-L1 was not found (P> 0.05).Conclusion: PD-L1 deglycosylation enhances the detection of PD-L1 when utilizing a 28– 8 antibody. Moreover, the response to deglycosylation of PD-L1 may predict the survival of certain patients with lung adenocarcinoma.Keywords: programmed death ligand 1, deglycosylation, lung adenocarcinoma, mutation, survival

Published

2022

30. Do I Need to Trypsin Digest Before Releasing IgG Glycans With PNGase-F?

Author

Birx, Lily, Popov, Marla, and Orlando, Ron

Published

2023

31. Mechanism of antibody-specific deglycosylation and immune evasion by Streptococcal IgG-specific endoglycosidases.

Author

Trastoy, Beatriz, Du, Jonathan J., Cifuente, Javier O., Rudolph, Lorena, García-Alija, Mikel, Klontz, Erik H., Deredge, Daniel, Sultana, Nazneen, Huynh, Chau G., Flowers, Maria W., Li, Chao, Sastre, Diego E., Wang, Lai-Xi, Corzana, Francisco, Mallagaray, Alvaro, Sundberg, Eric J., and Guerin, Marcelo E.

Subjects

ENDOGLYCOSIDASES, SMALL-angle X-ray scattering, DEGLYCOSYLATION, MOLECULAR dynamics, NUCLEAR magnetic resonance, FC receptors, GLYCANS, POLYKETIDE synthases

Abstract

Bacterial pathogens have evolved intricate mechanisms to evade the human immune system, including the production of immunomodulatory enzymes. Streptococcus pyogenes serotypes secrete two multi-modular endo-β-N-acetylglucosaminidases, EndoS and EndoS2, that specifically deglycosylate the conserved N-glycan at Asn297 on IgG Fc, disabling antibody-mediated effector functions. Amongst thousands of known carbohydrate-active enzymes, EndoS and EndoS2 represent just a handful of enzymes that are specific to the protein portion of the glycoprotein substrate, not just the glycan component. Here, we present the cryoEM structure of EndoS in complex with the IgG1 Fc fragment. In combination with small-angle X-ray scattering, alanine scanning mutagenesis, hydrolytic activity measurements, enzyme kinetics, nuclear magnetic resonance and molecular dynamics analyses, we establish the mechanisms of recognition and specific deglycosylation of IgG antibodies by EndoS and EndoS2. Our results provide a rational basis from which to engineer novel enzymes with antibody and glycan selectivity for clinical and biotechnological applications. Bacterial pathogens have evolved intricate mechanisms to evade the human immune system, including the production of immunomodulatory enzymes. Here, the authors establish the mechanisms of recognition and specific deglycosylation of IgG antibodies by the multi-modular enzymes EndoS and EndoS2 [ABSTRACT FROM AUTHOR]

Published

2023

32. Evaluation of agricultural wastes as a sustainable carbon source for the production of β-glucosidase from Bacillus stercoris, its purification and characterization.

Author

Ur Rahman, Ubaid, Qasim, Salma, Zada, Numan Saleh, Ahmad, Sohail, Shah, Aamer Ali, Badshah, Malik, Hasan, Fariha, and Khan, Samiullah

Subjects

*AGRICULTURAL wastes, *GLUCOSIDASES, *BACILLUS (Bacteria), *WHEAT bran, *ORANGE peel, *AMMONIUM sulfate

Abstract

β-glucosidases are found in all domains of life and has the ability to hydrolyse the glycosidic bond between carbohydrates and non-carbohydrates residues making it a potent enzyme from an industrial and agricultural perspective. The aim of the current study was isolation, screening, and identification of bacterial strains having maximum β-glucosidase activity from soil sample of Jacobabad, Pakistan. The isolates were screened primarily, and efficient isolates were confirmed for β-glucosidase production through secondary screening. Among the different isolated strains, 1j2 was selected as the best β-glucosidase producer. The isolate showed 99% similarity with Bacillus stercoris after 16S rRNA sequencing. Different culture conditions were optimized for effective β-glucosidase production. Enhanced level of β-glucosidase was achieved at 40°C, pH 8 at 150 rpm in a β-glucosidase production medium supplemented with a combination of agricultural residues of wheat bran 0.25% (w/v) and orange peel 0.25% (w/v), using 5% inoculum. Bacillus stercoris produced a higher yield (2.89U/mg) of β-glucosidase under optimized conditions. Partial purification of β-glucosidase was achieved after 80% ammonium sulfate precipitation. The enzyme was purified and had shown maximum specific activity of 53.2 U/mg with molecular weight of approximately 36 kDa. In all the tested metals Cu2+ was observed to have inhibitory effect while Ca2+ had not affected the enzyme activity significantly. While organic solvents and surfactants had significantly reduced the β-glucosidase activity. Based on the afore mentioned abilities of purified β-glucosidase from Bacillus stercoris strain it could be a promising player for the industrial applications of lignocellulose hydrolysis found in agricultural residues for the cheap production of biofuels. [ABSTRACT FROM AUTHOR]

Published

2023

33. Deglycosylation Differentially Regulates Weaned Porcine Gut Alkaline Phosphatase Isoform Functionality along the Longitudinal Axis.

Author

Yin, Xindi, Wang, Weijun, Seah, Stephen Y. K., Mine, Yoshinori, and Fan, Ming Z.

Subjects

DEGLYCOSYLATION, GROWTH disorders, LARGE intestine, PEPTIDES, GUT microbiome, AFFINITY chromatography, ALKALINE phosphatase, ENZYME kinetics, GLYCOSIDASES

Abstract

Gut alkaline phosphatases (AP) dephosphorylate the lipid moiety of endotoxin and other pathogen-associated-molecular patterns members, thus maintaining gut eubiosis and preventing metabolic endotoxemia. Early weaned pigs experience gut dysbiosis, enteric diseases and growth retardation in association with decreased intestinal AP functionality. However, the role of glycosylation in modulation of the weaned porcine gut AP functionality is unclear. Herein three different research approaches were taken to investigate how deglycosylation affected weaned porcine gut AP activity kinetics. In the first approach, weaned porcine jejunal AP isoform (IAP) was fractionated by the fast protein-liquid chromatography and purified IAP fractions were kinetically characterized to be the higher-affinity and lower-capacity glycosylated mature IAP (p < 0.05) in comparison with the lower-affinity and higher-capacity non-glycosylated pre-mature IAP. The second approach enzyme activity kinetic analyses showed that N-deglycosylation of AP by the peptide N-glycosidase-F enzyme reduced (p < 0.05) the IAP maximal activity in the jejunum and ileum and decreased AP affinity (p < 0.05) in the large intestine. In the third approach, the porcine IAP isoform-X1 (IAPX1) gene was overexpressed in the prokaryotic ClearColiBL21 (DE3) cell and the recombinant porcine IAPX1 was associated with reduced (p < 0.05) enzyme affinity and maximal enzyme activity. Therefore, levels of glycosylation can modulate plasticity of weaned porcine gut AP functionality towards maintaining gut microbiome and the whole-body physiological status. [ABSTRACT FROM AUTHOR]

Published

2023

34. Enhanced antibody-defucosylation capability of α-L-fucosidase by proximity-based protein fusion.

Author

Fan, Shuquan, Li, Wanzhen, Zhang, Kuixing, Zou, Xiangman, Shi, Wei, Liu, Zhi, Tang, Caihong, Huang, Wei, and Tang, Feng

Subjects

*CHIMERIC proteins, *LACTOBACILLUS casei, *CATALYTIC domains, *IMMUNOGLOBULIN G, *ENZYMES, *DEGLYCOSYLATION

Abstract

Up to date, the reported fucosidases generally show poor activities toward the IgG core-fucose, which limits the efficiency of ENGase-catalyzed glycoengineering process. However, EndoS or EndoS2 owns excellent activity and great selectivity towards the N-glycosylation of IgGs, and their non-catalytic domains are deduced to have specific interactions to IgG Fc domain that result in the great activity and selectivity. Herein, we constructed a series fusion protein of AlfC (an α- l -fucosidase from Lactobacillus casei BL23) with EndoS/S2 non-catalytic domain by replacing the catalytic GH (glycan hydrolase) domain of EndoS/S2 with the AlfC. We found that all these fused AlfCs showed significantly enhanced defucosylation activity toward the deglycosylated IgGs (Fucα1,6GlcNAc-IgG). We also performed the kinetic study of these fusion enzymes, and our results tend to tell that the EndoS-based fusion proteins have higher k cat values while the EndoS2-based ones possess lower K m values other than higher k cat. Conclusively, our research provides an effective approach to improve the activity of AlfC and remarkably shortened the defucosylation process within several minutes, which will significantly promote the development of glycoengineered antibodies in the future. A series of robust IgG specific fucosidases were developed by constructing the fusion protein of AlfC and non-catalytic domain of EndoS/S2, which could accomplish the deglycosylation and defucosylation of wild-type IgG within 10 min together with ENGase. [Display omitted] • A series of novel fucosidase fusion proteins were developed. • Fused AlfCs possess higher k cat and/or lower Km than that of WT to IgG. • Fused AlfCs could defucosylate IgG within 10 min with EndoS. [ABSTRACT FROM AUTHOR]

Published

2023

35. Differential enzymatic deglycosylation reveals attachment of red cell B antigen onto the carbohydrate moiety of glycophorin A and glycophorin B.

Author

Hsu, Kate

Subjects

*ERYTHROCYTES, *B cells, *ERYTHROCYTE membranes, *DEGLYCOSYLATION, *MOIETIES (Chemistry)

Abstract

Background and Objectives: Early studies indicate that red cell A and B antigens are attached primarily onto band 3 and GLUT1 on the erythrocyte membrane and little onto glycophorin A (GPA) and glycophorin B (GPB). But as GPA and band 3 form stable protein complexes and GPA is much more heavily glycosylated than band 3, this study re‐examined the association between ABO antigens and GPA/GPB. Materials and Methods: Band 3/GPA‐associated protein complexes were first immunoprecipitated, followed by differential enzymatic deglycosylation that removed sialic acids, N‐glycans and O‐glycans. Serological anti‐A (BIRMA 1) and anti‐B IgM (GAMA 110) could be used for western blot (WB); however, only the anti‐B IgM showed significant reactivity for the immunoprecipitates isolated by anti‐band 3. The expression of the B antigen in un‐deglycosylated and differentially deglycosylated band 3 immunoprecipitates was thus compared. Results: Besides attachment to band 3, red cell B antigen expressed substantially on GPA monomer and homodimer, GPA*GPB heterodimer, and GPB monomer and dimer via attachments through the N‐ and O‐glycans. Conclusion: Immunoprecipitation (IP), as a means of protein separation and concentration, was used in combination with a WB to differentiate glycosylation on different proteins and oligomers. This study implemented differential enzymatic deglycosylation during IP of the band 3 complexes. This combined approach allowed separate identification of the B antigen on GPA/GPB monomer and dimer and GPA*GPB heterodimer, and band 3 on the WB and verified non‐trivial expression of the B antigen on GPA and GPB on the erythrocyte surface. [ABSTRACT FROM AUTHOR]

Published

2023

36. Development of QM/MM (ABEEM polarizable force field) method to simulate the excision reaction mechanism of damaged cytosine.

Author

Liu, Cui, Ren, Yang, Gao, Xiao‐qin, Du, Xue, and Yang, Zhong‐zhi

Subjects

*CYTOSINE, *ACTIVATION energy, *CHEMICAL bonds, *DNA damage, *DEGLYCOSYLATION, *CHARGE transfer

Abstract

DNA damages are regarded as having harmful effects on cell. The base excision repair mechanism combats these effects by removing damaged bases. The deglycosylation mechanism of excising damaged bases by DNA glycosylase and the state of the leaving base have been controversial. The enzymatic reaction of DNA glycosylase to remove the damaged bases involves not only the formation and breaking of chemical bonds, but also complex polarization effect and charge transfer, which cannot be accurately simulated by the QM/MM method combined with the fixed charge force field. This work has developed the ABEEM fluctuating polarizable force field combining with the QM method, that is (QM/MM[ABEEM]), to accurately simulate the proton transfer, charge transfer and the charge distribution. The piecewise function is used as the valence‐state electronegativity in the QM/MM (ABEEM) to realize the accurate fitting of the charge distribution in reaction. And the charge transfer is accurately simulated by the local charge conservation conditions. Four deglycosylation mechanisms including the monofunctional and difunctional mechanisms of four neutral and protonated cytosine derivatives are explored. It is confirmed that the monofunctional mechanism of Asp‐activated nucleophile water is a better deglycosylation mechanism and the base is protonated before the reaction occurs. Protonization of the base reduced the activation energy by 10.00–17.00 kcal/mol. Asp provides the necessary charge for the reaction, and DNA glycosylase preferentially cleaves ɛC. This work provides a theoretical basis for the research of excising damaged bases by DNA glycosylase. [ABSTRACT FROM AUTHOR]

Published

2022

37. Lowering effect of combined sweet potato and onion intake on plasma quercetin concentration and underlying mechanism involving intestinal β-glucosidase activity.

Author

Nuka, Erika, Takahashi, Masako, Okitsu, Masami, Nayama, Chisako, Nishijima, Honomi, Sogawa, Ryutaro, Kawabata, Kyuichi, Terao, Junji, and Mukai, Rie

Subjects

*QUERCETIN, *SWEET potatoes, *ONIONS, *INTESTINES, *GLUCOSIDES, *SACCHARIDES, *DEGLYCOSYLATION

Abstract

A combined intake of cooked sweet potato and fried onion in humans was found to suppress the increase of plasma quercetin metabolite concentration. Experiments using rat β-glucosidase indicated that excess carbohydrate digestion products, especially glucose-containing saccharides, interfere with the deglycosylation of quercetin glucosides during intestinal epithelial uptake. Combined meals of sweet potato and onion may lower the bioavailability of onion quercetin glucosides. [ABSTRACT FROM AUTHOR]

Published

2022

38. Chemical or enzymatic deglycosylation and germination abrogates the inhibitory activity of Cyamopsis tetragonoloba trypsin inhibitor.

Author

Patidar, Preeti, Bhayal, Mamta, Hajela, Sumati, and Hajela, Krishnan

Abstract

A glycosylated heat stable trypsin chymotrypsin inhibitor was isolated from Cyamopsis tetragonoloba seeds. It is being reported for the first time that deglycosylation of the inhibitor chemically by Trifluoro methane sulfonic acid or enzymatically by salivary amylase or fungal diastase abrogates the inhibitory activity indicating that glycosylation was important for inhibitory activity of the protein. Treatment with salivary amylase decreases the inhibition in in vitro digestion experiment also. Germination of Cyamopsis tetragonoloba seeds results in reduction in inhibitory activity with concomitant increase in amylase activity. It is speculated that increase in amylase during germination decreases the protease inhibitory activity by deglycosylating the inhibitor. [ABSTRACT FROM AUTHOR]

Published

2022

39. PNGase H + variant from Rudaea cellulosilytica with improved deglycosylation efficiency for rapid analysis of eukaryotic N‐glycans and hydrogen deuterium exchange mass spectrometry analysis of glycoproteins.

Author

Guo, Rui‐Rui, Zhang, Tian‐Chan, Lambert, Thomas Ole Tandrup, Wang, Ting, Voglmeir, Josef, Rand, Kasper D., and Liu, Li

Subjects

*GLYCOPROTEIN analysis, *DEUTERIUM, *LIQUID chromatography-mass spectrometry, *DEGLYCOSYLATION, *PEPTIDE mass fingerprinting, *HORSERADISH peroxidase, *GLYCOPROTEINS

Abstract

The analysis of glycoproteins and the comparison of protein N‐glycosylation from different eukaryotic origins require unbiased and robust analytical workflows. The structural and functional analysis of vertebrate protein N‐glycosylation currently depends extensively on bacterial peptide‐N4‐(N‐acetyl‐β‐glucosaminyl) asparagine amidases (PNGases), which are indispensable enzymatic tools in releasing asparagine‐linked oligosaccharides (N‐glycans) from glycoproteins. So far, only limited PNGase candidates are available for N‐glycans analysis, and particularly the analysis of plant and invertebrate N‐glycans is hampered by the lack of suitable PNGases. Furthermore, liquid chromatography–mass spectrometry (LC–MS) workflows, such as hydrogen deuterium exchange mass spectrometry (HDX‐MS), require a highly efficient enzymatic release of N‐glycans at low pH values to facilitate the comprehensive structural analysis of glycoproteins. Herein, we describe a previously unstudied superacidic bacterial N‐glycanase (PNGase H+) originating from the soil bacterium Rudaea cellulosilytica (Rc), which has significantly improved enzymatic properties compared to previously described PNGase H+ variants. Active and soluble recombinant PNGase Rc was expressed at a higher protein level (3.8‐fold) and with higher specific activity (~56% increase) compared to the currently used PNGase H+ variant from Dyella japonicum (Dj). Recombinant PNGase Rc was able to deglycosylate the glycoproteins horseradish peroxidase and bovine lactoferrin significantly faster than PNGase Dj (10 min vs. 6 h). The versatility of PNGase Rc was demonstrated by releasing N‐glycans from a diverse array of samples such as peach fruit, king trumpet mushroom, mouse serum, and the soil nematode Caenorhabditis elegans. The presence of only two disulfide bonds shown in the AlphaFold protein model (so far all other superacidic PNGases possess more disulfide bonds) could be corroborated by intact mass‐ and peptide mapping analysis and provides a possible explanation for the improved recombinant expression yield of PNGase Rc. [ABSTRACT FROM AUTHOR]

Published

2022

40. Deglycosylation Increases the Aggregation and Angiogenic Properties of Mutant Tissue Inhibitor of Metalloproteinase 3 Protein: Implications for Sorsby Fundus Dystrophy.

Author

Qi, Jian Hua and Anand-Apte, Bela

Subjects

*PRESENILINS, *VASCULAR endothelial growth factors, *MUTANT proteins, *DYSTROPHY, *DEGLYCOSYLATION, *ENDOTHELIAL cells

Abstract

Sorsby fundus dystrophy (SFD) is an autosomal dominant macular disorder caused by mutations in tissue Inhibitor of the metalloproteinase-3 (TIMP3) gene with the onset of symptoms including choroidal neovascularization as early as the second decade of life. We have previously reported that wild-type TIMP3 is an endogenous angiogenesis inhibitor that inhibits Vascular Endothelial Growth Factor (VEGF)-mediated signaling in endothelial cells. In contrast, SFD-related S179C-TIMP3 when expressed in endothelial cells, does not have angiogenesis-inhibitory properties. To evaluate if this is a common feature of TIMP3 mutants associated with SFD, we examined and compared endothelial cells expressing S179C, Y191C and S204C TIMP3 mutants for their angiogenesis-inhibitory function. Western blot analysis, zymography and reverse zymography and migration assays were utilized to evaluate TIMP3 protein, Matrix Metalloproteinase (MMP) and MMP inhibitory activity, VEGF signaling and in vitro migration in endothelial cells expressing (VEGF receptor-2 (VEGFR-2) and wild-type TIMP3 or mutant-TIMP3. We demonstrate that mutant S179C, Y191C- and S204C-TIMP3 all show increased glycosylation and multimerization/aggregation of the TIMP3 protein. In addition, endothelial cells expressing TIMP3 mutations show increased angiogenic activities and elevated VEGFR-2. Removal of N-glycosylation by mutation of Asn184, the only potential N-glycosylation site in mutant TIMP3, resulted in increased aggregation of TIMP3, further upregulation of VEGFR-2, VEGF-induced phosphorylation of VEGFR2 and VEGF-mediated migration concomitant with reduced MMP inhibitory activity. These results suggest that even though mutant TIMP3 proteins are more glycosylated, post-translational deglycosylation may play a critical role in the aggregation of mutant TIMP3 and contribute to the pathogenesis of SFD. The identification of factors that might contribute to changes in the glycome of patients with SFD will be useful. Future studies will evaluate whether variations in the glycosylation of mutant TIMP3 proteins are contributing to the severity of the disease. [ABSTRACT FROM AUTHOR]

Published

2022

41. Anti-Inflammatory Activity of Biotransformed Platycodon grandiflorum Root Extracts Containing 3- O -β-D-Glucopyranosyl Platycosides in LPS-Stimulated Alveolar Macrophages, NR8383 Cells.

Author

Choi JW, Choi HJ, Na CS, Lee H, Lee BJ, Shin KC, and Jeong JB

Subjects

Animals, Rats, Cell Line, NF-kappa B metabolism, Nitric Oxide Synthase Type II metabolism, Nitric Oxide Synthase Type II genetics, Biotransformation, Heme Oxygenase-1 metabolism, Heme Oxygenase-1 genetics, Aspergillus niger drug effects, Saponins pharmacology, Saponins metabolism, Cytokines metabolism, Signal Transduction drug effects, Tumor Necrosis Factor-alpha metabolism, Platycodon chemistry, Lipopolysaccharides pharmacology, Anti-Inflammatory Agents pharmacology, Macrophages, Alveolar drug effects, Macrophages, Alveolar metabolism, Plant Extracts pharmacology, Plant Roots chemistry, Acute Lung Injury drug therapy, Acute Lung Injury metabolism, Nitric Oxide metabolism, NF-E2-Related Factor 2 metabolism

Abstract

Acute lung injury (ALI) is a severe inflammatory condition characterized by excessive immune responses and oxidative stress, leading to significant tissue damage. Given the need for novel therapeutic agents, this study aimed to explore the anti-inflammatory activity and mechanisms of biotransformed Platycodon grandiflorum root extracts (BT-PGR), which were enzymatically processed using rapidsase PL Classic from Aspergillus niger . The goal was to assess the potential of BT-PGR as a natural treatment for ALI. BT-PGR effectively inhibited the production of NO, iNOS, IL-1β, IL-6, and TNF-α induced by LPS in NR8383 cells. BT-PGR inhibited the phosphorylation of ERK1/2, p38, JNK and p65 in LPS-stimulated NR8383 cells. In addition, BT-PGR suppressed LPS-mediated activation of NF-κB luciferase activity. BT-PGR increased the levels of HO-1 and the inhibition of HO-1 by ZnPP attenuated BT-PGR-mediated inhibition of NO production. In addition, the inhibition of PI3K by LY294002 blocked the BT-PGR-mediated increase of HO-1 level. BT-PGR increased nuclear Nrf2 level and the knockdown of Nrf2 by siRNA inhibited BT-PGR-mediated increase of HO-1 level. In addition, inhibition of PI3K by LY294002 suppressed the increase of nuclear Nrf2 level. Based on these results, it can be inferred that BT-PGR exhibits anti-inflammatory activity in rat alveolar macrophages, suggesting its potential as a natural candidate for the improvement of ALI.

Published

2024

42. Production of Taxifolin from Astilbin by Fungal Biotransformation.

Author

Mei, Jianfeng, Chen, Xiang, Wang, Pingya, Wu, Yichun, Yi, Yu, and Ying, Guoqing

Subjects

*BIOCONVERSION, *ASPERGILLUS fumigatus, *WOOD, *FOOD additives, *DEGLYCOSYLATION

Abstract

Taxifolin is known to have multiple biological functions. It has been widely used as a multifunctional food additive, and consequently, the global demand for taxifolin is increasing. The main method for taxifolin production is an extraction from larch wood, but the global resources of larch are limited. Astilbin, taxifolin-3-o-rhamnoside, is abundant in many plants and much more readily available, meaning taxifolin can be obtained by deglycosylation of astilbin. In this study, a fungal strain, Aspergillus fumigatus SQH4, was isolated from an enrichment culture of Smilax glabra rhizome to achieve the deglycosylation reaction. A culture of SQH4, adjusted to pH 6.5, with 5 g/L astilbin achieved a yield of taxifolin of 91.3% after biotransformation for 14 h at 35 °C. These findings offer an alternative method for the production of taxifolin. [ABSTRACT FROM AUTHOR]

Published

2022

43. Deglycosylation of pathological specimens alters performance of diagnostic PDL1 antibodies.

Author

Dressler, Franz F., Dabadghao, Devang S., Klapper, Luise, Perner, Sven, Idel, Christian, and Ribbat-Idel, Julika

Abstract

Immunohistochemical (IHC) predictive quantitation of PDL1 expression is obligatory in many cancer entities with improved response to immune checkpoint inhibition in PDL1-positive subgroups. With recent demonstration of increased positivity rates after enzymatic deglycosylation in breast cancer specimens, a comparative analysis with two different antibodies and extended controls was performed in a cohort of head and neck squamous cell cancer samples (HNSCC). Formalin-fixed paraffin-embedded tissue from HNSCC specimens was used for initial on-slide method optimization based on the PNGase F assay. SDS-PAGE and immunoblotting with the PDL1 antibody 28–8 was performed to evaluate deglycosylation efficiency. A tissue micro array of n = 527 tissue cores of 181 patients with HNSCC was used to determine the effects of deglycosylation on staining pattern and intensity with PDL1 antibodies 28–8 and E1L3N. Successful on-slide deglycosylation with PNGase F was confirmed by immunoblot but varied across replicates. Using E1L3N (intracellular binding domain, most probably not glycosylated), mean signal intensity as well as the fraction of PDL1 positive cells was increased by deglycosylation. Opposite effects were observed with 28–8 (extracellular binding domain, glycosylated). Deglycosylation reduces diagnostic performance of the PDL1 antibody 28–8. In contrast, effects for E1L3N are complex and probably involve reduction of off-target binding leading to specifically improved signal intensity. However, enzymatic deglycosylation adds further variance to IHC. [ABSTRACT FROM AUTHOR]

Published

2022

44. Anticipating the unexpected.

Author

Chappell, Joe

Subjects

*DEGLYCOSYLATION, *BOMBS, *MUSTARD

Abstract

This article is a Commentary on Lacchini et al. (2023), 239: 705–719. [ABSTRACT FROM AUTHOR]

Published

2023

45. Audiologic follow up results of child with NGLY1 deficiency.

Author

Gundogdu, Ogulcan, Yeral, Cem, Yilmaz, Oguz, and Bayazit, Yildirim Ahmet

Subjects

*AUDITORY neuropathy, *DEGLYCOSYLATION, *DEAFNESS, *EPILEPSY, *MOVEMENT disorders

Abstract

NGLY1 deficiency is a rare in which affected individuals show developmental delay/intellectual disability in the mild to profound range, epilepsy, auditory neuropathy, abnormal liver function, complex hyperkinetic movement disorder and poor growth. Here, we present the follow-up results of hearing status in a patient with NGLY1 deficiency. [ABSTRACT FROM AUTHOR]

Published

2023

46. Prospective phenotyping of NGLY1-CDDG, the first congenital disorder of deglycosylation

Author

Lam, Christina, Ferreira, Carlos, Krasnewich, Donna, Toro, Camilo, Latham, Lea, Zein, Wadih M, Lehky, Tanya, Brewer, Carmen, Baker, Eva H, Thurm, Audrey, Farmer, Cristan A, Rosenzweig, Sergio D, Lyons, Jonathan J, Schreiber, John M, Gropman, Andrea, Lingala, Shilpa, Ghany, Marc G, Solomon, Beth, Macnamara, Ellen, Davids, Mariska, Stratakis, Constantine A, Kimonis, Virginia, Gahl, William A, and Wolfe, Lynne

Subjects

Biological Sciences, Genetics, Neurosciences, Eye Disease and Disorders of Vision, Clinical Research, Clinical Trials and Supportive Activities, Adolescent, Adult, Albumins, Cerebrospinal Fluid Proteins, Child, Child, Preschool, Developmental Disabilities, Female, Glycoproteins, Glycosylation, Humans, Male, Mutation, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, Phenotype, Young Adult, deglycosylation, glycosylation, natural history, NGLY1, NGLY1-CDDG, Clinical Sciences, Genetics & Heredity

Abstract

PurposeThe cytosolic enzyme N-glycanase 1, encoded by NGLY1, catalyzes cleavage of the β-aspartyl glycosylamine bond of N-linked glycoproteins, releasing intact N-glycans from proteins bound for degradation. In this study, we describe the clinical spectrum of NGLY1 deficiency (NGLY1-CDDG).MethodsProspective natural history protocol.ResultsIn 12 individuals ages 2 to 21 years with confirmed, biallelic, pathogenic NGLY1 mutations, we identified previously unreported clinical features, including optic atrophy and retinal pigmentary changes/cone dystrophy, delayed bone age, joint hypermobility, and lower than predicted resting energy expenditure. Novel laboratory findings include low cerebral spinal fluid (CSF) total protein and albumin and unusually high antibody titers toward rubella and/or rubeola following vaccination. We also confirmed and further quantified previously reported findings noting that decreased tear production, transient transaminitis, small feet, a complex hyperkinetic movement disorder, and varying degrees of global developmental delay with relatively preserved socialization are the most consistent features.ConclusionOur prospective phenotyping expands the clinical spectrum of NGLY1-CDDG, offers prognostic information, and provides baseline data for evaluating therapeutic interventions.Genet Med 19 2, 160-168.

Published

2017

47. A newly isolated human intestinal strain deglycosylating flavonoid C-glycosides.

Author

Wang, Sha, Liu, Siqi, Wang, Jing, Tao, Jiayue, Wu, Mengjiao, Ma, Wenfu, and Wang, Rufeng

Abstract

Glycosidic bond of C-glycosides is difficult to be broken due to its chemical stability. Screening specific microbe from microbiota is a practical way to deglycosylate these compounds. In this study, a new strain W974-1 which is capable of cleaving C-glycosidic bonds was isolated from human gut microbiota by spread plate method. It deglycosylates flavonoid 8-C-glycosides such as orientin and vitexin to their aglycones with the enzymes secreted outside the bacterial cells. This strain was identified as Enterococcus avium by 16S rDNA sequencing, physiological and biochemical characterization. [ABSTRACT FROM AUTHOR]

Published

2022

48. Mechanism-Based Pharmacokinetic Model for the Deglycosylation Kinetics of 20(S)-Ginsenosides Rh2.

Author

Ren, Hong-can, Sun, Jian-guo, A, Ji-ye, Gu, Sheng-hua, Shi, Jian, Shao, Feng, Ai, Hua, Zhang, Jing-wei, Peng, Ying, Yan, Bei, Huang, Qing, Liu, Lin-sheng, Sai, Yang, Wang, Guang-ji, and Yang, Cheng-guang

Subjects

DEGLYCOSYLATION, PHARMACOKINETICS, ANTINEOPLASTIC agents

Abstract

Aim: The 20(S)-ginsenoside Rh2 (Rh2) is being developed as a new antitumor drug. However, to date, little is known about the kinetics of its deglycosylation metabolite (protopanoxadiol) (PPD) following Rh2 administration. The aim of this work was to 1) simultaneously characterise the pharmacokinetics of Rh2 and PPD following intravenous and oral Rh2 administration, 2) develop and validate a mechanism-based pharmacokinetic model to describe the deglycosylation kinetics and 3) predict the percentage of Rh2 entering the systemic circulation in PPD form. Methods: Plasma samples were collected from rats after the I.V. or P.O. administration of Rh2. The plasma Rh2 and PPD concentrations were determined using HPLC-MS. The transformation from Rh2 to PPD, its absorption, and elimination were integrated into the mechanism based pharmacokinetic model to describe the pharmacokinetics of Rh2 and PPD simultaneously at 10 mg/kg. The concentration data collected following a 20 mg/kg dose of Rh2 was used for model validation. Results: Following Rh2 administration, PPD exhibited high exposure and atypical double peaks. The model described the abnormal kinetics well and was further validated using external data. A total of 11% of the administered Rh2 was predicted to be transformed into PPD and enter the systemic circulation after I.V. administration, and a total of 20% of Rh2 was predicted to be absorbed into the systemic circulation in PPD form after P.O. administration of Rh2. Conclusion: The developed model provides a useful tool to quantitatively study the deglycosylation kinetics of Rh2 and thus, provides a valuable resource for future pharmacokinetic studies of glycosides with similar deglycosylation metabolism. [ABSTRACT FROM AUTHOR]

Published

2022

49. Mechanism-Based Pharmacokinetic Model for the Deglycosylation Kinetics of 20(S)-Ginsenosides Rh2

Author

Hong-can Ren, Jian-guo Sun, Ji-ye A, Sheng-hua Gu, Jian Shi, Feng Shao, Hua Ai, Jing-wei Zhang, Ying Peng, Bei Yan, Qing Huang, Lin-sheng Liu, Yang Sai, Guang-ji Wang, and Cheng-guang Yang

Subjects

traditional Chinese medicine, ginsenosides, pharmacokinetics, deglycosylation, modelling and simulation, Therapeutics. Pharmacology, RM1-950

Abstract

Aim: The 20(S)-ginsenoside Rh2 (Rh2) is being developed as a new antitumor drug. However, to date, little is known about the kinetics of its deglycosylation metabolite (protopanoxadiol) (PPD) following Rh2 administration. The aim of this work was to 1) simultaneously characterise the pharmacokinetics of Rh2 and PPD following intravenous and oral Rh2 administration, 2) develop and validate a mechanism-based pharmacokinetic model to describe the deglycosylation kinetics and 3) predict the percentage of Rh2 entering the systemic circulation in PPD form.Methods: Plasma samples were collected from rats after the I.V. or P.O. administration of Rh2. The plasma Rh2 and PPD concentrations were determined using HPLC-MS. The transformation from Rh2 to PPD, its absorption, and elimination were integrated into the mechanism based pharmacokinetic model to describe the pharmacokinetics of Rh2 and PPD simultaneously at 10 mg/kg. The concentration data collected following a 20 mg/kg dose of Rh2 was used for model validation.Results: Following Rh2 administration, PPD exhibited high exposure and atypical double peaks. The model described the abnormal kinetics well and was further validated using external data. A total of 11% of the administered Rh2 was predicted to be transformed into PPD and enter the systemic circulation after I.V. administration, and a total of 20% of Rh2 was predicted to be absorbed into the systemic circulation in PPD form after P.O. administration of Rh2.Conclusion: The developed model provides a useful tool to quantitatively study the deglycosylation kinetics of Rh2 and thus, provides a valuable resource for future pharmacokinetic studies of glycosides with similar deglycosylation metabolism.

Published

2022

50. Flavone, flavanone and flavonol metabolism from soybean and flaxseed extracts by the intestinal microbiota of adults and infants.

Subjects

*FLAXSEED, *GUT microbiome, *ISOFLAVONES, *SOYBEAN, *LUTEOLIN, *CHEMICAL industry, *INFANTS, *FLAVONES

Abstract

BACKGROUND: Flaxseed and soybean are an important source of lignans and flavonoids. Previously, the metabolism of isoflavones and lignans from soybean and flaxseed extracts by the microbiota of adult individuals (n = 14) and infants (n = 23) was analyzed. Thus, the present study aimed to examine the metabolism of flavones, flavanones and flavonols, as well as the production of phenolic acids, by the intestinal microbiota of these individuals. RESULTS: Concentrations of aglycones of flavonoids, such as herbacetin, quercetin, quercetagetin, myricetin, kaempferol, apigenin and luteolin, increased for most of individuals as a consequence of deglycosylation reactions. On the other hand, a diminution in the antioxidant activity and phenolic compound concentration and an increase in the concentration of 3,4‐dihydroxyphenylacetic acid, 2‐(4‐hydroxyphenyl)‐propionic acid, protocatechuic acid and catechol was also observed. CONCLUSION: The present study found that deglycosylation reactions were the main reactions and accelerated the formation of more bioavailable flavonoids, with greater biological activity, in most of the individuals. However, other reactions also occurred, including the total or partial catabolism of flavonoids. © 2021 Society of Chemical Industry. [ABSTRACT FROM AUTHOR]

Published

2022