Your search keyword '"Boopathy Ramakrishnan"' showing total 66 results

1. Applications of site-specific labeling to study HAMLET, a tumoricidal complex of α-lactalbumin and oleic acid.

Author

Natalia Mercer, Boopathy Ramakrishnan, Elizabeth Boeggeman, and Pradman K Qasba

Subjects

Medicine, Science

Abstract

Alpha-lactalbumin (α-LA) is a calcium-bound mammary gland-specific protein that is found in milk. This protein is a modulator of β1,4-galactosyltransferase enzyme, changing its acceptor specificity from N-acetyl-glucosamine to glucose, to produce lactose, milk's main carbohydrate. When calcium is removed from α-LA, it adopts a molten globule form, and this form, interestingly, when complexed with oleic acid (OA) acquires tumoricidal activity. Such a complex made from human α-LA (hLA) is known as HAMLET (Human A-lactalbumin Made Lethal to Tumor cells), and its tumoricidal activity has been well established.In the present work, we have used site-specific labeling, a technique previously developed in our laboratory, to label HAMLET with biotin, or a fluoroprobe for confocal microscopy studies. In addition to full length hLA, the α-domain of hLA (αD-hLA) alone is also included in the present study. We have engineered these proteins with a 17-amino acid C-terminal extension (hLA-ext and αD-hLA-ext). A single Thr residue in this extension is glycosylated with 2-acetonyl-galactose (C2-keto-galactose) using polypeptide-α-N-acetylgalactosaminyltransferase II (ppGalNAc-T2) and further conjugated with aminooxy-derivatives of fluoroprobe or biotin molecules.We found that the molten globule form of hLA and αD-hLA proteins, with or without C-terminal extension, and with and without the conjugated fluoroprobe or biotin molecule, readily form a complex with OA and exhibits tumoricidal activity similar to HAMLET made with full-length hLA protein. The confocal microscopy studies with fluoroprobe-labeled samples show that these proteins are internalized into the cells and found even in the nucleus only when they are complexed with OA. The HAMLET conjugated with a single biotin molecule will be a useful tool to identify the cellular components that are involved with it in the tumoricidal activity.

Published

2011

2. A Proliferation Inducing Ligand (APRIL) targeted antibody is a safe and effective treatment of murine IgA nephropathy

Author

Andrew M. Wollacott, Hitoshi Suzuki, Ketan D. Deotale, Zachary Shriver, Toshiki Kano, Frank Engler, Yusuke Suzuki, Boopathy Ramakrishnan, James R. Myette, Brian J.G. Pereira, Kristy J. Szretter, Hedy Adari, and Susan Sloan

Subjects

Male, 0301 basic medicine, medicine.drug_class, Injections, Subcutaneous, Tumor Necrosis Factor Ligand Superfamily Member 13, Population, Drug Evaluation, Preclinical, 030232 urology & nephrology, Antigen-Antibody Complex, Antibodies, Monoclonal, Humanized, Monoclonal antibody, Models, Biological, Epitope, Nephropathy, Pathogenesis, Mice, 03 medical and health sciences, 0302 clinical medicine, Immune system, medicine, Animals, Humans, Computer Simulation, education, Autoimmune disease, B-Lymphocytes, education.field_of_study, biology, business.industry, Glomerulonephritis, IGA, medicine.disease, Immunoglobulin A, Disease Models, Animal, Macaca fascicularis, 030104 developmental biology, Nephrology, Injections, Intravenous, Immunology, biology.protein, Epitopes, B-Lymphocyte, Female, Antibody, business

Abstract

IgA nephropathy (IgAN) is the most prevalent primary chronic glomerular disease for which no safe disease-specific therapies currently exist. IgAN is an autoimmune disease involving the production of autoantigenic, aberrantly O-glycosylated IgA1 and ensuing deposition of nephritogenic immune complexes in the kidney. A Proliferation Inducing Ligand (APRIL) has emerged as a key B-cell–modulating factor in this pathogenesis. Using a mouse anti-APRIL monoclonal antibody (4540), we confirm both the pathogenic role of APRIL in IgAN and the therapeutic efficacy of antibody-directed neutralization of APRIL in the grouped mouse ddY disease model. Treatment with 4540 directly translated to a reduction in relevant pathogenic mechanisms including suppressed serum IgA levels, reduced circulating immune complexes, significantly lower kidney deposits of IgA, IgG and C3, and suppression of proteinuria compared to mice receiving vehicle or isotype control antibodies. Furthermore, we translated these findings to the pharmacological characterization of VIS649, a highly potent, humanized IgG2κ antibody targeting and neutralizing human APRIL through unique epitope engagement, leading to inhibition of APRIL-mediated B-cell activities. VIS649 treatment of non-human primates showed dose-dependent reduction of serum IgA levels of up to 70%. A reduction of IgA+, IgM+, and IgG+ B cells was noted in the gut-associated mucosa of VIS649-treated animals. Population-based modeling predicted a favorable therapeutic dosing profile for subcutaneous administration of VIS649 in the clinical setting. Thus, our data highlight the potential therapeutic benefit of VIS649 for the treatment of IgAN.

Published

2019

3. Characterization of an Antibody Recognizing the Conserved Inner Core of

Author

Stefano, Elli, Anna, Alekseeva, Boopathy, Ramakrishnan, Tyree, Koch, Andrew, Wollacott, Karthik, Viswanathan, Kai, Li, James C, Delaney, Zachary, Shriver, Obadiah, Plante, and Marco, Guerrini

Subjects

Lipopolysaccharides, Epitopes, Polysaccharides, Pseudomonas aeruginosa, Pseudomonas Infections, Antibodies, Bacterial

Abstract

Bacterial infections are a growing public health threat with carbapenem-resistant

Published

2020

4. VIS832, a novel CD138-targeting monoclonal antibody, potently induces killing of human multiple myeloma and further synergizes with IMiDs or bortezomib in vitro and in vivo

Author

Yan Xu, Phillip A Hsieh, Gang An, Hedy Adari, Kenneth C. Anderson, Yuyin Li, Zachary Shriver, Kenneth Wen, Lijie Xing, Lugui Qiu, Gregory J. Babcock, James R. Myette, Liang Lin, Andrew M. Wollacott, Bharat Chaganty, Boopathy Ramakrishnan, Hailin Chen, Wenjuan Yang, Karthik Viswanathan, Nikhil C. Munshi, Shih-Feng Cho, Yu-Tzu Tai, and Tengteng Yu

Subjects

Indatuximab ravtansine, Immunoconjugates, medicine.drug_class, Mice, SCID, Monoclonal antibody, lcsh:RC254-282, Article, Bortezomib, Mice, Antineoplastic Agents, Immunological, Targeted therapies, Antigen, In vivo, immune system diseases, hemic and lymphatic diseases, Cell Line, Tumor, medicine, Animals, Humans, Maytansine, Multiple myeloma, Lenalidomide, Cancer, business.industry, Daratumumab, Drug Synergism, Hematology, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, medicine.disease, Xenograft Model Antitumor Assays, Neoplasm Proteins, Oncology, Cancer research, Syndecan-1, business, Multiple Myeloma, medicine.drug

Abstract

Therapeutically targeting CD138, a define multiple myeloma (MM) antigen, is not yet approved for patients. We here developed and determined the preclinical efficacy of VIS832, a novel therapeutic monoclonal antibody (MoAb) with differentiated CD138 target binding to BB4 that is anti-CD138 MoAb scaffold for indatuximab ravtansine (BT062). VIS832 demonstrated enhanced CD138-binding avidity and significantly improved potency to kill MM cell lines and autologous patient MM cells regardless of resistance to current standard-of-care therapies, via robust antibody-dependent cellular cytotoxicity and phagocytosis mediated by NK and macrophage effector cells, respectively. Specifically, CD38-targeting daratumumab-resistant MM cells were highly susceptible to VIS832 which, unlike daratumumab, spares NK cells. Superior maximal cytolysis of VIS832 vs. daratumumab corresponded to higher CD138 vs. CD38 levels in MM cells. Furthermore, VIS832 acted synergistically with lenalidomide or bortezomib to deplete MM cells. Importantly, VIS832 at a sub-optimal dose inhibited disseminated MM1S tumors in vivo as monotherapy (P

Published

2020

5. First Photographic Evidence of Occurrence of Indian Pangolin Manis crassicaudata at its Highest Elevation Limit in Nilgiris, Tamil Nadu, India

Author

Boopathy Ramakrishnan, R. Deepan, A. Samson, A Cleamant Kiran Kumar, and R. Logeshvarma

Subjects

Veterinary medicine, Geography, biology, Tamil, Pangolin, language, Elevation, Limit (mathematics), biology.organism_classification, Manis crassicaudata, language.human_language

Published

2020

6. Extending human IgG half-life using structure-guided design

Author

Zachary Shriver, Brian J. Booth, Boopathy Ramakrishnan, Kristin Narayan, Karthik Viswanathan, Andrew M. Wollacott, and Gregory J. Babcock

Subjects

0301 basic medicine, Genetically modified mouse, half-life, Immunology, Antibody Affinity, Mice, Transgenic, Receptors, Fc, Biology, Protein Engineering, effector functions, Cell Line, 03 medical and health sciences, Mice, Structure-Activity Relationship, Neonatal Fc receptor, Pharmacokinetics, Allosteric Regulation, Report, Immunology and Allergy, Animals, Humans, Gene Regulatory Networks, Effector functions, Antibody, B-Lymphocytes, neonatal Fc receptor, Protein Stability, Antibody-Dependent Cell Cytotoxicity, Half-life, Molecular biology, FcRn, Macaca fascicularis, 030104 developmental biology, Immunoglobulin G, Mutation, biology.protein, pharmacokinetics, structure-guided engineering, amino acid interaction network, Protein Binding, Signal Transduction

Abstract

Engineering of antibodies for improved pharmacokinetics through enhanced binding to the neonatal Fc receptor (FcRn) has been demonstrated in transgenic mice, non-human primates and humans. Traditionally, such approaches have largely relied on random mutagenesis and display formats, which fail to address related critical attributes of the antibody, such as effector functions or biophysical stability. We have developed a structure- and network-based framework to interrogate the engagement of IgG with multiple Fc receptors (FcRn, C1q, TRIM21, FcγRI, FcγRIIa/b, FcγRIIIa) simultaneously. Using this framework, we identified features that govern Fc-FcRn interactions and identified multiple distinct pathways for enhancing FcRn binding in a pH-specific manner. Network analysis provided a novel lens to study the allosteric impact of half-life-enhancing Fc mutations on FcγR engagement, which occurs distal to the FcRn binding site. Applying these principles, we engineered a panel of unique Fc variants that enhance FcRn binding while maintaining robust biophysical properties and wild type-like binding to activating receptors. An antibody harboring representative Fc designs demonstrates a half-life improvement of > 9 fold in transgenic mice and > 3.5 fold in cynomolgus monkeys, and maintains robust effector functions such as antibody-dependent cell-mediated cytotoxicity and complement-dependent cytotoxicity.

Published

2018

7. A Novel CD138-Targeting Monoclonal Antibody Induces Potent Myeloma Killing and Further Synergizes with IMiDs or Bortezomib in in Vitro and In Vivo Preclinical Models of Human Multiple Myeloma

Author

Andrew M. Wollacott, Yan Xu, Hailin Chen, Boopathy Ramakrishnan, Liang Lin, Nikhil C. Munshi, Shih-Feng Cho, Lugui Qiu, Wenjuan Yang, Lijie Xing, Hedy Adari, Gang An, Karthik Viswanathan, Phillip A Hsieh, Yu-Tzu Tai, Tengteng Yu, Gregory J. Babcock, Zach Shriver, Kenneth Wen, Bharat Chaganty, Yuyin Li, James R. Myette, and Kenneth C. Anderson

Subjects

Oncology, Antibody-dependent cell-mediated cytotoxicity, medicine.medical_specialty, Bortezomib, medicine.drug_class, business.industry, Immunology, Daratumumab, Cell Biology, Hematology, Monoclonal antibody, medicine.disease, Pomalidomide, Biochemistry, medicine.anatomical_structure, Internal medicine, medicine, Bone marrow, business, Multiple myeloma, medicine.drug, Lenalidomide

Abstract

Immunotherapeutically targeting CD138 has not been successfully translated into substantial clinical benefit in multiple myeloma (MM) patients. We here developed and determined in preclinical models of human MM the efficacy of VIS832, a novel humanized monoclonal antibody (MoAb) with differentiated CD138 target binding to the anti-CD138 MoAb BB4 within indatuximab ravtansine (BT082). Compared with BB4, VIS832 has significantly improved binding (P8). In the reporter-based antibody-dependent cellular cytotoxicity (ADCC) bioassay, EC50 of VIS832 was approximately 99.31 ng/ml (0.66 nM), whereas the BB4 possessing an isotype matched human IgG1 minimally induced ADCC against U266 MM cells. Evaluation of VIS832-induced ADCC in NK-MM cell co-cultures determined its EC50 values ranged from 2.22 + 0.37 to 15.3 + 2.71 ng/ml, with % maximal lysis of 37.06 + 1.45 % to 97.3 + 3.34 %, across tested MM cell lines (n=12), both sensitive or resistant to current therapies including dexamethasone, IMiDs, and bortezomib. While VIS832 effectively induced ADCC against parental cells with high and low CD138 levels, no lysis was detected in paired CD138-knockout MM cells. In the presence of BM stromal cells or osteoclasts, two key MM-supporting accessory cells in the BM milieu, VIS832-induced MM cytolysis was minimally affected. Importantly, VIS832 eliminated autologous MM cells of bone marrow (BM) samples from relapsed/refractory (RRMM) patients, with > 60% maximal lysis and > 90% killing in 4 out of 7 patient BM samples. EC50 values of VIS832 were 8.58-86.04 ng/ml in this patient cohort, comparable to those (17.28-179.3 ng/ml) of its non-humanized predecessor mAb 2810 against another RRMM patient cohort (n=6). In contrast to its potent autologous CD138+ patient cell lysis, VIS832 did not affect CD138-negative patient BM cells. VIS832 induced higher maximal lysis (~3-fold) of all target MM cell lines than CD38-targeting daratumumab (dara), regardless of resistance to lenalidomide and pomalidomide. These results also confirmed significantly higher CD138 vs CD38 levels in all MM cell lines and patient MM cells (P60 days (P Disclosures Chaganty: Visterra Inc: Current Employment. Ramakrishnan:Visterra Inc: Current Employment. Wollacott:Visterra Inc: Current Employment. Viswanathan:Visterra Inc: Current Employment. Adari:Visterra Inc: Current Employment. Munshi:Karyopharm: Consultancy; Amgen: Consultancy; Legend: Consultancy; Adaptive: Consultancy; Janssen: Consultancy; C4: Current equity holder in private company; OncoPep: Consultancy, Current equity holder in private company, Membership on an entity's Board of Directors or advisory committees, Patents & Royalties; BMS: Consultancy; Takeda: Consultancy; AbbVie: Consultancy. Babcock:Visterra Inc: Current Employment. Shriver:Visterra Inc: Current Employment. Myette:Visterra Inc: Current Employment. Anderson:Celgene: Membership on an entity's Board of Directors or advisory committees; Millenium-Takeda: Membership on an entity's Board of Directors or advisory committees; Gilead: Membership on an entity's Board of Directors or advisory committees; Oncopep and C4 Therapeutics.: Other: Scientific Founder of Oncopep and C4 Therapeutics.; Bristol Myers Squibb: Membership on an entity's Board of Directors or advisory committees; Sanofi-Aventis: Membership on an entity's Board of Directors or advisory committees; Janssen: Membership on an entity's Board of Directors or advisory committees.

Published

2020

8. Structure-Guided Design of an Anti-dengue Antibody Directed to a Non-immunodominant Epitope

Author

Tyree Koch, David Cain, Chong Wai Liew, Hamid Tissire, James R. Myette, Jianzhu Chen, Zachary Shriver, Gregory J. Babcock, Yee Hwa Wong, Julien Lescar, Sylvie Alonso, Rama Sanjay Kirloskar, Vivian Vasconcelos Costa, Kuan Rong Chan, Eng Eong Ooi, Luke Robinson, Kirk J. Rowley, Boopathy Ramakrishnan, Li Ching Ong, Viswanathan Sasisekharan, Ram Sasisekharan, Hwee Cheng Tan, Karthik Viswanathan, Kannan Tharakaraman, Harvard University--MIT Division of Health Sciences and Technology, Massachusetts Institute of Technology. Department of Biological Engineering, Massachusetts Institute of Technology. Department of Biology, Koch Institute for Integrative Cancer Research at MIT, Robinson, Luke Nathaniel, Cain, David Joseph, Kirloskar, Rama Sanjay, Sasisekharan, Viswanathan, Chen, Jianzhu, and Sasisekharan, Ram

Subjects

Models, Molecular, Viral protein, Molecular Sequence Data, Viremia, Receptors, Fc, Protein Engineering, medicine.disease_cause, Article, General Biochemistry, Genetics and Molecular Biology, Epitope, Dengue fever, Dengue, Mice, Immune system, Phagocytosis, medicine, Animals, Amino Acid Sequence, biology, Biochemistry, Genetics and Molecular Biology(all), Immunodominant Epitopes, Dengue Virus, medicine.disease, Antibodies, Neutralizing, Virology, 3. Good health, Disease Models, Animal, Immunology, Humanized mouse, biology.protein, Viral disease, Antibody, Sequence Alignment

Abstract

Dengue is the most common vector-borne viral disease, causing nearly 400 million infections yearly. Currently there are no approved therapies. Antibody epitopes that elicit weak humoral responses may not be accessible by conventional B cell panning methods. To demonstrate an alternative strategy to generating a therapeutic antibody, we employed a non-immunodominant, but functionally relevant, epitope in domain III of the E protein, and engineered by structure-guided methods an antibody directed to it. The resulting antibody, Ab513, exhibits high-affinity binding to, and broadly neutralizes, multiple genotypes within all four serotypes. To assess therapeutic relevance of Ab513, activity against important human clinical features of dengue was investigated. Ab513 mitigates thrombocytopenia in a humanized mouse model, resolves vascular leakage, reduces viremia to nearly undetectable levels, and protects mice in a maternal transfer model of lethal antibody-mediated enhancement. The results demonstrate that Ab513 may reduce the public health burden from dengue., National Institutes of Health (U.S.) (NIH Award (1R01AI111395)), National Institute of Environmental Health Sciences (NIEHS training grant (2T32ES007020)), National Institutes of Health (U.S.) (NIH Merit Award (R37 GM057073-13)), National Science Foundation (U.S.)

Published

2015

9. Structural prediction of antibody-APRIL complexes by computational docking constrained by antigen saturation mutagenesis library data

Author

Andrew M. Wollacott, Karthik Viswanathan, Zachary Shriver, Luke Robinson, Gregory J. Babcock, Hamid Tissire, and Boopathy Ramakrishnan

Subjects

Models, Molecular, Computer science, Tumor Necrosis Factor Ligand Superfamily Member 13, Antigen-Antibody Complex, Computational biology, Crystallography, X-Ray, 010402 general chemistry, 01 natural sciences, Epitopes, Antigen, Structural Biology, Humans, Saturated mutagenesis, Molecular Biology, Gene Library, Binding Sites, biology, Cryoelectron Microscopy, 010401 analytical chemistry, Disease progression, 0104 chemical sciences, Molecular Docking Simulation, Workflow, Epitope mapping, Docking (molecular), Mutation, biology.protein, Experimental methods, Antibody, Protein Binding

Abstract

IgA nephropathy (IgAN) is the most prevalent cause of primary glomerular disease worldwide, and the cytokine A PRoliferation-Inducing Ligand (APRIL) is emerging as a key player in IgAN pathogenesis and disease progression. For a panel of anti-human APRIL antibodies with known antagonistic activity, we sought to define their structural mode of engagement to understand molecular mechanisms of action and aid rational antibody engineering. Reliable computational prediction of antibody-antigen complexes remains challenging, and experimental methods such as X-ray co-crystallography and cryoEM have considerable technical, resource, and throughput barriers. To overcome these limitations, we implemented an integrated and accessible experimental-computational workflow to more accurately predict structures of antibody-APRIL complexes. Specifically, a yeast surface display library encoding site-saturation mutagenized surface positions of APRIL was screened against a panel of anti-APRIL antibodies to rapidly obtain a comprehensive biochemical profile of mutational impact on binding for each antibody. The experimentally derived mutational profile data were used as quantitative constraints in a computational docking workflow optimized for antibodies, resulting in robust structural models of antibody-antigen complexes. The model results were confirmed by solving the cocrystal structure of one antibody-APRIL complex, which revealed strong agreement with our model. The models were used to rationally select and engineer one antibody for cross-species APRIL binding, which quite often aids further testing in relevant animal models. Collectively, we demonstrate a rapid, integrated computational-experimental approach to robustly predict antibody-antigen structures information, which can aid rational antibody engineering and provide insights into molecular mechanisms of action.

Published

2019

10. Crystal Structures of β-1,4-Galactosyltransferase 7 Enzyme Reveal Conformational Changes and Substrate Binding

Author

Boopathy Ramakrishnan, Yuko Tsutsui, and Pradman K. Qasba

Subjects

Stereochemistry, Mutation, Missense, Glycobiology and Extracellular Matrices, Xylose, Crystallography, X-Ray, Biochemistry, Uridine Diphosphate Galactose, Hydrophobic effect, Structure-Activity Relationship, chemistry.chemical_compound, Protein structure, Xylobiose, Animals, Drosophila Proteins, Humans, Moiety, Molecular Biology, Ternary complex, Binding Sites, Chemistry, Substrate (chemistry), Hydrogen Bonding, Cell Biology, Galactosyltransferases, Acceptor, carbohydrates (lipids), Crystallography, Drosophila melanogaster, Amino Acid Substitution, Protein Binding

Abstract

The β-1,4-galactosyltransferase 7 (β4GalT7) enzyme is involved in proteoglycan synthesis. In the presence of a manganese ion, it transfers galactose from UDP-galactose to xylose on a proteoglycan acceptor substrate. We present here the crystal structures of human β4GalT7 in open and closed conformations. A comparison of these crystal structures shows that, upon manganese and UDP or UDP-Gal binding, the enzyme undergoes conformational changes involving a small and a long loop. We also present the crystal structures of Drosophila wild-type β4GalT7 and D211N β4GalT7 mutant enzymes in the closed conformation in the presence of the acceptor substrate xylobiose and the donor substrate UDP-Gal, respectively. To understand the catalytic mechanism, we have crystallized the ternary complex of D211N β4GalT7 mutant enzyme in the presence of manganese with the donor and the acceptor substrates together in the same crystal structure. The galactose moiety of the bound UDP-Gal molecule forms seven hydrogen bonds with the protein molecule. The nonreducing end of the xylose moiety of xylobiose binds to the hydrophobic acceptor sugar binding pocket created by the conformational changes, whereas its extended xylose moiety forms hydrophobic interactions with a Tyr residue. In the ternary complex crystal structure, the nucleophile O4 oxygen atom of the xylose molecule is found in close proximity to the C1 and O5 atoms of the galactose moiety. This is the first time that a Michaelis complex of a glycosyltransferase has been described, and it clearly suggests an SN2 type catalytic mechanism for the β4GalT7 enzyme.

Published

2013

11. A Structural and Mathematical Modeling Analysis of the Likelihood of Antibody Dependent Enhancement in Influenza

Author

Rahul Raman, Boopathy Ramakrishnan, Zachary Shriver, Kannan Tharakaraman, Gregory J. Babcock, Karthik Viswanathan, Vlado Dančík, Ram Sasisekharan, Massachusetts Institute of Technology. Department of Biological Engineering, Tharakaraman, Kannan, Raman, Rahul, and Sasisekharan, Ram

Subjects

0301 basic medicine, Microbiology (medical), Models, Molecular, medicine.drug_class, viruses, 030106 microbiology, Hemagglutinin (influenza), Context (language use), Viremia, Monoclonal antibody, Antibodies, Viral, Microbiology, Models, Biological, Virus, Article, Dengue fever, Dengue, 03 medical and health sciences, Epitopes, Virology, Influenza, Human, medicine, Humans, Antibody-dependent enhancement, biology, virus diseases, Antibodies, Monoclonal, medicine.disease, Antibodies, Neutralizing, Antibody-Dependent Enhancement, 030104 developmental biology, Infectious Diseases, Virus Diseases, Immunology, biology.protein, Antibody

Abstract

Broadly neutralizing monoclonal antibodies (bNAbs) for viral infections, such as HIV, respiratory syncytial virus (RSV), and influenza, are increasingly entering clinical development. For influenza, most neutralizing antibodies target influenza virus hemagglutinin. These bNAbs represent an emerging, promising modality for treatment and prophylaxis of influenza due to their multiple mechanisms of antiviral action and generally safe profile. Preclinical work in other viral diseases, such as dengue, has demonstrated the potential for antibody-based therapies to enhance viral uptake, leading to enhanced viremia and worsening of disease. This phenomenon is referred to as antibody-dependent enhancement (ADE). In the context of influenza, ADE has been used to explain several preclinical and clinical phenomena. Using structural and viral kinetics modeling, we assess the role of ADE in the treatment of influenza with a bNAb., National Institutes of Health (U.S.) (Merit Award R37 GM057073-13), National Institutes of Health (U.S.) (Grant RO1 AI111395-03)

Published

2016

12. The N-acetyl-binding pocket of N-acetylglucosaminyltransferases also accommodates a sugar analog with a chemical handle at C2

Author

Elizabeth Boeggeman, Andrés E. Dulcey, Marta Pasek, Gary L. Griffiths, Natalia Mercer, Boopathy Ramakrishnan, and Pradman K. Qasba

Subjects

Models, Molecular, Glycosylation, Surface Properties, Stereochemistry, Recombinant Fusion Proteins, Molecular Sequence Data, Oligosaccharides, N-Acetylglucosaminyltransferases, Biochemistry, Chromatography, Affinity, Acetylglucosamine, chemistry.chemical_compound, Glycosyltransferase, Carbohydrate Conformation, Escherichia coli, Humans, Moiety, Cloning, Molecular, Binding site, Binding Sites, biology, Intracellular Signaling Peptides and Proteins, Galactose, Membrane Proteins, Substrate (chemistry), Hydrogen Bonding, Original Articles, Factor VII, Acceptor, carbohydrates (lipids), Amino Acid Substitution, Carbohydrate Sequence, Hexosyltransferases, chemistry, Glucosyltransferases, biology.protein, Mutant Proteins, lipids (amino acids, peptides, and proteins), Carbohydrate conformation, Hydrophobic and Hydrophilic Interactions, Protein Binding

Abstract

In recent years, sugars with a unique chemical handle have been used to detect and elucidate the function of glycoconjugates. Such chemical handles have generally been part of an N-acetyl moiety of a sugar. We have previously developed several applications using the single mutant Y289L-β1,4-galactosyltransferase I (Y289L-β4Gal-T1) and the wild-type polypeptide-α-GalNAc-T enzymes with UDP-C2-keto-Gal. Here, we describe for the first time that the GlcNAc-transferring enzymes-R228K-Y289L-β4Gal-T1 mutant enzyme, the wild-type human β1,3-N-acetylglucosaminyltransferase-2 and human Maniac Fringe-can also transfer the GlcNAc analog C2-keto-Glc molecule from UDP-C2-keto-Glc to their respective acceptor substrates. Although the R228K-Y289L-β4Gal-T1 mutant enzyme transfers the donor sugar substrate GlcNAc or its analog C2-keto-Glc only to its natural acceptor substrate, GlcNAc, it does not transfer to its analog C2-keto-Glc. Thus, these observations suggest that the GlcNAc-transferring glycosyltransferases can generally accommodate a chemical handle in the N-acetyl-binding cavity of the donor sugar substrate, but not in the N-acetyl-binding cavity of the acceptor sugar.

Published

2011

13. Crystal Structure of the Catalytic Domain of Drosophila β1,4-Galactosyltransferase-7

Author

Boopathy Ramakrishnan and Pradman K. Qasba

Subjects

Models, Molecular, Glycosylation, Protein Conformation, Stereochemistry, Molecular Sequence Data, Glycobiology and Extracellular Matrices, Crystal structure, Plasma protein binding, Xylose, Crystallography, X-Ray, Biochemistry, Uridine Diphosphate, chemistry.chemical_compound, Protein structure, Catalytic Domain, N-Acetyllactosamine Synthase, Side chain, Animals, Humans, Amino Acid Sequence, Molecular Biology, Peptide sequence, Galactosyltransferase, Manganese, Sequence Homology, Amino Acid, Chemistry, Cell Biology, Drosophila melanogaster, Protein Binding

Abstract

The beta1,4-galactosyltransferase-7 (beta4Gal-T7) enzyme, one of seven members of the beta4Gal-T family, transfers in the presence of manganese Gal from UDP-Gal to an acceptor sugar (xylose) that is attached to a side chain hydroxyl group of Ser/Thr residues of proteoglycan proteins. It exhibits the least protein sequence similarity with the other family members, including the well studied family member beta4Gal-T1, which, in the presence of manganese, transfers Gal from UDP-Gal to GlcNAc. We report here the crystal structure of the catalytic domain of beta4Gal-T7 from Drosophila in the presence of manganese and UDP at 1.81 A resolution. In the crystal structure, a new manganese ion-binding motif (HXH) has been observed. Superposition of the crystal structures of beta4Gal-T7 and beta4Gal-T1 shows that the catalytic pocket and the substrate-binding sites in these proteins are similar. Compared with GlcNAc, xylose has a hydroxyl group (instead of an N-acetyl group) at C2 and lacks the CH(2)OH group at C5; thus, these protein structures show significant differences in their acceptor-binding site. Modeling of xylose in the acceptor-binding site of the beta4Gal-T7 crystal structure shows that the aromatic side chain of Tyr(177) interacts strongly with the C5 atom of xylose, causing steric hindrance to any additional group at C5. Because Drosophila Cd7 has a 73% protein sequence similarity to human Cd7, the present crystal structure offers a structure-based explanation for the mutations in human Cd7 that have been linked to Ehlers-Danlos syndrome.

Published

2010

14. Multiple Site-Specific in Vitro Labeling of Single-Chain Antibody

Author

Kristin H. Loomis, Pradman K. Qasba, Anu Puri, Maria Manzoni, Dimiter S. Dimitrov, Elizabeth Boeggeman, Zhongyu Zhu, and Boopathy Ramakrishnan

Subjects

Models, Molecular, Protein Folding, Glycosylation, Receptor, ErbB-2, medicine.medical_treatment, Molecular Sequence Data, Biomedical Engineering, Gene Expression, Pharmaceutical Science, chemical and pharmacologic phenomena, Bioengineering, Plasma protein binding, Article, Inclusion bodies, law.invention, chemistry.chemical_compound, law, Cell Line, Tumor, Escherichia coli, medicine, Humans, Amino Acid Sequence, Threonine, Peptide sequence, Fluorescent Dyes, Pharmacology, Protease, Organic Chemistry, Antibodies, Monoclonal, respiratory system, Fusion protein, Molecular biology, Biochemistry, chemistry, Recombinant DNA, Protein Binding, Biotechnology

Abstract

For multiple site-specific conjugations of bioactive molecules to a single-chain antibody (scFv) molecule, we have constructed a human anti HER2 receptor, scFv, with a C-terminal fusion polypeptide containing 1, 3, or 17 threonine (Thr) residues. The C-terminal extended fusion polypeptides of these recombinant scFv fusion proteins are used as the acceptor substrate for human polypeptide-alpha-Nu-acetylgalactosaminyltransferase II (h-ppGalNAc-T2) that transfers either GalNAc or 2-keto-Gal, a modified galactose with a chemical handle, from their respective UDP-sugars to the side-chain hydroxyl group of the Thr residue(s). The recombinant scFv fusion proteins are expressed in E. coli as inclusion bodies and in vitro refolded and glycosylated with h-ppGalNAc-T2. Upon protease cleavage, the MALDI-TOF spectra of the glycosylated C-terminal fusion polypeptides showed that the glycosylated scFv fusion protein with a single Thr residue is fully glycosylated with a single 2-keto-Gal, whereas the glycosylated scFv fusion protein with 3 and 17 Thr residues is found as an equal mixture of 2-3 and 5-8 2-keto-Gal glycosylated fusion proteins, respectively. These fusion scFv proteins with the modified galactose are then conjugated with a fluorescence probe, Alexa488, that carries an orthogonal reactive group. The fluorescence labeled scFv proteins bind specifically to a human breast cancer cell line (SK-BR-3) that overexpresses the HER2 receptor, indicating that the in vitro folded scFv fusion proteins are biologically active and the presence of conjugated multiple Alexa488 probes in their C-terminal end does not interfere with their binding to the antigen.

Published

2009

15. Bioconjugation and Detection of Lactosamine Moiety using α1,3-Galactosyltransferase Mutants That Transfer C2-Modified Galactose with a Chemical Handle

Author

Pradman K. Qasba, Marta Pasek, Timothy J. Waybright, Maria Manzoni, Boopathy Ramakrishnan, and Elizabeth Boeggeman

Subjects

Models, Molecular, Glycan, Glycoconjugate, Stereochemistry, Molecular Sequence Data, Mutant, Biomedical Engineering, Pharmaceutical Science, Bioengineering, Article, chemistry.chemical_compound, Glycolipid, Glycosyltransferase, Animals, Humans, Moiety, Amino Acid Sequence, Trisaccharide, Pharmacology, chemistry.chemical_classification, Base Sequence, biology, Organic Chemistry, Galactose, Amino Sugars, Galactosyltransferases, carbohydrates (lipids), Kinetics, chemistry, Biochemistry, Mutation, biology.protein, Cattle, Sequence Alignment, Biotechnology

Abstract

Studies on wild-type and mutant glycosyltransferases have shown that they can transfer modified sugars with a versatile chemical handle, such as keto or azido group, that can be used for conjugation chemistry and detection of glycan residues on glycoconjugates. To detect the most prevalent glycan epitope, N-acetyllactosamine (LacNAc (Galbeta1-4GalNAcbeta)), we have mutated a bovine alpha1,3-galactosyltransferse (alpha3Gal-T)() enzyme which normally transfers Gal from UDP-Gal to the LacNAc acceptor, to transfer GalNAc or C2-modified galactose from their UDP derivatives. The alpha3Gal-T enzyme belongs to the alpha3Gal/GalNAc-T family that includes human blood group A and B glycosyltransferases, which transfer GalNAc and Gal, respectively, to the Gal moiety of the trisaccharide Fucalpha1-2Galbeta1-4GlcNAc. On the basis of the sequence and structure comparison of these enzymes, we have carried out rational mutation studies on the sugar donor-binding residues in bovine alpha3Gal-T at positions 280 to 282. A mutation of His280 to Leu/Thr/Ser/Ala or Gly and Ala281 and Ala282 to Gly resulted in the GalNAc transferase activity by the mutant alpha3Gal-T enzymes to 5-19% of their original Gal-T activity. We show that the mutants (280)SGG(282) and (280)AGG(282) with the highest GalNAc-T activity can also transfer modified sugars such as 2-keto-galactose or GalNAz from their respective UDP-sugar derivatives to LacNAc moiety present at the nonreducing end of glycans of asialofetuin, thus enabling the detection of LacNAc moiety of glycoproteins and glycolipids by a chemiluminescence method.

Published

2009

16. Deoxygenated Disaccharide Analogs as Specific Inhibitors of β1–4-Galactosyltransferase 1 and Selectin-mediated Tumor Metastasis

Author

Boopathy Ramakrishnan, Pradman K. Qasba, Jeffrey D. Esko, Jillian R. Brown, Anjana Sinha, Yitzhak Tor, and Feng Yang

Subjects

Glycan, Stereochemistry, Disaccharide, Glycobiology and Extracellular Matrices, Disaccharides, Biochemistry, Carcinoma, Lewis Lung, Mice, chemistry.chemical_compound, Glycosyltransferase, medicine, Animals, Humans, Trisaccharide, Enzyme Inhibitors, Neoplasm Metastasis, Molecular Biology, chemistry.chemical_classification, biology, Lewis lung carcinoma, U937 Cells, Cell Biology, Galactosyltransferases, Sialyl-Lewis X, Mechanism of action, chemistry, Acetylation, Selectins, biology.protein, Drug Screening Assays, Antitumor, medicine.symptom, Neoplasm Transplantation

Abstract

The disaccharide peracetylated GlcNAcbeta1-3Galbeta-O-naphthalenemethanol (disaccharide 1) diminishes the formation of the glycan sialyl Lewis X (Neu5Acalpha2-3Galbeta1-4(Fucalpha1-3) GlcNAc; sLe(X)) in tumor cells. Previous studies showed that the mechanism of action of disaccharide 1 involves three steps: (i) deacetylation by carboxyesterases, (ii) action as a biosynthetic intermediate for downstream enzymes involved in sLe(X) assembly, and (iii) generation of several glycans related to sLe(X). In this report, we show that GlcNAcbeta1-3Galbeta-O-naphthalenemethanol binds to the acceptor site of human beta1-4-galactosyltransferase much like the acceptor trisaccharide, GlcNAcbeta1-2Manbeta1-6Man, which is present on N-linked glycans. The 4'-deoxy analog, in which the acceptor hydroxyl group was replaced by -H, did not act as a substrate but instead acted as a competitive inhibitor of the enzyme. The acetylated form of this compound inhibited sLe(X) formation in U937 monocytic leukemia cells, suggesting that it had inhibitory activity in vivo as well. A series of synthetic acetylated analogs of 1 containing -H, -F, -N(3), -NH(2), or -OCH(3) instead of the hydroxyl groups at C-3'- and C-4'-positions of the terminal N-acetylglucosamine residue also blocked sLe(X) formation in cells. The reduction of sLe(X) by the 4'-deoxy analog also diminished experimental tumor metastasis by Lewis lung carcinoma in vivo. These data suggest that nonsubstrate disaccharides have therapeutic potential through their ability to bind to glycosyltransferases in vivo and to alter glycan-dependent pathologic processes.

Published

2009

17. Structure and Function of β -1,4-Galactosyltransferase

Author

Boopathy Ramakrishnan, Pradman K. Qasba, and Elizabeth Boeggeman

Subjects

Pharmacology, Conformational change, biology, Stereochemistry, Clinical Biochemistry, Metal Binding Site, chemistry.chemical_compound, Protein structure, chemistry, Drug Discovery, Glycosyltransferase, Native state, biology.protein, Molecular Medicine, Glycosyl, Binding site, Binding domain

Abstract

Beta-1,4-galactosylransferase (beta4Gal-T1) participates in the synthesis of Galbeta1-4-GlcNAc-disaccharide unit of glycoconjugates. It is a trans-Golgi glycosyltransferase (Glyco-T) with a type II membrane protein topology, a short N-terminal cytoplasmic domain, a membrane-spanning region, as well as a stem and a C-terminal catalytic domain facing the trans-Golgi-lumen. Its hydrophobic membrane-spanning region, like that of other Glyco-T, has a shorter length compared to plasma membrane proteins, an important feature for its retention in the trans-Golgi. The catalytic domain has two flexible loops, a long and a small one. The primary metal binding site is located at the N-terminal hinge region of the long flexible loop. Upon binding of metal ion and sugar-nucleotide, the flexible loops undergo a marked conformational change, from an open to a closed conformation. Conformational change simultaneously creates at the C-terminal region of the flexible loop an oligosaccharide acceptor binding site that did not exist before. The loop acts as a lid covering the bound donor substrate. After completion of the transfer of the glycosyl unit to the acceptor, the saccharide product is ejected; the loop reverts to its native conformation to release the remaining nucleotide moiety. The conformational change in beta4Gal-T1 also creates the binding site for a mammary gland-specific protein, alpha-lactalbumin (LA), which changes the acceptor specificity of the enzyme toward glucose to synthesize lactose during lactation. The specificity of the sugar donor is generally determined by a few residues in the sugar-nucleotide binding pocket of Glyco-T, conserved among the family members from different species. Mutation of these residues has allowed us to design new and novel glycosyltransferases, with broader or requisite donor and acceptor specificities, and to synthesize specific complex carbohydrates as well as specific inhibitors for these enzymes.

Published

2008

18. Applications of glycosyltransferases in the site-specific conjugation of biomolecules and the development of a targeted drug delivery system and contrast agents for MRI

Author

Pradman K. Qasba, Boopathy Ramakrishnan, and Elizabeth Boeggeman

Subjects

Drug, Glycan, media_common.quotation_subject, medicine.medical_treatment, Contrast Media, Pharmaceutical Science, Article, Drug Delivery Systems, Glycosyltransferase, medicine, Animals, Humans, Binding site, media_common, chemistry.chemical_classification, Binding Sites, biology, Biomolecule, Glycosyltransferases, Immunotherapy, Magnetic Resonance Imaging, Pharmaceutical Preparations, chemistry, Biochemistry, Targeted drug delivery, Mutation, biology.protein, Conjugate

Abstract

Background: The delivery of drugs to the proposed site of action is a challenging task. Tissue and cell-specific guiding molecules are being used to carry a cargo of therapeutic molecules. The cargo molecules need to be conjugated in a site-specific manner to the therapeutic molecules such that the bioefficacy of these molecules is not compromised. Methods: Using wild-type and mutant glycosyltransferases, the sugar moiety with a unique chemical handle is incorporated at a specific site in the cargo or therapeutic molecules, making it possible to conjugate these molecules through the chemical handle present on the modified glycan. Results/conclusions: The modified glycan residues introduced at specific sites on the cargo molecule make it possible to conjugate fluorophores for ELISA-based assays, radionuclides for imaging and immunotherapy applications, lipids for the assembly of immunoliposomes, cytotoxic drugs, cytokines, or toxins for antibody-based cancer therapy and the development of a targeted drug d...

Published

2008

19. Novel Method for in Vitro O-Glycosylation of Proteins: Application for Bioconjugation

Author

Elizabeth Boeggeman, Boopathy Ramakrishnan, and Pradman K. Qasba

Subjects

Models, Molecular, Protein Folding, Glycosylation, Molecular Sequence Data, Biomedical Engineering, Pharmaceutical Science, Bioengineering, Catalysis, chemistry.chemical_compound, Residue (chemistry), Genes, Reporter, Humans, Peptide sequence, Inclusion Bodies, Pharmacology, chemistry.chemical_classification, Bioconjugation, biology, Biomolecule, Organic Chemistry, Proteins, Lectin, chemistry, Biochemistry, Galactose, biology.protein, Protein folding, Biotechnology

Abstract

Here, we describe a new method for the bioconjugation of a nonglycoprotein with biomolecules. Using polypeptide-alpha- N-acetylgalactosaminyltransferase II (ppGalNAc-T2), we transfer a C2-modified galactose that has a chemical handle, such as ketone or azide, from its respective UDP-sugars to the Ser/Thr residue(s) of an acceptor polypeptide fused to the nonglycoprotein. The protein with the modified galactose is then coupled to a biomolecule that carries an orthogonal reactive group. As a model system for the nonglycoprotein, we engineered glutathione- S-transferase (GST) protein with a 17-amino-acid-long fusion peptide at the C-terminal end that was expressed as a soluble protein in E. coli. The ppGalNAc-T2 protein, the catalytic domain with the C-terminal lectin domain, was expressed as inclusion bodies in E. coli, and an in vitro folding method was developed to produce milligram quantities of the active enzyme from a liter of bacterial culture. This ppGalNAc-T2 enzyme transfers from the UDP-sugars not only GalNAc but also C2-modified galactose with a chemical handle to the Ser/Thr residue(s) in the fusion peptide. The chemical handle at the C2 of galactose is used for conjugation and assembly of bionanoparticles and preparation of immuno-liposomes for a targeted drug delivery system. This novel method enables one to glycosylate, using ppGalNAc-T2, the important biological nonglycoproteins, such as single-chain antibodies, growth factors, or bacterial toxins, with an engineered 17-residue peptide sequence at the C-terminus of the molecule, for conjugation and coupling.

Published

2007

20. Role of a Single Amino Acid in the Evolution of Glycans of Invertebrates and Vertebrates

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

Protein Folding, Glycan, Acetylgalactosamine, Glycoconjugate, Molecular Sequence Data, medicine.disease_cause, Article, Catalysis, Uridine Diphosphate, Evolution, Molecular, Glycolipid, Polysaccharides, Structural Biology, biology.animal, medicine, Animals, Humans, Amino Acid Sequence, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Manganese, Mutation, Sequence Homology, Amino Acid, biology, Vertebrate, myr, Galactosyltransferases, Invertebrates, Recombinant Proteins, Enzyme, Amino Acid Substitution, chemistry, Biochemistry, Vertebrates, Lactalbumin, biology.protein, N-Acetylgalactosaminyltransferases, Drosophila, Glycoconjugates

Abstract

Structures of glycoconjugate N-glycans and glycolipids of invertebrates show significant differences from those of vertebrates. These differences are due largely to the vertebrate beta1,4-galactosyltransferase-1 (beta4Gal-T1), which is found as a beta1,4-N-acetylgalactosaminyltransferase (beta4GalNAc-T1) in invertebrates. Mutation of Tyr285 to Ile or Leu in human beta4Gal-T1 converts the enzyme into an equally efficient beta4GalNAc-T1. A comparison of all the human beta4Gal-T1 ortholog enzymes shows that this Tyr285 residue in human beta4Gal-T1 is conserved either as Tyr or Phe in all vertebrate enzymes, while in all invertebrate enzymes it is conserved as an Ile or Leu. We find that mutation of the corresponding Ile residue to Tyr in Drosophila beta4GalNAc-T1 converts the enzyme to a beta4Gal-T1 by reducing its N-acetylgalactosaminyltransferase activity by nearly 1000-fold, while enhancing its galactosyltransferase activity by 80-fold. Furthermore, we find that, similar to the vertebrate/mammalian beta4Gal-T1 enzymes, the wild-type Drosophila beta4GalNAc-T1 enzyme binds to a mammary gland-specific protein, alpha-lactalbumin (alpha-LA). Thus, it would seem that, during the evolution of vertebrates from invertebrates over 500 million years ago, beta4Gal-T1 appeared as a result of the single amino acid substitution of Tyr or Phe for Leu or Ile in the invertebrate beta4GalNAc-T1. Subsequently, the pre-existing alpha-LA-binding site was utilized during mammalian evolution to synthesize lactose in the mammary gland during lactation.

Published

2007

21. Structural Snapshots of β-1,4-Galactosyltransferase-I Along the Kinetic Pathway

Author

Boopathy Ramakrishnan, Pradman K. Qasba, and Velavan Ramasamy

Subjects

Models, Molecular, Protein Conformation, Stereochemistry, Molecular Sequence Data, Oxocarbenium, Crystal structure, Crystallography, X-Ray, Uridine Diphosphate, Acetylglucosamine, Enzyme catalysis, Structural Biology, Catalytic Domain, N-Acetyllactosamine Synthase, Animals, Humans, Molecule, Moiety, Molecular Biology, Manganese, Molecular Structure, Chemistry, Hydrogen bond, Galactose, Water, carbohydrates (lipids), Catalytic cycle, Covalent bond, Cattle

Abstract

During the catalytic cycle of beta1,4-galactosyltransferase-1 (Gal-T1), upon the binding of Mn(2+) followed by UDP-Gal, two flexible loops, a long and a short loop, change their conformation from open to closed. We have determined the crystal structures of a human M340H-Gal-T1 mutant in the open conformation (apo-enzyme), its Mn(2+) and Mn(2+)-UDP-Gal-bound complexes, and of a pentenary complex of bovine Gal-T1-Mn(2+)-UDP-GalNAc-Glc-alpha-lactalbumin. These studies show that during the conformational changes in Gal-T1, the coordination of Mn(2+) undergoes significant changes. It loses a coordination bond with a water molecule bound in the open conformation of Gal-T1 while forming a new coordination bond with another water molecule in the closed conformation, creating an active ground-state structure that facilitates enzyme catalysis. In the crystal structure of the pentenary complex, the N-acetylglucosamine (GlcNAc) moiety is found cleaved from UDP-GalNAc and is placed 2.7A away from the O4 oxygen atom of the acceptor Glc molecule, yet to form the product. The anomeric C1 atom of the cleaved GalNAc moiety has only two covalent bonds with its non-hydrogen atoms (O5 and C2 atoms), similar to either an oxocarbenium ion or N-acetylgalactal form, which are crystallographically indistinguishable at the present resolution. The structure also shows that the newly formed, metal-coordinating water molecule forms a hydrogen bond with the beta-phosphate group of the cleaved UDP moiety. This hydrogen bond formation results in the rotation of the beta-phosphate group of UDP away from the cleaved GalNAc moiety, thereby preventing the re-formation of the UDP-sugar during catalysis. Therefore, this water molecule plays an important role during catalysis in ensuring that the catalytic reaction proceeds in a forward direction.

Published

2006

22. Mutation of Arginine 228 to Lysine Enhances the Glucosyltransferase Activity of Bovine β-1,4-Galactosyltransferase I

Author

Elizabeth Boeggeman, Boopathy Ramakrishnan, and Pradman K. Qasba

Subjects

Uridine Diphosphate Glucose, Steric effects, Arginine, Macromolecular Substances, Stereochemistry, Lysine, Crystallography, X-Ray, Biochemistry, Uridine Diphosphate Galactose, chemistry.chemical_compound, Side chain, Animals, Moiety, Carboxylate, Galactosyltransferase, Manganese, Wild type, Galactosyltransferases, Enzyme Activation, carbohydrates (lipids), Kinetics, chemistry, Glucosyltransferases, Lactalbumin, Mutagenesis, Site-Directed, Cattle, Crystallization

Abstract

β-1,4-Galactosyltransferase I (β4Gal-T1) normally transfers Gal from UDP-Gal to GlcNAc in the presence of Mn 2 + ion (Gal-T activity) and also transfers Glc from UDP-Glc to GlcNAc (Glc-T activity), albeit at only 0.3% efficiency. In addition, α-lactalbumin (LA) enhances this Glc-T activity more than 25 times. Comparison of the crystal structures of UDP-Gal- and UDP-Glc-bound β4Gal-T1 reveals that the 04 hydroxyl group in both Gal and Glc moieties forms a hydrogen bond with the side chain carboxylate group of Glu317. The orientation of the 04 hydroxyl of glucose causes a steric hindrance to the side chain carboxylate group of Glu317, accounting for the enzyme's low Glc-T activity. In this study, we show that mutation of Arg228, a residue in the vicinity of Glu317, to lysine (R228K-Gal-T1) results in a 15-fold higher Glc-T activity, which is further enhanced by LA to nearly 25% of the Gal-T activity of the wild type. The kinetic parameters indicate that the main effect of the mutation of Arg228 to lysine is on the k c a t of Glc-T, which increases 3-4-fold, both in the absence and in the presence of LA; simultaneously, the k c a t for the Gal-T reaction is reduced 30-fold. The crystal structure of R228K-Gal-T1 complexed with LA, UDP-Gal, and Mn 2 + determined at 1.9 A resolution shows that the Asp318 side chain exhibits a minor alternate conformation, compared to that in the wild type. This alternate conformation now causes a steric hindrance to the 04 hydroxyl group of the Gal moiety of UDP-Gal, probably causing the dissociation of UDP-Gal and the reduced k c a t of the Gal-T reaction.

Published

2005

23. Effect of the Met344His Mutation on the Conformational Dynamics of Bovine β-1,4-Galactosyltransferase: Crystal Structure of the Met344His Mutant in Complex with Chitobiose

Author

Pradman K. Qasba, Elizabeth Boeggeman, and Boopathy Ramakrishnan

Subjects

Galactosyltransferase, chemistry.chemical_classification, Conformational change, Stereochemistry, Mutant, Metal Binding Site, Chitobiose, Oligosaccharide, Biochemistry, carbohydrates (lipids), chemistry.chemical_compound, chemistry, Oligosaccharide binding, Binding site

Abstract

β-1,4-Galactosyltransferase (β4Gal-T1) in the presence of manganese ion transfers galactose from UDP-galactose (UDP-Gal) to N-acetylglucosamine (GlcNAc) that is either free or linked to an oligosaccharide. Crystallographic studies on bovine β4Gal-T1 have shown that the primary metal binding site is located in the hinge region of a long flexible loop, which upon Mn2+ and UDP-Gal binding changes from an open to a closed conformation. This conformational change creates an oligosaccharide binding site in the enzyme. Neither UDP nor UDP analogues efficiently induce these conformational changes in the wild-type enzyme, thereby restricting the structural analysis of the acceptor binding site. The binding of Mn2+ involves an uncommon coordination to the Sδ atom of Met344; when it is mutated to His, the mutant M344H, in the presence of Mn2+ and UDP-hexanolamine, readily changes to a closed conformation, facilitating the structural analysis of the enzyme bound with an oligosaccharide acceptor. Although the mutant M...

Published

2004

24. The Role of Tryptophan 314 in the Conformational Changes of β1,4-Galactosyltransferase-I

Author

Pradman K. Qasba, Boopathy Ramakrishnan, Elizabeth Boeggeman, and Velavan Ramasamy

Subjects

Models, Molecular, Macromolecular Substances, Protein Conformation, Stereochemistry, Mutant, Crystal structure, In Vitro Techniques, Crystallography, X-Ray, Cleavage (embryo), Chromatography, Affinity, Uridine Diphosphate, Acetylglucosamine, Substrate Specificity, Structural Biology, Catalytic Domain, Animals, Transferase, Molecular Biology, Galactosyltransferase, chemistry.chemical_classification, Manganese, Tryptophan, Substrate (chemistry), Galactosyltransferases, Recombinant Proteins, Crystallography, Enzyme, chemistry, Lactalbumin, Mutagenesis, Site-Directed

Abstract

beta1,4-Galactosyltransferase-I (beta4Gal-T1) undergoes critical conformational changes upon substrate binding from an open conformation (conf-I) to the closed conformation (conf-II). This change involves two flexible loops: the small (residues 313-316) and the long loop (residues 345-365). Upon substrate binding, Trp314 in the small flexible loop moves towards the catalytic pocket and interacts with the donor and the acceptor substrates. For a better understanding of the role played by Trp314 in the conformational changes of beta4Gal-T1, we mutated it to Ala and carried out substrate-binding, proteolytic and crystallographic studies. The W314A mutation reduces the enzymatic activity, binding to substrates and to the modifier protein, alpha-lactalbumin (LA), by over 99%. The limited proteolysis with Glu-C or Lys-C proteases shows differences in the rate of cleavage of the long loop of the wild-type and mutant W314A, indicating conformational differences in the region between the two proteins. Without substrate, the mutant crystallizes in a conformation (conf-I') (1.9A resolution crystal structure), that is not identical with, but close to an open conformation (conf-I), whereas its complex with the substrates and alpha-lactalbumin, crystallizes in a conformation (2.3A resolution crystal structure) that is identical with the closed conformation (conf-II). This study shows the crucial role Trp314 plays in the conformational state of the long loop, in the binding of substrates and in the catalytic mechanism of the enzyme.

Published

2003

25. Near-atomic resolution crystal structure of an A-DNA decamer d(CCCGATCGGG): cobalt hexammine interaction with A-DNA

Author

Chandra Sekharudu, Boopathy Ramakrishnan, Muttaiya Sundaralingam, and Baocheng Pan

Subjects

Models, Molecular, Guanine, Crystal structure, Crystallography, X-Ray, Ion, chemistry.chemical_compound, Tetragonal crystal system, Isomerism, Structural Biology, A-DNA, Nucleotide, chemistry.chemical_classification, Base Sequence, Hydrogen bond, Temperature, Water, Hydrogen Bonding, Cobalt, DNA, General Medicine, Organophosphates, Crystallography, Oligodeoxyribonucleotides, chemistry, Duplex (building), Nucleic Acid Conformation, Protein Binding

Abstract

The structure of the DNA decamer d(CCCGATCGGG) has been determined at 1.25 A resolution. The decamer crystallized in the tetragonal space group P4(3)2(1)2, with unit-cell parameters a = b = 44.3, c = 24.8 A and one strand in the asymmetric unit. The structure was solved by the molecular-replacement method and refined to R(work) and R(free) values of 16.3 and 18.5%, respectively, for 5969 reflections. The decamer forms the A-form DNA duplex, with the abutting crystal packing typical of A-DNA. The crystal packing interactions seem to distort the local conformation: A5 adopts the trans/trans conformation for the torsion angles alpha and gamma instead of the usual gauche(-)/gauche(+) conformations, yielding G*(G.C) base triplets. The highly hydrated [Co(NH(3))(6)](3+) ion adopts a novel binding mode to the DNA duplex, binding directly to phosphate groups and connecting to N7 and O6 atoms of guanines by water bridges. Analysis of thermal parameters (B factors) shows that the nucleotides involved in abutting crystal packing are thermally more stable than other nucleotides in the duplex.

Published

2002

26. Structure-based Design of β1,4-Galactosyltransferase I (β4Gal-T1) with Equally Efficient N-Acetylgalactosaminyltransferase Activity

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

Galactosyltransferase, Chemistry, Hydrogen bond, Stereochemistry, Mutant, Wild type, Cell Biology, Biochemistry, carbohydrates (lipids), Acetylgalactosaminyltransferase activity, Residue (chemistry), parasitic diseases, lipids (amino acids, peptides, and proteins), Steady state (chemistry), Beta (finance), Molecular Biology

Abstract

β1,4-Galactosyltransferase I (Gal-T1) normally transfers Gal from UDP-Gal to GlcNAc in the presence of Mn2+ ion. In the presence of α-lactalbumin (LA), the Gal acceptor specificity is altered from GlcNAc to Glc. Gal-T1 also transfers GalNAc from UDP-GalNAc to GlcNAc, but with only ∼0.1% of Gal-T activity. To understand this low GalNAc-transferase activity, we have carried out the crystal structure analysis of the Gal-T1·LA complex with UDP-GalNAc at 2.1-A resolution. The crystal structure reveals that the UDP-GalNAc binding to Gal-T1 is similar to the binding of UDP-Gal to Gal-T1, except for an additional hydrogen bond formed between the N-acetyl group of GalNAc moiety with the Tyr-289 side chain hydroxyl group. Elimination of this additional hydrogen bond by mutating Tyr-289 residue to Leu, Ile, or Asn enhances the GalNAc-transferase activity. Although all three mutants exhibit enhanced GalNAc-transferase activity, the mutant Y289L exhibits GalNAc-transferase activity that is nearly 100% of its Gal-T activity, even while completely retaining its Gal-T activity. The steady state kinetic analyses on the Leu-289 mutant indicate that theK m for GlcNAc has increased compared to the wild type. On the other hand, the catalytic constant (k cat) in the Gal-T reaction is comparable with the wild type, whereas it is 3–5-fold higher in the GalNAc-T reaction. Interestingly, in the presence of LA, these mutants also transfer GalNAc to Glc instead of to GlcNAc. The present study demonstrates that, in the Gal-T family, the Tyr-289/Phe-289 residue largely determines the sugar donor specificity.

Published

2002

27. Site-specific antibody-drug conjugation through an engineered glycotransferase and a chemically reactive sugar

Author

Yanping Wang, Jinyu Li, Marzena A. Dyba, Dimiter S. Dimitrov, Pradman K. Qasba, Zhongyu Zhu, Simona Colantonio, Ponraj Prabakaran, Yang Feng, and Boopathy Ramakrishnan

Subjects

Models, Molecular, Glycan, Phage display, Immunoconjugates, medicine.drug_class, Cell Survival, Receptor, ErbB-2, Immunology, Carbohydrates, Monoclonal antibody, Protein Engineering, Epitope, Antibodies, Cell Line, Tumor, medicine, Immunology and Allergy, Humans, Aminobenzoates, skin and connective tissue diseases, biology, Chemistry, Antibodies, Monoclonal, Glycosyltransferases, Small molecule, Protein Structure, Tertiary, Biochemistry, Pharmaceutical Preparations, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Cancer cell, biology.protein, MCF-7 Cells, Antibody, Oligopeptides, Conjugate, Protein Binding, Reports

Abstract

Conjugation of small molecule drugs to specific sites on the antibody molecule has been increasingly used for the generation of relatively homogenous preparations of antibody-drug conjugates (ADCs) with physicochemical properties similar or identical to those of the naked antibody. Previously a method for conjugation of small molecules to glycoproteins through existing glycans by using an engineered glycotransferase and a chemically reactive sugar as a handle was developed. Here, for the first time, we report the use of this method with some modifications to generate an ADC from a monoclonal antibody, m860, which we identified from a human naïve phage display Fab library by panning against the extracellular domain of human HER2. M860 bound to cell surface-associated HER2 with affinity comparable to that of Trastuzumab (Herceptin®), but to a different epitope. The m860ADC was generated by enzymatically adding a reactive keto-galactose to m860 using an engineered glycotransferase and conjugating the reactive m860 to aminooxy auristatin F. It exhibited potent and specific cell-killing activity against HER2 positive cancer cells, including trastuzumab-resistant breast cancer cells. This unique ADC may have utility as a potential therapeutic for HER2 positive cancers alone or in combination with other drugs. Our results also validate the keto-galactose/engineered glycotransferase method for generation of functional ADCs, which could potentially also be used for preparation of ADCs targeting other disease markers.

Published

2014

28. UDP-Gal: BetaGlcNAc Beta 1,4-Galactosyltransferase, Polypeptide 1 (B4GALT1)

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

Galactosyltransferase, Beta-1 adrenergic receptor, Biochemistry, Chemistry

Published

2014

29. Crystal structure of lactose synthase reveals a large conformational change in its catalytic component, the β1,4-galactosyltransferase-I11Edited by R. Huber

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

Galactosyltransferase, Conformational change, biology, Stereochemistry, Hydrogen bond, Lactose synthase, Substrate (chemistry), Carbohydrate, chemistry.chemical_compound, Crystallography, chemistry, Structural Biology, biology.protein, Lactose, Binding site, Molecular Biology

Abstract

The lactose synthase (LS) enzyme is a 1:1 complex of a catalytic component, β1,4-galactosyltransferse (β4Gal-T1) and a regulatory component, α-lactalbumin (LA), a mammary gland-specific protein. LA promotes the binding of glucose (Glc) to β4Gal-T1, thereby altering its sugar acceptor specificity from N-acetylglucosamine (GlcNAc) to glucose, which enables LS to synthesize lactose, the major carbohydrate component of milk. The crystal structures of LS bound with various substrates were solved at 2 A resolution. These structures reveal that upon substrate binding to β4Gal-T1, a large conformational change occurs in the region comprising residues 345 to 365. This repositions His347 in such a way that it can participate in the coordination of a metal ion, and creates a sugar and LA-binding site. At the sugar-acceptor binding site, a hydrophobic N-acetyl group-binding pocket is found, formed by residues Arg359, Phe360 and Ile363. In the Glc-bound structure, this hydrophobic pocket is absent. For the binding of Glc to LS, a reorientation of the Arg359 side-chain occurs, which blocks the hydrophobic pocket and maximizes the interactions with the Glc molecule. Thus, the role of LA is to hold Glc by hydrogen bonding with the O-1 hydroxyl group in the acceptor-binding site on β4Gal-T1, while the N-acetyl group-binding pocket in β4Gal-T1 adjusts to maximize the interactions with the Glc molecule. This study provides details of a structural basis for the partially ordered kinetic mechanism proposed for lactose synthase.

Published

2001

30. Letter to the Glyco-Forum: Catalytic domains of glycosyltransferases with ‘add-on’ domains

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

biology, Chemistry, Glycosyltransferase, biology.protein, Computational biology, Biochemistry

Published

2007

31. In vitro folding of β-1,4galactosyltransferase and polypeptide-α-N-acetylgalactosaminyltransferase from the inclusion bodies

Author

Boopathy, Ramakrishnan and Pradman K, Qasba

Subjects

Inclusion Bodies, N-Acetyllactosamine Synthase, Animals, Humans, N-Acetylgalactosaminyltransferases, Electrophoresis, Polyacrylamide Gel, Sulfones, Protein Refolding, Recombinant Proteins

Abstract

The aim of this article is to present a unique in vitro folding technique for glycosyltransferases to generate active proteins that can be used for X-ray crystallographic and bioconjugation protocols. Although a number of in vitro refolding methods are available, β1,4galactosyltransferases in large quantities can be made using the current protocol only. This technique is not only limited to glycosyltransferases alone but has been successfully used to refold single-chain antibodies and other molecules. Although this in vitro folding method is quite similar to other methods, it differs from them by the use of S-sulfonation of the inclusion bodies before setting up the in vitro refolding of the protein.

Published

2013

32. Investigations on β1,4-galactosyltransferase I using 6-sulfo-GlcNAc as an acceptor sugar substrate

Author

Tyler A. Davis, Boopathy Ramakrishnan, Lisa A. Holland, Anthony J. Moncrief, and Pradman K. Qasba

Subjects

chemistry.chemical_classification, Galactosyltransferase, Conformational change, Stereochemistry, Molecular Sequence Data, Cell Biology, Galactosyltransferases, Biochemistry, Acetylglucosamine, Substrate Specificity, chemistry.chemical_compound, Enzyme, chemistry, Catalytic cycle, Galactose, Side chain, Transferase, Moiety, Animals, Cattle, Amino Acid Sequence, Molecular Biology

Abstract

6-sulfate modified N-acetylglucosamine (6-sulfo-GlcNAc) is often found as part of many biologically important carbohydrate epitopes such as 6-sulfo-Le(X). In these epitopes, the 6-sulfo-GlcNAc moiety is extended by a galactose sugar in a β1-4 linkage. The β4GalT1 enzyme transfers galactose (Gal) from UDP-Gal to N-acetylglucosamine (GlcNAc) in the presence of manganese. Here we report that the β4GalT1 enzyme transfers Gal to the 6-sulfo-GlcNAc and 4-methylumbelliferyl-6-sulfo-N-acetyl-β-D-glucosaminide (6-sulfo-βGlcNAc-MU) acceptor substrates, although with very low efficiency. To understand the effect that the 6-sulfate group on the GlcNAc acceptor has on the catalytic activity of the β4GalT1 molecule, we have determined the crystal structure of the catalytic domain of bovine β4GalT1 mutant enzyme M344H-β4GalT1 complex with the 6-sulfo-GlcNAc molecule. In the crystal structure, the 6-sulfo-GlcNAc is bound to the protein in a way that is similar to the GlcNAc molecule. However, the 6-sulfate group engages in additional interactions with the hydrophobic region, residues 276-285, of the protein molecule, and this group is found wedged between the aromatic side chains of Phe-280 and Trp314 residues. Since the side chain of the Trp314 residue undergoes conformational changes during the catalytic cycle of the enzyme, molecular interaction between Trp314 and the 6-sulfate group might hinder this conformational change. Therefore, the lack of a favorable binding environment, together with hindrance to the conformational changes, might be responsible for the poor catalytic activity.

Published

2013

33. In Vitro Folding of β-1,4Galactosyltransferase and Polypeptide-α-N-Acetylgalactosaminyltransferase from the Inclusion Bodies

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

Folding (chemistry), Bioconjugation, Biochemistry, biology, Chemistry, Glycosyltransferase, biology.protein, Inclusion bodies, In vitro

Abstract

The aim of this article is to present a unique in vitro folding technique for glycosyltransferases to generate active proteins that can be used for X-ray crystallographic and bioconjugation protocols. Although a number of in vitro refolding methods are available, β1,4galactosyltransferases in large quantities can be made using the current protocol only. This technique is not only limited to glycosyltransferases alone but has been successfully used to refold single-chain antibodies and other molecules. Although this in vitro folding method is quite similar to other methods, it differs from them by the use of S-sulfonation of the inclusion bodies before setting up the in vitro refolding of the protein.

Published

2013

34. Binding of N-acetylglucosamine (GlcNAc) β1-6-branched oligosaccharide acceptors to β4-galactosyltransferase I reveals a new ligand binding mode

Author

Boopathy Ramakrishnan, Pradman K. Qasba, and Elizabeth Boeggeman

Subjects

Oligosaccharides, Branched-Chain, Beta-4Gal-T1, Stereochemistry, Glycobiology and Extracellular Matrices, Crystallography, X-Ray, Biochemistry, Acetylglucosamine, Oligosaccharide, Oligosaccharide binding, Structural Biology, Glycosyltransferase, Moiety, Tetrasaccharide, Humans, Binding site, Molecular Biology, Multiple Carbohydrate Binding Site, chemistry.chemical_classification, Enzyme Kinetics, Binding Sites, i/I-Antigen Synthesis, biology, Glycosyltransferases, Cell Biology, Galactosyltransferases, Acceptor, Enzyme structure, Protein Structure, Tertiary, chemistry, Enzyme Structure, biology.protein, Hydrophobic and Hydrophilic Interactions

Abstract

Background: The enzyme β4Gal-T1 synthesizes the LacNAc moiety of glycans. Results: The extended oligosaccharide moiety of β1–6-branched GlcNAc acceptors binds to a different region on the enzyme. Conclusion: β4Gal-T1 has two different oligosaccharide binding regions for extended oligosaccharide moieties of different acceptor substrates. Significance: Multiple carbohydrate acceptor binding regions are observed on a glycosyltransferase., N-Acetyllactosamine is the most prevalent disaccharide moiety in the glycans on the surface of mammalian cells and often found as repeat units in the linear and branched polylactosamines, known as i- and I-antigen, respectively. The β1–4-galactosyltransferase-I (β4Gal-T1) enzyme is responsible for the synthesis of the N-acetyllactosamine moiety. To understand its oligosaccharide acceptor specificity, we have previously investigated the binding of tri- and pentasaccharides of N-glycan with a GlcNAc at their nonreducing end and found that the extended sugar moiety in these acceptor substrates binds to the crevice present at the acceptor substrate binding site of the β4Gal-T1 molecule. Here we report seven crystal structures of β4Gal-T1 in complex with an oligosaccharide acceptor with a nonreducing end GlcNAc that has a β1–6-glycosidic link and that are analogous to either N-glycan or i/I-antigen. In the crystal structure of the complex of β4Gal-T1 with I-antigen analog pentasaccharide, the β1–6-branched GlcNAc moiety is bound to the sugar acceptor binding site of the β4Gal-T1 molecule in a way similar to the crystal structures described previously; however, the extended linear tetrasaccharide moiety does not interact with the previously found extended sugar binding site on the β4Gal-T1 molecule. Instead, it interacts with the different hydrophobic surface of the protein molecule formed by the residues Tyr-276, Trp-310, and Phe-356. Results from the present and previous studies suggest that β4Gal-T1 molecule has two different oligosaccharide binding regions for the binding of the extended oligosaccharide moiety of the acceptor substrate.

Published

2012

35. Bioconjugation using mutant glycosyltransferases for the site-specific labeling of biomolecules with sugars carrying chemical handles

Author

Boopathy, Ramakrishnan, Elizabeth, Boeggeman, Marta, Pasek, and Pradman K, Qasba

Subjects

Drug Carriers, Binding Sites, Glycosylation, Staining and Labeling, Receptor, ErbB-2, Recombinant Fusion Proteins, Asialoglycoproteins, Glycosyltransferases, Oligosaccharides, Protein Engineering, Chromatography, Affinity, Mass Spectrometry, Substrate Specificity, Luminescent Measurements, Mutation, Carbohydrate Metabolism, Humans, Peptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase, Biotinylation, alpha-Fetoproteins, Fetuins, Staphylococcal Protein A, Glycoproteins, Single-Chain Antibodies

Abstract

This chapter presents a technique that employs mutant glycosyltransferase enzymes for the site-specific bioconjugation of biomolecules via a glycan moiety to facilitate the development of a targeted drug delivery system. The target specificity of this methodology is based on unique sugar residues that are present on glycoproteins or engineered glycopeptides. The glycosyltransferases used in this approach have been manipulated in a way that confers the ability to transfer a modified sugar residue with a chemical handle to a sugar moiety of the glycoprotein or to a polypeptide tag of an engineered nonglycoprotein. The availability of the modified sugar moiety thus makes it possible to link cargo molecules at specific sites. The cargo may be comprised of, for example, biotin or fluorescent tags for detection, imaging agents for magnetic resonance imaging (MRI), or cytotoxic drugs for cancer therapy.

Published

2011

36. Bioconjugation Using Mutant Glycosyltransferases for the Site-Specific Labeling of Biomolecules with Sugars Carrying Chemical Handles

Author

Elizabeth Boeggeman, Marta Pasek, Boopathy Ramakrishnan, and Pradman K. Qasba

Subjects

Glycan, Residue (chemistry), Bioconjugation, Biochemistry, biology, Targeted drug delivery, Chemistry, Biotinylation, Glycosyltransferase, biology.protein, Moiety, Binding site

Abstract

This chapter presents a technique that employs mutant glycosyltransferase enzymes for the site-specific bioconjugation of biomolecules via a glycan moiety to facilitate the development of a targeted drug delivery system. The target specificity of this methodology is based on unique sugar residues that are present on glycoproteins or engineered glycopeptides. The glycosyltransferases used in this approach have been manipulated in a way that confers the ability to transfer a modified sugar residue with a chemical handle to a sugar moiety of the glycoprotein or to a polypeptide tag of an engineered nonglycoprotein. The availability of the modified sugar moiety thus makes it possible to link cargo molecules at specific sites. The cargo may be comprised of, for example, biotin or fluorescent tags for detection, imaging agents for magnetic resonance imaging (MRI), or cytotoxic drugs for cancer therapy.

Published

2011

37. Structure-based Evolutionary Relationship of Glycosyltransferases: A Case Study of Vertebrate β1, 4-Galactosyltransferase, Invertebrate β1,4-N-acetylgalactosaminyltransferase and α-Polypeptidyl-N-acetylgalactosaminyltransferase

Author

Pradman K. Qasba and Boopathy Ramakrishnan

Subjects

Glycan, Molecular Sequence Data, Biology, Article, Evolution, Molecular, Protein structure, Structural Biology, biology.animal, Glycosyltransferase, N-Acetyllactosamine Synthase, Animals, Humans, Amino Acid Sequence, Molecular Biology, Peptide sequence, Gene, chemistry.chemical_classification, Galactosyltransferase, Vertebrate, Glycosyltransferases, Invertebrates, Amino acid, chemistry, Biochemistry, Vertebrates, biology.protein, N-Acetylgalactosaminyltransferases

Abstract

Cell surface glycans play important cellular functions and are synthesized by glycosyltransferases. Structure and function studies show that the donor sugar specificity of the invertebrate β1,4-N-acetyl-glactosaminyltransferase (β4GalNAc-T) and the vertebrate β1,4-galactosyltransferase I (β4Gal-T1) are related by a single amino acid residue change. Comparison of the catalytic domain crystal structures of the β4Gal-T1 and the α-polypeptidyl-GalNAc-T (αppGalNAc-T) shows that their protein structure and sequences are similar. Therefore, it seems that the invertebrate β4GalNAc-T and the catalytic domain of αppGalNAc-T might have emerged from a common primordial gene. When vertebrates emerged from invertebrates, the amino acid that determines the donor sugar specificity of the invertebrate β4GalNAc-T might have mutated, thus converting the enzyme to a β4Gal-T1 in vertebrates.

Published

2010

38. Abstract 2486: Site-specific antibody-drug conjugation through an engineered glycotransferase and a chemically reactive sugar

Author

Zhu, Zhongyu, primary, Boopathy, Ramakrishnan, additional, Li, Jinyu, additional, Prabakaran, Ponraj, additional, Colantonio, Simona, additional, Feng, Yang, additional, Wang, Yanping, additional, Dyba, Marzena A., additional, and Dimitrov, Dimiter S., additional

Published

2015

39. Galectin-1 as a fusion partner for the production of soluble and folded human β-1,4-galactosyltransferase-T7 in E. coli

Author

Pradman K. Qasba, Elizabeth Boeggeman, Boopathy Ramakrishnan, and Marta Pasek

Subjects

Protein Folding, Galectin 1, Recombinant Fusion Proteins, Biophysics, Biology, medicine.disease_cause, Biochemistry, Inclusion bodies, Article, Protein structure, Affinity chromatography, TEV protease, medicine, Escherichia coli, Humans, Molecular Biology, Galectin, Circular Dichroism, Cell Biology, Galactosyltransferases, Fusion protein, Protein Structure, Tertiary, Solubility, Protein Biosynthesis, Protein folding, Spectrophotometry, Ultraviolet

Abstract

The expression of recombinant proteins in Escherichia coli often leads to inactive aggregated proteins known as the inclusion bodies. To date, the best available tool has been the use of fusion tags, including the carbohydrate-binding protein; e.g., the maltose-binding protein (MBP) that enhances the solubility of recombinant proteins. However, none of these fusion tags work universally with every partner protein. We hypothesized that galectins, which are also carbohydrate-binding proteins, may help as fusion partners in folding the mammalian proteins in E. coli. Here we show for the first time that a small soluble lectin, human galectin-1, one member of a large galectin family, can function as a fusion partner to produce soluble folded recombinant human glycosyltransferase, beta-1,4-galactosyltransferase-7 (beta4Gal-T7), in E. coli. The enzyme beta4Gal-T7 transfers galactose to xylose during the synthesis of the tetrasaccharide linker sequence attached to a Ser residue of proteoglycans. Without a fusion partner, beta4Gal-T7 is expressed in E. coli as inclusion bodies. We have designed a new vector construct, pLgals1, from pET-23a that includes the sequence for human galectin-1, followed by the Tev protease cleavage site, a 6x His-coding sequence, and a multi-cloning site where a cloned gene is inserted. After lactose affinity column purification of galectin-1-beta4Gal-T7 fusion protein, the unique protease cleavage site allows the protein beta4Gal-T7 to be cleaved from galectin-1 that binds and elutes from UDP-agarose column. The eluted protein is enzymatically active, and shows CD spectra comparable to the folded beta4Gal-T1. The engineered galectin-1 vector could prove to be a valuable tool for expressing other proteins in E. coli.

Published

2010

40. Crystal structure of the Y52F/Y73F double mutant of phospholipase A2: Increased hydrophobic interactions of the phenyl groups compensate for the disrupted hydrogen bonds of the tyrosines

Author

Chandra Sekharudu, Boopathy Ramakrishnan, Baohua Huang, Muttaiya Sundaralingam, Ru-Tai Jiang, Ming-Daw Tsai, and Cynthia M. Dupureur

Subjects

Stereochemistry, Crystal structure, Biochemistry, Phospholipases A, Protein Structure, Secondary, Catalysis, Hydrophobic effect, chemistry.chemical_compound, Catalytic triad, Animals, Molecule, Amino Acid Sequence, Carboxylate, Pancreas, Molecular Biology, biology, Hydrogen bond, Active site, Hydrogen Bonding, Recombinant Proteins, Models, Structural, Phospholipases A2, chemistry, Mutagenesis, Site-Directed, biology.protein, Tyrosine, Cattle, Research Article

Abstract

The enzyme phospholipase A2 (PLA2) catalyzes the hydrolysis of the sn-2 ester bond of membrane phospholipids. The highly conserved Tyr residues 52 and 73 in the enzyme form hydrogen bonds to the carboxylate group of the catalytic Asp-99. These hydrogen bonds were initially regarded as essential for the interfacial recognition and the stability of the overall catalytic network. The elimination of the hydrogen bonds involving the phenolic hydroxyl groups of the Tyr-52 and -73 by changing them to Phe lowered the stability but did not significantly affect the catalytic activity of the enzyme. The X-ray crystal structure of the double mutant Y52F/Y73F has been determined at 1.93 A resolution to study the effect of the mutation on the structure. The crystals are trigonal, space group P3(1)21, with cell parameters a = b = 46.3 A and c = 102.95 A. Intensity data were collected on a Siemens area detector, 8,024 reflections were unique with an R(sym) of 4.5% out of a total of 27,203. The structure was refined using all the unique reflections by XPLOR to a final R-factor of 18.6% for 955 protein atoms, 91 water molecules, and 1 calcium ion. The root mean square deviation for the alpha-carbon atoms between the double mutant and wild type was 0.56 A. The crystal structure revealed that four hydrogen bonds were lost in the catalytic network; three involving the tyrosines and one involving Pro-68. However, the hydrogen bonds of the catalytic triad, His-48, Asp-99, and the catalytic water, are retained. There is no additional solvent molecule at the active site to replace the missing hydroxyl groups; instead, the replacement of the phenolic OH groups by H atoms draws the Phe residues closer to the neighboring residues compared to wild type; Phe-52 moves toward His-48 and Asp-99 of the catalytic diad, and Phe-73 moves toward Met-8, both by about 0.5 A. The closing of the voids left by the OH groups increases the hydrophobic interactions compensating for the lost hydrogen bonds. The conservation of the triad hydrogen bonds and the stabilization of the active site by the increased hydrophobic interactions could explain why the double mutant has activity similar to wild type. The results indicate that the aspartyl carboxylate group of the catalytic triad can function alone without additional support from the hydrogen bonds of the two Tyr residues.

Published

1992

41. Site specific conjugation of fluoroprobes to the remodeled Fc N-glycans of monoclonal antibodies using mutant glycosyltransferases: application for cell surface antigen detection

Author

Pradman K. Qasba, Elizabeth Boeggeman, Anu Puri, Timothy J. Waybright, Kristin H. Loomis, Marta Pasek, Boopathy Ramakrishnan, and Maria Manzoni

Subjects

PNGase F, Vascular Endothelial Growth Factor A, Glycan, Glycosylation, medicine.drug_class, Receptor, ErbB-2, Population, Biomedical Engineering, Pharmaceutical Science, Oligosaccharides, Bioengineering, Enzyme-Linked Immunosorbent Assay, Monoclonal antibody, Article, Substrate Specificity, chemistry.chemical_compound, Polysaccharides, Cell Line, Tumor, medicine, Animals, Humans, Biotinylation, education, Fluorescent Dyes, Pharmacology, education.field_of_study, Glucosamine, Binding Sites, biology, Staining and Labeling, Organic Chemistry, Antibodies, Monoclonal, Galactose, Glycosyltransferases, Molecular biology, Sialic acid, chemistry, Biochemistry, Immunoglobulin G, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Antigens, Surface, biology.protein, Mutant Proteins, Biotechnology

Abstract

The Fc N-glycan chains of four therapeutic monoclonal antibodies (mAbs), namely, Avastin, Rituxan, Remicade, and Herceptin, released by PNGase F, show by MALDI analysis that these biantennary N-glycans are a mixture of G0, G1, and G2 glycoforms. The G0 glycoform has no galactose on the terminal GlcNAc residues, and the G1 and G2 glycoforms have one or two terminal galactose residues, respectively, while no N-glycan with terminal sialic acid residue is observed. We show here that under native conditions we can convert the N-glycans of these mAbs to a homogeneous population of G0 glycoform using beta1,4 galactosidase from Streptococcus pneumoniae. The G0 glycoforms of mAbs can be galactosylated with a modified galactose having a chemical handle at the C2 position, such as ketone or azide, using a mutant beta1,4-galactosyltransferase (beta1,4Gal-T1-Y289L). The addition of the modified galactose at a specific glycan residue of a mAb permits the coupling of a biomolecule that carries an orthogonal reactive group. The linking of a biotinylated or a fluorescent dye carrying derivatives selectively occurs with the modified galactose, C2-keto-Gal, at the heavy chain of these mAbs, without altering their antigen binding activities, as shown by indirect enzyme linked immunosorbent assay (ELISA) and fluorescence activated cell sorting (FACS) methods. Our results demonstrate that the linking of cargo molecules to mAbs via glycans could prove to be an invaluable tool for potential drug targeting by immunotherapeutic methods.

Published

2009

42. Iterative cluster-NMA: A tool for generating conformational transitions in proteins

Author

Boopathy Ramakrishnan, Robert L. Jernigan, Pradman K. Qasba, Adam D. Schuyler, and Gregory S. Chirikjian

Subjects

Computational model, Protein Folding, Chemistry, Protein Conformation, Structure (category theory), Energy landscape, Computational Biology, Proteins, Biochemistry, Displacement (vector), Article, Structural Biology, Robustness (computer science), Normal mode, Computational chemistry, Cluster (physics), Cluster Analysis, Protein folding, Computer Simulation, Statistical physics, Databases, Protein, Molecular Biology

Abstract

Computational models provide insight into the structure-function relationship in proteins. These approaches, especially those based on normal mode analysis, can identify the accessible motion space around a given equilibrium structure. The large magnitude, collective motions identified by these methods are often well aligned with the general direction of the expected conformational transitions. However, these motions cannot realistically be extrapolated beyond the local neighborhood of the starting conformation. In this article, the iterative cluster-NMA (icNMA) method is presented for traversing the energy landscape from a starting conformation to a desired goal conformation. This is accomplished by allowing the evolving geometry of the intermediate structures to define the local accessible motion space, and thus produce an appropriate displacement. Following the derivation of the icNMA method, a set of sample simulations are performed to probe the robustness of the model. A detailed analysis of beta1,4-galactosyltransferase-T1 is also given, to highlight many of the capabilities of icNMA. Remarkably, during the transition, a helix is seen to be extended by an additional turn, emphasizing a new unknown role for secondary structures to absorb slack during transitions. The transition pathway for adenylate kinase, which has been frequently studied in the literature, is also discussed.

Published

2008

43. Site-Specific Linking of Biomolecules via Glycan Residues Using Glycosyltransferases

Author

Boopathy Ramakrishnan, Pradman K. Qasba, and Elizabeth Boeggeman

Subjects

chemistry.chemical_classification, Glycan, Binding Sites, biology, Glycoconjugate, Stereochemistry, Biomolecule, Glycosyltransferases, Article, Catalysis, carbohydrates (lipids), chemistry.chemical_compound, Residue (chemistry), Biopolymers, Cross-Linking Reagents, chemistry, Biochemistry, Polysaccharides, Galactose, Drug Design, Glycosyltransferase, biology.protein, Binding site, Biotechnology, Conjugate

Abstract

The structural information on glycosyltransferases has revealed that the sugar-donor specificity of these enzymes can be broadened to include modified sugars with a chemical handle that can be utilized for conjugation chemistry. Substitution of Tyr289 to Leu in the catalytic pocket of bovine beta-1,4-galactosyltransferase generates a novel glycosyltransferase that can transfer not only Gal but also GalNAc or a C2-modified galactose that has a chemical handle, from the corresponding UDP-derivatives, to the non-reducing end GlcNAc residue of a glycoconjugate. Similarly, the wild-type polypeptide-N-acetyl-galactosaminyltransferase, which naturally transfers GalNAc from UDP-GalNAc, can also transfer C2-modified galactose with a chemical handle from its UDP-derivative to the Ser/Thr residue of a polypeptide acceptor substrate that is tagged as a fusion peptide to a non-glycoprotein. The potential of wild-type and mutant glycosyltransferases to produce glycoconjugates carrying sugar moieties with chemical handle makes it possible to conjugate biomolecules with orthogonal reacting groups at specific sites. This methodology assists in the assembly of bio-nanoparticles that are useful for developing targeted drug-delivery systems and contrast agents for magnetic resonance imaging.

Published

2008

44. Direct identification of nonreducing GlcNAc residues on N-glycans of glycoproteins using a novel chemoenzymatic method

Author

Boopathy Ramakrishnan, Nelly Khidekel, Charlton Kilgore, Linda C. Hsieh-Wilson, Elizabeth Boeggeman, Pradman K. Qasba, and John T. Simpson

Subjects

PNGase F, Glycan, Ovalbumin, Glycoconjugate, Stereochemistry, Biomedical Engineering, Pharmaceutical Science, Bioengineering, Article, Acetylglucosamine, chemistry.chemical_compound, Polysaccharides, Ketoses, Animals, Biotinylation, Glycoproteins, Pharmacology, chemistry.chemical_classification, Galactosyltransferase, biology, Organic Chemistry, Galactose, Oligosaccharide, Galactosyltransferases, carbohydrates (lipids), chemistry, Biochemistry, Immunoglobulin G, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Mutation, biology.protein, Peptides, Glycoprotein, Glycoconjugates, Oxidation-Reduction, Biotechnology

Abstract

The mutant beta1,4-galactosyltransferase (beta4Gal-T1), beta4Gal-T1-Y289L, in contrast to wild-type beta4Gal-T1, can transfer GalNAc from the sugar donor UDP-GalNAc to the acceptor, GlcNAc, with efficiency as good as that of galactose from UDP-Gal. Furthermore, the mutant can also transfer a modified sugar, C2 keto galactose, from its UDP derivative to O-GlcNAc modification on proteins that provided a functional handle for developing a highly sensitive chemoenzymatic method for detecting O-GlcNAc post-translational modification on proteins. We report herein that the modified sugar, C2 keto galactose, can be transferred to free GlcNAc residues on N-linked glycoproteins, such as ovalbumin or asialo-agalacto IgG1. The transfer is strictly dependent on the presence of both the mutant enzyme and the ketone derivative of the galactose. Moreover, the PNGase F treatment of the glycoproteins, which cleaves the N-linked oligosaccharide chain, shows that the modified sugar has been transferred to the N-glycan chains of the glycoproteins and not to the protein portion. The application of the mutant galactosyltransferase, beta4Gal-T1-Y289L, to produce glycoconjugates carrying sugar moieties with reactive groups, is demonstrated. We envision a broad potential for this technology such as the possibilities to link cargo molecules to glycoproteins, such as monoclonal antibodies, via glycan chains, thereby assisting in the glycotargeting of drugs to the site of action or used as biological probes.

Published

2007

45. Mutant glycosyltransferases assist in the development of a targeted drug delivery system and contrast agents for MRI

Author

Elizabeth Boeggeman, Boopathy Ramakrishnan, and Pradman K. Qasba

Subjects

chemistry.chemical_classification, Glycan, biology, Chemistry, Pharmaceutical Science, Contrast Media, Glycosyltransferases, Oligosaccharide, Magnetic Resonance Imaging, Article, law.invention, Residue (chemistry), Glycolipid, Drug Delivery Systems, Targeted drug delivery, Biochemistry, law, Glycosyltransferase, biology.protein, Recombinant DNA, Animals, Humans, Glycoprotein, Genetic Engineering, Glycoconjugates

Abstract

The availability of structural information on glycosyltransferases is beginning to make structure-based reengineering of these enzymes possible. Mutant glycosyltransferases have been generated that can transfer a sugar residue with a chemically reactive unique functional group to a sugar moiety of glycoproteins, glycolipids, and proteoglycans (glyco-conjugates). The presence of modified sugar moiety on a glycoprotein makes it possible to link bioactive molecules via modified glycan chains, thereby assisting in the assembly of bionanoparticles that are useful for developing the targeted drug delivery system and contrast agents for magnetic resonance imaging. The reengineered recombinant glycosyltransferases also make it possible to (1) remodel the oligosaccharide chains of glycoprotein drugs, and (2) synthesize oligosaccharides for vaccine development.

Published

2006

46. Oligosaccharide preferences of beta1,4-galactosyltransferase-I: crystal structures of Met340His mutant of human beta1,4-galactosyltransferase-I with a pentasaccharide and trisaccharides of the N-glycan moiety

Author

Pradman K. Qasba, Velavan Ramasamy, Daniel M. Ratner, Peter H. Seeberger, Elizabeth Boeggeman, and Boopathy Ramakrishnan

Subjects

Models, Molecular, Glycan, Stereochemistry, Mannose, Oligosaccharides, Chitobiose, Crystallography, X-Ray, Catalysis, Substrate Specificity, chemistry.chemical_compound, Residue (chemistry), Methionine, Structural Biology, Carbohydrate Conformation, Humans, Trisaccharide, Molecular Biology, Galactosyltransferase, chemistry.chemical_classification, biology, Oligosaccharide, Galactosyltransferases, Protein Structure, Tertiary, Kinetics, chemistry, Mutation, biology.protein, Glycoprotein

Abstract

beta-1,4-Galactosyltransferase-I (beta4Gal-T1) transfers galactose from UDP-galactose to N-acetylglucosamine (GlcNAc) residues of the branched N-linked oligosaccharide chains of glycoproteins. In an N-linked biantennary oligosaccharide chain, one antenna is attached to the 3-hydroxyl-(1,3-arm), and the other to the 6-hydroxyl-(1,6-arm) group of mannose, which is beta-1,4-linked to an N-linked chitobiose, attached to the aspargine residue of a protein. For a better understanding of the branch specificity of beta4Gal-T1 towards the GlcNAc residues of N-glycans, we have carried out kinetic and crystallographic studies with the wild-type human beta4Gal-T1 (h-beta4Gal-T1) and the mutant Met340His-beta4Gal-T1 (h-M340H-beta4Gal-T1) in complex with a GlcNAc-containing pentasaccharide and several GlcNAc-containing trisaccharides present in N-glycans. The oligosaccharides used were: pentasaccharide GlcNAcbeta1,2-Manalpha1,6 (GlcNAcbeta1,2-Manalpha1,3)Man; the 1,6-arm trisaccharide, GlcNAcbeta1,2-Manalpha1,6-Manbeta-OR (1,2-1,6-arm); the 1,3-arm trisaccharides, GlcNAcbeta1,2-Manalpha1,3-Manbeta-OR (1,2-1,3-arm) and GlcNAcbeta1,4-Manalpha1,3-Manbeta-OR (1,4-1,3-arm); and the trisaccharide GlcNAcbeta1,4-GlcNAcbeta1,4-GlcNAc (chitotriose). With the wild-type h-beta4Gal-T1, the K(m) of 1,2-1,6-arm is approximately tenfold lower than for 1,2-1,3-arm and 1,4-1,3-arm, and 22-fold lower than for chitotriose. Crystal structures of h-M340H-beta4Gal-T1 in complex with the pentasaccharide and various trisaccharides at 1.9-2.0A resolution showed that beta4Gal-T1 is in a closed conformation with the oligosaccharide bound to the enzyme, and the 1,2-1,6-arm trisaccharide makes the maximum number of interactions with the enzyme, which is in concurrence with the lowest K(m) for the trisaccharide. Present studies suggest that beta4Gal-T1 interacts preferentially with the 1,2-1,6-arm trisaccharide rather than with the 1,2-1,3-arm or 1,4-1,3-arm of a bi- or tri-antennary oligosaccharide chain of N-glycan.

Published

2005

47. Structure and catalytic cycle of beta-1,4-galactosyltransferase

Author

Elizabeth Boeggeman, Boopathy Ramakrishnan, Velavan Ramasamy, and Pradman K. Qasba

Subjects

chemistry.chemical_classification, Galactosyltransferase, Models, Molecular, Molecular Structure, Stereochemistry, Protein Conformation, Oligosaccharide, Acceptor, Catalysis, Protein structure, chemistry, Catalytic cycle, Structural Biology, Lactose Synthase, Metals, N-Acetyllactosamine Synthase, Moiety, Binding site, Molecular Biology, Alpha helix

Abstract

Beta-1,4-galactosyltransferase-1, a housekeeping enzyme that functions in the synthesis of glycoconjugates, has two flexible loops, one short and one long. Upon binding a metal ion and UDP-galactose, the loops change from an open to a closed conformation, repositioning residues to lock the ligands in place. Residues at the N-terminal region of the long loop form the metal-binding site and those at the C-terminal region form a helix, which becomes part of the binding site for the oligosaccharide acceptor; the remaining residues cover the bound sugar-nucleotide. After binding of the oligosaccharide acceptor and transfer of the galactose moiety, the product disaccharide unit is ejected and the enzyme returns to the open conformation, repeating the catalytic cycle.

Published

2004

48. Effect of the Met344His mutation on the conformational dynamics of bovine beta-1,4-galactosyltransferase: crystal structure of the Met344His mutant in complex with chitobiose

Author

Boopathy, Ramakrishnan, Elizabeth, Boeggeman, and Pradman K, Qasba

Subjects

Manganese, Protein Conformation, Monosaccharides, Crystallography, X-Ray, Disaccharides, Catalysis, Acetylglucosamine, Uridine Diphosphate Galactose, Structure-Activity Relationship, Methionine, N-Acetyllactosamine Synthase, Carbohydrate Conformation, Mutagenesis, Site-Directed, Animals, Hexanes, Thermodynamics, Tyrosine, Cattle, Histidine, Magnesium, Crystallization

Abstract

Beta-1,4-galactosyltransferase (beta4Gal-T1) in the presence of manganese ion transfers galactose from UDP-galactose (UDP-Gal) to N-acetylglucosamine (GlcNAc) that is either free or linked to an oligosaccharide. Crystallographic studies on bovine beta4Gal-T1 have shown that the primary metal binding site is located in the hinge region of a long flexible loop, which upon Mn(2+) and UDP-Gal binding changes from an open to a closed conformation. This conformational change creates an oligosaccharide binding site in the enzyme. Neither UDP nor UDP analogues efficiently induce these conformational changes in the wild-type enzyme, thereby restricting the structural analysis of the acceptor binding site. The binding of Mn(2+) involves an uncommon coordination to the Sdelta atom of Met344; when it is mutated to His, the mutant M344H, in the presence of Mn(2+) and UDP-hexanolamine, readily changes to a closed conformation, facilitating the structural analysis of the enzyme bound with an oligosaccharide acceptor. Although the mutant M344H loses 98% of its Mn(2+)-dependent activity, it exhibits 25% of its activity in the presence of Mg(2+). The crystal structures of M344H-Gal-T1 in complex with either UDP-Gal.Mn(2+) or UDP-Gal.Mg(2+), determined at 2.3 A resolution, show that the mutant enzyme in these complexes is in a closed conformation, and the coordination stereochemistry of Mg(2+) is quite similar to that of Mn(2+). Although either Mn(2+) or Mg(2+), together with UDP-Gal, binds and changes the conformation of the M344H mutant to the closed one, it is the Mg(2+) complex that engages efficiently in catalyses. Thus, this property enabled us to crystallize the M344H mutant for the first time with the acceptor substrate chitobiose in the presence of UDP-hexanolamine and Mn(2+). The crystal structure determined at 2.3 A resolution reveals that the GlcNAc residue at the nonreducing end of chitobiose makes extensive hydrophobic interactions with the highly conserved Tyr286 residue.

Published

2004

49. A Chemoenzymatic Approach toward the Rapid and Sensitive Detection of O-GlcNAc Posttranslational Modifications

Author

Sabine Arndt, Boopathy Ramakrishnan, Nelly Khidekel, Linda C. Hsieh-Wilson, Alexander R. Lippert, Nathan Lamarre-Vincent, Pradman K. Qasba, and Katherine G. Poulin-Kerstien

Subjects

Glycosylation, Ketone, Mutant, Fluorescence spectrometry, Biotin, Biochemistry, Catalysis, Analyse qualitative, Acetylglucosamine, chemistry.chemical_compound, Colloid and Surface Chemistry, Qualitative analysis, Bacterial Proteins, N-Acetyllactosamine Synthase, Animals, Moiety, alpha-Crystallins, Cyclic AMP Response Element-Binding Protein, Horseradish Peroxidase, Glycoproteins, chemistry.chemical_classification, General Chemistry, chemistry, Luminescent Measurements

Abstract

We report a new chemoenzymatic strategy for the rapid and sensitive detection of O-GlcNAc posttranslational modifications. The approach exploits the ability of an engineered mutant of beta-1,4-galactosyltransferase to selectively transfer an unnatural ketone functionality onto O-GlcNAc glycosylated proteins. Once transferred, the ketone moiety serves as a versatile handle for the attachment of biotin, thereby enabling chemiluminescent detection of the modified protein. Importantly, this approach permits the rapid visualization of proteins that are at the limits of detection using traditional methods. Moreover, it bypasses the need for radioactive precursors and captures the glycosylated species without perturbing metabolic pathways. We anticipate that this general chemoenzymatic strategy will have broad application to the study of posttranslational modifications.

Published

2003

50. The N-terminal stem region of bovine and human beta1,4-galactosyltransferase I increases the in vitro folding efficiency of their catalytic domain from inclusion bodies

Author

Pradman K. Qasba, Elizabeth Boeggeman, and Boopathy Ramakrishnan

Subjects

Protein Folding, Molecular Sequence Data, Protein Renaturation, medicine.disease_cause, Inclusion bodies, Chromatography, Affinity, law.invention, law, Catalytic Domain, N-Acetyllactosamine Synthase, medicine, Escherichia coli, Animals, Humans, Amino Acid Sequence, Galactosyltransferase, Inclusion Bodies, biology, Base Sequence, Circular Dichroism, In vitro, Recombinant Proteins, N-terminus, Biochemistry, Chaperone (protein), Recombinant DNA, biology.protein, Protein folding, Cattle, Biotechnology

Abstract

Many recombinant proteins overexpressed in Escherichia coli are generally misfolded, which then aggregate and accumulate as inclusion bodies. The catalytic domain (CD) of bovine and human β1,4-galactosyltransferase (β4Gal-T), expressed in E. coli , it also accumulates as inclusion bodies. We studied the effect of the fusion of the stem region (SR), as an N-terminal extension of the catalytic domain, on the in vitro folding efficiencies of the inclusion bodies. The stem region fused to the catalytic domain (SRCD) increases the folding efficiency of recombinant protein with native fold compared to the protein that contains only the CD. During in vitro folding, also promotes considerably the solubility of the misfolded proteins, which do not bind to UDP–agarose columns and exhibit no galactosyltransferase activity. In contrast, the misfolded proteins that consist of only the CD are insoluble and precipitate out of solution. It is concluded that a protein domain that is produced in a soluble form does not guarantee the presence of the protein molecules in a properly folded and active form. The stem domain has a positive effect on the in vitro folding efficiency of the catalytic domain of both human and bovine β4Gal-T1, suggesting that the stem region acts as a chaperone during protein folding. Furthermore, investigation of the folding conditions of the sulphonated inclusion bodies resulted in identifying a condition in which the presence of PEG-4000 and l -arginine, compared to their absence, increased the yields of native CD and SRCD 7- and 3-fold, respectively.

Published

2003