159 results on '"YONG-LIANG JIANG"'
Search Results
52. Coordinating carbon and nitrogen metabolic signaling through the cyanobacterial global repressor NdhR
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Hui Sun, Gui-Ming Lin, Ning Cui, Cong-Zhao Zhou, Ju-Yuan Zhang, Zhiyong Zhang, Shu-Jing Han, Cheng-Cai Zhang, Yuxing Chen, Yong-Liang Jiang, Xue-Ping Wang, Wei-Fang Li, Wang Cheng, and Dong-Dong Cao
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0301 basic medicine ,Oxygenase ,Nitrogen ,Ribulose-Bisphosphate Carboxylase ,030106 microbiology ,Repressor ,Cyanobacteria ,03 medical and health sciences ,chemistry.chemical_compound ,Bacterial Proteins ,Genes, Regulator ,NAD(P)H Dehydrogenase (Quinone) ,Multidisciplinary ,biology ,Chemistry ,Ribulose ,RuBisCO ,Gene Expression Regulation, Bacterial ,Carbon Dioxide ,Biological Sciences ,Carbon ,Glycolates ,Pyruvate carboxylase ,Regulon ,Biochemistry ,biology.protein ,Ketoglutaric Acids ,Photorespiration ,Corepressor ,Signal Transduction - Abstract
The coordination of carbon and nitrogen metabolism is essential for bacteria to adapt to nutritional variations in the environment, but the underlying mechanism remains poorly understood. In autotrophic cyanobacteria, high CO2 levels favor the carboxylase activity of ribulose 1,5 bisphosphate carboxylase/oxygenase (RuBisCO) to produce 3-phosphoglycerate, whereas low CO2 levels promote the oxygenase activity of RuBisCO, leading to 2-phosphoglycolate (2-PG) production. Thus, the 2-PG level is reversely correlated with that of 2-oxoglutarate (2-OG), which accumulates under a high carbon/nitrogen ratio and acts as a nitrogen-starvation signal. The LysR-type transcriptional repressor NAD(P)H dehydrogenase regulator (NdhR) controls the expression of genes related to carbon metabolism. Based on genetic and biochemical studies, we report here that 2-PG is an inducer of NdhR, while 2-OG is a corepressor, as found previously. Furthermore, structural analyses indicate that binding of 2-OG at the interface between the two regulatory domains (RD) allows the NdhR tetramer to adopt a repressor conformation, whereas 2-PG binding to an intradomain cleft of each RD triggers drastic conformational changes leading to the dissociation of NdhR from its target DNA. We further confirmed the effect of 2-PG or 2-OG levels on the transcription of the NdhR regulon. Together with previous findings, we propose that NdhR can sense 2-OG from the Krebs cycle and 2-PG from photorespiration, two key metabolites that function together as indicators of intracellular carbon/nitrogen status, thus representing a fine sensor for the coordination of carbon and nitrogen metabolism in cyanobacteria.
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- 2017
53. Virulence factors on the surface of Gram-positive pathogens and mechanisms of host-pathogen recognition
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Tengchuan Jin, Yong-Liang Jiang, Yuxing Chen, and Cong-Zhao Zhou
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Pathogenesis ,Innate immune system ,Staphylococcus aureus ,Host (biology) ,Streptococcus pneumoniae ,medicine ,Virulence ,Pharmacology (medical) ,Human pathogen ,Biology ,medicine.disease_cause ,Pathogen ,Microbiology - Abstract
Gram-positive pathogens encode various virulence factors, which are required for their growth and pathogenesis. These virulence factors not only participate in cell division and proliferation, but also mediate adhesion to and invasion of the host. Owing to investigations on the two important human pathogens Streptococcus pneumoniae and Staphylococcus aureus in the last decade, we have obtained some meaningful insights into the virulence factors on the bacterial surface. Here, we focus on the structures and functions of several major virulence factors in order to elucidate the molecular mechanism by which they contribute to pathogen-host recognition.
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- 2017
54. Crystal structure of a novel fold protein Gp72 from the freshwater cyanophage Mic1
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Wei-Fang Li, Yan-Yan Zhao, Hua Jin, Yong-Liang Jiang, Zhi-Peng Chen, Qiong Li, Yuxing Chen, Ying Wang, Feng Yang, and Cong-Zhao Zhou
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Cyanobacteria ,Models, Molecular ,Protein Conformation, alpha-Helical ,Protein Folding ,Hypothetical protein ,Genetic Vectors ,Gene Expression ,Fresh Water ,Crystal structure ,Crystallography, X-Ray ,Biochemistry ,03 medical and health sciences ,Viral Proteins ,Structural Biology ,Escherichia coli ,Bacteriophages ,Protein Interaction Domains and Motifs ,Amino Acid Sequence ,Disulfides ,Cloning, Molecular ,Cyanophages ,Molecular Biology ,030304 developmental biology ,Genetics ,0303 health sciences ,Binding Sites ,biology ,Sequence Homology, Amino Acid ,Chemistry ,030302 biochemistry & molecular biology ,Disulfide bond ,Cyanophage ,Protein superfamily ,biology.organism_classification ,Recombinant Proteins ,Protein Conformation, beta-Strand ,Protein Multimerization ,Oxidation-Reduction ,Sequence Alignment ,Protein Binding - Abstract
Cyanophages, widespread in aquatic systems, are a class of viruses that specifically infect cyanobacteria. Though they play important roles in modulating the homeostasis of cyanobacterial populations, little is known about the freshwater cyanophages, especially those hypothetical proteins of unknown function. Mic1 is a freshwater siphocyanophage isolated from the Lake Chaohu. It encodes three hypothetical proteins Gp65, Gp66, and Gp72, which share an identity of 61.6% to 83%. However, we find these three homologous proteins differ from each other in oligomeric state. Moreover, we solve the crystal structure of Gp72 at 2.3 A, which represents a novel fold in the α + β class. Structural analyses combined with redox assays enable us to propose a model of disulfide bond mediated oligomerization for Gp72. Altogether, these findings provide structural and biochemical basis for further investigations on the freshwater cyanophage Mic1.
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- 2019
55. Molecular basis for the assembly of RuBisCO assisted by the chaperone Raf1
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Ling-Yun, Xia, Yong-Liang, Jiang, Wen-Wen, Kong, Hui, Sun, Wei-Fang, Li, Yuxing, Chen, and Cong-Zhao, Zhou
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Bacterial Proteins ,Ribulose-Bisphosphate Carboxylase ,Amino Acid Sequence ,Anabaena ,Sequence Alignment ,Protein Structure, Secondary ,Molecular Chaperones ,Plant Proteins - Abstract
The folding and assembly of RuBisCO, the most abundant enzyme in nature, needs a series of chaperones, including the RuBisCO accumulation factor Raf1, which is highly conserved in cyanobacteria and plants. Here, we report the crystal structures of Raf1 from cyanobacteria Anabaena sp. PCC 7120 and its complex with RuBisCO large subunit RbcL. Structural analyses and biochemical assays reveal that each Raf1 dimer captures an RbcL dimer, with the C-terminal tail inserting into the catalytic pocket, and further mediates the assembly of RbcL dimers to form the octameric core of RuBisCO. Furthermore, the cryo-electron microscopy structures of the RbcL-Raf1-RbcS assembly intermediates enable us to see a dynamic assembly process from RbcL
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- 2019
56. Structural insights into repression of the Pneumococcal fatty acid synthesis pathway by repressor FabT and co-repressor acyl-ACP
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Yong-Liang Jiang, Yuxing Chen, Gang Zuo, Chengtao Ding, Cong-Zhao Zhou, Zhiyong Zhang, Zhi-Peng Chen, Qiong Li, and Zhongliang Zhu
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DNA, Bacterial ,Biophysics ,Repressor ,medicine.disease_cause ,Biochemistry ,03 medical and health sciences ,chemistry.chemical_compound ,Bacterial Proteins ,Structural Biology ,Streptococcus pneumoniae ,Genetics ,medicine ,Acyl Carrier Protein ,Molecular Biology ,Psychological repression ,Fatty acid synthesis ,030304 developmental biology ,chemistry.chemical_classification ,0303 health sciences ,Co repressor ,Binding Sites ,biology ,030302 biochemistry & molecular biology ,Fatty Acids ,Fatty acid ,Cell Biology ,In vitro ,Molecular Docking Simulation ,Acyl carrier protein ,chemistry ,biology.protein ,lipids (amino acids, peptides, and proteins) ,Protein Binding ,Transcription Factors - Abstract
The Streptococcus pneumoniae fatty acid synthesis (FAS) pathway is globally controlled at the transcriptional level by the repressor FabT and its co-repressor acyl carrier protein (acyl-ACP), the intermediate of phospholipid synthesis. Here, we report the crystal structure of FabT complexed with a 23-bp dsDNA, which indicates that FabT is a weak repressor with low DNA-binding affinity in the absence of acyl-ACP. Modification of ACP with a long-chain fatty acid is necessary for the formation of a stable complex with FabT, mimicked in vitro by cross-linking, which significantly elevates the DNA-binding affinity of FabT. Altogether, we propose a putative working model of gene repression under the double control of FabT and acyl-ACP, elucidating a distinct repression network for Pneumococcus to precisely coordinate FAS.
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- 2019
57. Crystal structure of pentameric shell protein CsoS4B of Halothiobacillus neapolitanus α-carboxysome
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Yan-Yan Zhao, Yuxing Chen, Yong-Liang Jiang, Cong-Zhao Zhou, and Qiong Li
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0301 basic medicine ,Models, Molecular ,Pentamer ,Pentameric protein ,Protein subunit ,Static Electricity ,Biophysics ,Shell (structure) ,Crystal structure ,Crystallography, X-Ray ,Biochemistry ,Halothiobacillus neapolitanus ,03 medical and health sciences ,0302 clinical medicine ,Bacterial Proteins ,Amino Acid Sequence ,Molecular Biology ,Chemistry ,Cell Biology ,Halothiobacillus ,Carboxysome ,030104 developmental biology ,Structural Homology, Protein ,030220 oncology & carcinogenesis ,Helix ,Protein Multimerization - Abstract
Carboxysome, encapsulating an enzymatic core within an icosahedral-shaped semipermeable protein shell, could enhance CO2 fixation under low CO2 conditions in the environment. The shell of Halothiobacillus neapolitanus α-carboxysome possesses two 38% sequence-identical pentameric proteins, namely CsoS4A and CsoS4B. However, the functions of two paralogous pentameric proteins in α-carboxysome assembly remain unknown. Here we report the crystal structure of CsoS4B at 2.15 A resolution. It displays as a stable pentamer, each subunit of which consists of a β-barrel core domain, in addition to an insertion of helix α1 that forms the central pore. Structural comparisons and multiple-sequence alignment strongly indicate that CsoS4A and CsoS4B differ from each other in interacting with various components of α-carboxysome, despite they share a similar overall structure. These findings provide the structural basis for further investigations on the self-assembly process of carboxysome.
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- 2019
58. Multi-functional regulator MapZ controls both positioning and timing of FtsZ polymerization
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Cong-Zhao Zhou, Yong-Liang Jiang, Jiahai Zhang, Zhang Feng, Da Xu, and Yuxing Chen
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Cell division ,Regulator ,Cooperativity ,Cytokinetic ring ,macromolecular substances ,GTPase ,physiological processes ,Biochemistry ,03 medical and health sciences ,Bacterial Proteins ,Protein Domains ,FtsZ ,Molecular Biology ,030304 developmental biology ,0303 health sciences ,biology ,030306 microbiology ,Chemistry ,Hydrolysis ,Cell Biology ,Cytoskeletal Proteins ,Streptococcus pneumoniae ,Polymerization ,Membrane protein ,Biophysics ,biology.protein ,bacteria ,Guanosine Triphosphate ,biological phenomena, cell phenomena, and immunity ,Protein Multimerization - Abstract
The tubulin-like GTPase protein FtsZ, which forms a discontinuous cytokinetic ring at mid-cell, is a central player to recruit the division machinery to orchestrate cell division. To guarantee the production of two identical daughter cells, the assembly of FtsZ, namely Z-ring, and its precise positioning should be finely regulated. In Streptococcus pneumoniae, the positioning of Z-ring at the division site is mediated by a bitopic membrane protein MapZ (mid-cell-anchored protein Z) through direct interactions between the intracellular domain (termed MapZ-N (the intracellular domain of MapZ)) and FtsZ. Using nuclear magnetic resonance titration experiments, we clearly assigned the key residues involved in the interactions. In the presence of MapZ-N, FtsZ gains a shortened activation delay, a lower critical concentration for polymerization and a higher cooperativity towards GTP hydrolysis. On the other hand, MapZ-N antagonizes the lateral interactions of single-stranded filaments of FtsZ, thus slows down the formation of highly bundled FtsZ polymers and eventually maintains FtsZ at a dynamic state. Altogether, we conclude that MapZ is not only an accelerator to trigger the polymerization of FtsZ, but also a brake to tune the velocity to form the end-product, FtsZ bundles. These findings suggest that MapZ is a multi-functional regulator towards FtsZ that controls both the precise positioning and proper timing of FtsZ polymerization.
- Published
- 2019
59. F-CphI represents a new homing endonuclease family using the Endo VII catalytic motif
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Qinglu Zeng, Yong-Liang Jiang, Kim K.C. Li, and Xiaoting Fang
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Endonuclease VII ,0301 basic medicine ,Genetics ,Tn3 transposon ,Multiple sequence alignment ,lcsh:QH426-470 ,Phylogenetic tree ,Research ,Cyanophage ,Biology ,biology.organism_classification ,Genome ,Homing endonuclease ,Bacteriophage ,lcsh:Genetics ,03 medical and health sciences ,Restriction enzyme ,030104 developmental biology ,biology.protein ,F-CphI ,Group I intron ,Molecular Biology - Abstract
Background There are six known families of homing endonucleases, LAGLIDADG, GIY-YIG, HNH, His-Cys box, PD-(D/E)-XK, and EDxHD, which are characterized by their conserved residues. Previously, we discovered a novel homing endonuclease F-CphI encoded by ORF177 of cyanophage S-PM2. F-CphI does not resemble any characterized homing endonucleases. Instead, the C-terminus of F-CphI aligns well with the N-terminal catalytic domain of a Holliday junction DNA resolvase, phage T4 endonuclease VII (Endo VII). Results A PSI-BLAST search resulted in a total of 313 Endo VII motif–containing sequences in sequenced genomes. Multiple sequence alignment showed that the catalytically important residues of T4 Endo VII were all well conserved in these proteins. Our site-directed mutagenesis studies further confirmed that the catalytically important residues of T4 Endo VII were also essential for F-CphI activity, and thus F-CphI might use a similar protein fold as Endo VII for DNA cleavage. A phylogenetic tree of the Endo VII motif–containing sequences showed that putative resolvases grouped into one clade while putative homing endonucleases and restriction endonucleases grouped into another clade. Conclusions Based on the unique conserved residues, we proposed that F-CphI represents a new homing endonuclease family, which was named the DHHRN family. Our phylogenetic analysis could be used to predict the functions of many previously unknown proteins. Electronic supplementary material The online version of this article (10.1186/s13100-018-0132-5) contains supplementary material, which is available to authorized users.
- Published
- 2018
60. Crystal structure of the effector-binding domain of Synechococcus elongatus CmpR in complex with ribulose 1,5-bisphosphate
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Yong-Liang Jiang, Didel M Mahounga, and Hui Sun
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0301 basic medicine ,Cyanobacteria ,Stereochemistry ,Dimer ,Ribulose-Bisphosphate Carboxylase ,030106 microbiology ,Biophysics ,Biochemistry ,Protein Structure, Secondary ,Research Communications ,03 medical and health sciences ,chemistry.chemical_compound ,Bacterial Proteins ,Structural Biology ,Transcription (biology) ,Genetics ,Amino Acid Sequence ,Gene ,Ribulose 1,5-bisphosphate ,Binding Sites ,biology ,Effector ,Ribulose ,Condensed Matter Physics ,biology.organism_classification ,DNA-Binding Proteins ,030104 developmental biology ,chemistry ,Crystallization ,Binding domain - Abstract
The CO2-concentrating mechanism (CCM) has evolved to improve the efficiency of photosynthesis in autotrophic cyanobacteria. CmpR, a LysR-type transcriptional regulator (LTTR) from Synechococcus elongatus PCC 7942, was found to regulate CCM-related genes under low-CO2 conditions. Here, the dimeric structure of the effector-binding domain of CmpR (CmpR-EBD) in complex with the co-activator ribulose 1,5-bisphosphate (RuBP) is reported at 2.15 Å resolution. One RuBP molecule binds to the inter-domain cleft between the two subunits of the CmpR-EBD dimer. Structural comparison combined with sequence analyses demonstrated that CmpR-EBD has an overall structure similar to those of LTTRs of known structure, but possesses a distinctly different effector-binding pattern.
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- 2018
61. Structural and enzymatic analyses of Anabaena heterocyst-specific alkaline invertase InvB
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Ling-Yun Xia, Kun Cai, Yuxing Chen, Hai-Xi Hu, Cong-Zhao Zhou, Feng Yang, Jin Xie, and Yong-Liang Jiang
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0301 basic medicine ,Cyanobacteria ,Models, Molecular ,030106 microbiology ,Biophysics ,Biochemistry ,03 medical and health sciences ,Species Specificity ,Structural Biology ,Catalytic Domain ,Hydrolase ,Genetics ,Extreme environment ,Amino Acid Sequence ,Molecular Biology ,Conserved Sequence ,Phylogeny ,Heterocyst ,biology ,beta-Fructofuranosidase ,Chemistry ,Anabaena ,Cell Biology ,biology.organism_classification ,Invertase ,Nitrogen fixation ,bacteria ,Proteobacteria - Abstract
Anabaena sp. PCC 7120 encodes two alkaline/neutral invertases, namely InvA and InvB. Following our recently reported InvA structure, here we report the crystal structure of the heterocyst-specific InvB. Despite sharing an overall structure similar to InvA, InvB possesses a much higher catalytic activity. Structural comparisons of the catalytic pockets reveal that Arg430 of InvB adopts a different conformation, which may facilitate the deprotonation of the catalytic residue Glu415. We propose that the higher activity may be responsible for the vital role of InvB in heterocyst development and nitrogen fixation. Furthermore, phylogenetic analysis combined with activity assays also suggests the role of this highly conserved arginine in plants and cyanobacteria, as well as some proteobacteria living in highly extreme environments.
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- 2018
62. The GDP-switched GAF domain of DcpA modulates the concerted synthesis/hydrolysis of c-di-GMP in
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Hui-Jie, Chen, Na, Li, Ye, Luo, Yong-Liang, Jiang, Cong-Zhao, Zhou, Yuxing, Chen, and Qiong, Li
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Bacterial Proteins ,3',5'-Cyclic-GMP Phosphodiesterases ,Protein Conformation ,Hydrolysis ,Mycobacterium smegmatis ,Sequence Homology ,Protein Interaction Domains and Motifs ,Amino Acid Sequence ,Cyclic GMP ,Guanosine Diphosphate - Abstract
The second messenger c-di-GMP [bis-(3'-5')-cyclic dimeric guanosine monophosphate] plays a key role in bacterial growth, survival and pathogenesis, and thus its intracellular homeostasis should be finely maintained.
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- 2018
63. Crystallization and preliminary X-ray diffraction analysis of a putative carbon–carbon bond hydrolase fromMycobacterium abscessus103
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Yi Wu, Yong-Liang Jiang, Zhang Zhang, and Yong-Xing He
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Hydrolases ,Molecular Sequence Data ,Biophysics ,Pseudomonas fluorescens ,Mycobacterium abscessus ,Phloretin hydrolase ,Biochemistry ,Mycobacterium ,Research Communications ,law.invention ,chemistry.chemical_compound ,X-Ray Diffraction ,Structural Biology ,law ,Hydrolase ,Genetics ,Amino Acid Sequence ,Crystallization ,chemistry.chemical_classification ,biology ,Chemistry ,bacterial infections and mycoses ,Condensed Matter Physics ,biology.organism_classification ,Carbon ,Crystallography ,Carbon–carbon bond ,biological sciences ,X-ray crystallography ,health occupations ,Chromatography, Gel ,bacteria ,Lithium chloride - Abstract
The PhlG protein fromMycobacterium abscessus103 (mPhlG), which shares 30% sequence identity with phloretin hydrolase fromEubacterium ramulusand 38% sequence identity with 2,4-diacetylphloroglucinol hydrolase fromPseudomonas fluorescensPf-5, is a putative carbon–carbon bond hydrolase. Here, the expression, purification and crystallization of mPhlG are reported. Crystals were obtained using a precipitant consisting of 100 mMcitric acid pH 5.0, 1.0 Mlithium chloride, 8%(w/v) polyethylene glycol 6000. The crystals diffracted to 1.87 Å resolution and belonged to space groupP21, with unit-cell parametersa= 71.0,b= 63.4,c= 74.7 Å, α = 90.0, β = 103.2, γ = 90.0°. Assuming the presence of two mPhlG molecules in the asymmetric unit,VMwas calculated to be 2.5 Å3 Da−1, which corresponds to a solvent content of 50%.
- Published
- 2015
64. Defining the enzymatic pathway for polymorphic O-glycosylation of the pneumococcal serine-rich repeat protein PsrP
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Rong-Li Zhao, Hong-Bo Yang, Shiliang Wang, Hua Jin, Cong-Zhao Zhou, Yong-Liang Jiang, and Yuxing Chen
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0301 basic medicine ,Glycan ,Glycosylation ,030106 microbiology ,Protein domain ,Glycobiology and Extracellular Matrices ,Biology ,Biochemistry ,Serine ,03 medical and health sciences ,chemistry.chemical_compound ,Bacterial Proteins ,Protein Domains ,Glycosyltransferase ,Transferase ,Humans ,Molecular Biology ,Glycoproteins ,chemistry.chemical_classification ,Glycosyltransferases ,Cell Biology ,carbohydrates (lipids) ,030104 developmental biology ,Enzyme ,Streptococcus pneumoniae ,chemistry ,biology.protein ,Glycoprotein - Abstract
Protein O-glycosylation is an important post-translational modification in all organisms, but deciphering the specific functions of these glycans is difficult due to their structural complexity. Understanding the glycosylation of mucin-like proteins presents a particular challenge as they are modified numerous times with both the enzymes involved and the glycosylation patterns being poorly understood. Here we systematically explored the O-glycosylation pathway of a mucin-like serine-rich repeat protein PsrP from the human pathogen Streptococcus pneumoniae TIGR4. Previous works have assigned the function of 3 of the 10 glycosyltransferases thought to modify PsrP, GtfA/B, and Gtf3 as catalyzing the first two reactions to form a unified disaccharide core structure. We now use in vivo and in vitro glycosylation assays combined with hydrolytic activity assays to identify the glycosyltransferases capable of decorating this core structure in the third and fourth steps of glycosylation. Specifically, the full-length GlyE and GlyG proteins and the GlyD DUF1792 domain participate in both steps, whereas full-length GlyA and the GlyD GT8 domain catalyze only the fourth step. Incorporation of different sugars to the disaccharide core structure at multiple sites along the serine-rich repeats results in a highly polymorphic product. Furthermore, crystal structures of apo- and UDP-complexed GlyE combined with structural analyses reveal a novel Rossmann-fold "add-on" domain that we speculate to function as a universal module shared by GlyD, GlyE, and GlyA to forward the peptide acceptor from one enzyme to another. These findings define the complete glycosylation pathway of a bacterial glycoprotein and offer a testable hypothesis of how glycosyltransferase coordination facilitates glycan assembly.
- Published
- 2017
65. Crystal structure of juvenile hormone epoxide hydrolase from the silkwormBombyx mori
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Ning Jia, Jie-Pin Yang, Yuxing Chen, Cong-Zhao Zhou, Sheng Li, Yong-Liang Jiang, Chen Hu, Kang Zhou, and Wei-Fang Li
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biology ,Juvenile-hormone esterase ,Epoxide ,biology.organism_classification ,Biochemistry ,chemistry.chemical_compound ,chemistry ,Structural Biology ,Bombyx mori ,Microsomal epoxide hydrolase ,Juvenile hormone ,Hydrolase ,Catalytic triad ,Epoxide Hydrolases ,Molecular Biology - Abstract
The juvenile hormone (JH) is a kind of epoxidecontaining sesquiterpene ester secreted by a pair of corpora allatum behind the brain of insects.1 It controls the metamorphosis development of insects together with the ecdysone.2,3 Thus the synthesis and degradation of JH are tightly regulated in different development stages.4 The degradation of JH is catalyzed by two hydrolases, juvenile hormone epoxide hydrolase (JHEH) and juvenile hormone esterase. JHEH is responsible for opening the epoxide ring of JH to produce JH diol, whereas JHE catalyzes the removal of the methyl ester moiety of JH to form JH acid.5,6 JHEH belongs to the microsomal epoxide hydrolase (mEH) (EC 3.3.2.9) family, which is one of the most widely distributed families of epoxide hydrolases (EHs). EHs can transform epoxides to compounds with decreased chemical reactivity, increased water solubility, and altered biological activity.7,8 In addition to participating in the catabolism of JH in insects, mEHs also play important roles in cytoprotection, steroid metabolism, bile acid transport, and xenobiotic metabolism.9 To date, the only structure of the mEH from the fungus Aspergillus niger (termed AnEH, PDB 1QO7) revealed a typical a/b-hydrolase core composed of a twisted eightstranded b-sheet packing on both sides with several a-helices.10,11 Structural analyses suggested a bimolecular nucleophilic substitution (SN2) reaction mechanism involving a standard nucleophile–histidine–acid catalytic triad of Asp–His–Glu/Asp.11 However, the mechanism of substrate recognition and catalysis of mEHs remains unclear. Here we report the crystal structure of Bombyx mori JHEH (BmJHEH) at 2.30 A resolution. Structural analyses together with molecular simulation reveal insights into the specific binding of JH in the active-site pocket. These findings increase our understanding of the substrate recognition and catalysis of mEHs and might help the design of JH-derived pesticides.
- Published
- 2014
66. Structure of a Novel O-Linked N-Acetyl-d-glucosamine (O-GlcNAc) Transferase, GtfA, Reveals Insights into the Glycosylation of Pneumococcal Serine-rich Repeat Adhesins
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Yan Min Ren, Qiuyan Shao, Fan Zhu, Wei Wei Shi, Hui Wu, Yong-Liang Jiang, Cong-Zhao Zhou, Yi Hu Yang, Hong-Bo Yang, and Yuxing Chen
- Subjects
Glycosylation ,Crystallography, X-Ray ,O-GlcNAc transferase ,Biochemistry ,Serine ,chemistry.chemical_compound ,stomatognathic system ,Multienzyme Complexes ,Glycosyltransferase ,Transferase ,Adhesins, Bacterial ,Protein Structure, Quaternary ,Molecular Biology ,Transaminases ,chemistry.chemical_classification ,biology ,Cell Biology ,In vitro ,Protein Structure, Tertiary ,Bacterial adhesin ,stomatognathic diseases ,Streptococcus pneumoniae ,Enzyme ,chemistry ,Protein Structure and Folding ,biology.protein - Abstract
Protein glycosylation catalyzed by the O-GlcNAc transferase (OGT) plays a critical role in various biological processes. In Streptococcus pneumoniae, the core enzyme GtfA and co-activator GtfB form an OGT complex to glycosylate the serine-rich repeat (SRR) of adhesin PsrP (pneumococcal serine-rich repeat protein), which is involved in the infection and pathogenesis. Here we report the 2.0 Å crystal structure of GtfA, revealing a β-meander add-on domain beyond the catalytic domain. It represents a novel add-on domain, which is distinct from the all-α-tetratricopeptide repeats in the only two structure-known OGTs. Structural analyses combined with binding assays indicate that this add-on domain contributes to forming an active GtfA-GtfB complex and recognizing the acceptor protein. In addition, the in vitro glycosylation system enables us to map the O-linkages to the serine residues within the first SRR of PsrP. These findings suggest that fusion with an add-on domain might be a universal mechanism for diverse OGTs that recognize varying acceptor proteins/peptides.
- Published
- 2014
67. Structural and biochemical analyses of Microcystis aeruginosa O-acetylserine sulfhydrylases reveal a negative feedback regulation of cysteine biosynthesis
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Bo-Ying Xu, Yuxing Chen, Wang Cheng, Kang Zhou, Mo Lu, Yong-Liang Jiang, and Cong-Zhao Zhou
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Models, Molecular ,Microcystis ,Protein Conformation ,Stereochemistry ,Molecular Sequence Data ,Biophysics ,Cystine ,Biology ,Crystallography, X-Ray ,Biochemistry ,Analytical Chemistry ,chemistry.chemical_compound ,Catalytic Domain ,Microcystis aeruginosa ,Amino Acid Sequence ,Cysteine ,Cloning, Molecular ,Binding site ,Molecular Biology ,Gene ,Feedback, Physiological ,chemistry.chemical_classification ,Cysteine Synthase ,Sequence Homology, Amino Acid ,Substrate (chemistry) ,Molecular Sequence Annotation ,biology.organism_classification ,Enzyme ,chemistry ,O-Acetylserine ,Bacteria - Abstract
article i nfo O-acetylserine sulfhydrylase (OASS) catalyzes the final step of cysteine biosynthesis from O-acetylserine (OAS) and inorganic sulfide in plants and bacteria. Bioinformatics analyses combined with activity assays enabled us to annotate the two putative genes of Microcystis aeruginosa PCC 7806 to CysK1 and CysK2, which encode the two 75% sequence-identical OASS paralogs. Moreover, we solved the crystal structures of CysK1 at 2.30 Ǻ and cystine-complexed CysK2 at 1.91 Ǻ, revealing a quite similar overall structure that belongs to the family of fold-type II PLP-dependent enzymes. Structural comparison indicated a significant induced fi tu pon binding to the cystine, which occupies the binding site for the substrate OAS and blocks the product release tunnel. Subsequent enzymatic assays further confirmed that cystine is a competitive inhibitor of the substrate OAS. Moreover, multiple-sequence alignment revealed that the cystine-binding residues are highly conserved in all OASS proteins, suggesting that this auto-inhibition of cystine might be a universal mechanism of cysteine biosynthesis pathway.
- Published
- 2014
68. Capsid Structure of a Freshwater Cyanophage Siphoviridae Mic1
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Ke Zhou, Wei-Fang Li, Feng Yang, Yong-Liang Jiang, Yuxing Chen, Hua Jin, Jue Ju, Jun-Tao Zhang, and Cong-Zhao Zhou
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Models, Molecular ,Cyanobacteria ,Protein Folding ,Microcystis ,Protein Conformation ,viruses ,Siphoviridae ,03 medical and health sciences ,Protein Domains ,Structural Biology ,Cyanophages ,Molecular Biology ,030304 developmental biology ,0303 health sciences ,biology ,Chemistry ,Cryoelectron Microscopy ,030302 biochemistry & molecular biology ,Capsomere ,Cyanophage ,biology.organism_classification ,Capsid ,Global distribution ,Biophysics ,Capsid Proteins ,Protein Multimerization ,Microcystis wesenbergii - Abstract
Cyanobacteria are the most abundant photosynthetic microorganisms, the global distribution of which is mainly regulated by the corresponding cyanophages. A systematic screening of water samples in the Lake Chaohu enabled us to isolate a freshwater siphocyanophage that infects Microcystis wesenbergii, thus termed Mic1. Using cryoelectron microscopy, we solved the 3.5-Å structure of Mic1 capsid. The major capsid protein gp40 of an HK97-like fold forms two types of capsomers, hexons and pentons. The capsomers interact with each other via the interweaved N-terminal arms of gp40 in addition to a tail-in-mouth joint along the three-fold symmetric axis, resulting in the assembly of capsid in a mortise-and-tenon pattern. The novel-fold cement protein gp47 sticks at the two-fold symmetric axis and further fixes the capsid. These findings provide structural insights into the assembly of cyanophages, and set up a platform to explore the mechanism of specific interactions and co-evolution with cyanobacteria.
- Published
- 2019
69. Rubisco accumulation factor 1 (Raf1) plays essential roles in mediating Rubisco assembly and carboxysome biogenesis.
- Author
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Fang Huang, Wen-Wen Kong, Yaqi Sun, Taiyu Chen, Dykes, Gregory F., Yong-Liang Jiang, and Lu-Ning Liu
- Subjects
ORGANELLE formation ,SYNECHOCOCCUS elongatus ,CELL growth ,CARBON fixation ,CAPSIDS - Abstract
Carboxysomes are membrane-free organelles for carbon assimilation in cyanobacteria. The carboxysome consists of a proteinaceous shell that structurally resembles virus capsids and internal enzymes including ribulose 1,5-bisphosphate carboxylase/oxygenase (Rubisco), the primary carbon-fixing enzyme in photosynthesis. The formation of carboxysomes requires hierarchical self-assembly of thousands of protein subunits, initiated from Rubisco assembly and packaging to shell encapsulation. Here we study the role of Rubisco assembly factor 1 (Raf1) in Rubisco assembly and carboxysome formation in a model cyanobacterium, Synechococcus elongatus PCC7942 (Syn7942). Cryo-electron microscopy reveals that Raf1 facilitates Rubisco assembly by mediating RbcL dimer formation and dimer-dimer interactions. Syn7942 cells lacking Raf1 are unable to form canonical intact carboxysomes but generate a large number of intermediate assemblies comprising Rubisco, CcaA, CcmM, and CcmN without shell encapsulation and a low abundance of carboxysome-like structures with reduced dimensions and irregular shell shapes and internal organization. As a consequence, the Raf1-depleted cells exhibit reduced Rubisco content, CO2-fixing activity, and cell growth. Our results provide mechanistic insight into the chaperone-assisted Rubisco assembly and biogenesis of carboxysomes. Advanced understanding of the biogenesis and stepwise formation process of the biogeochemically important organelle may inform strategies for heterologous engineering of functional CO2-fixing modules to improve photosynthesis. [ABSTRACT FROM AUTHOR]
- Published
- 2020
- Full Text
- View/download PDF
70. Structures of Yeast Apa2 Reveal Catalytic Insights into a Canonical Ap4A Phosphorylase of the Histidine Triad Superfamily
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Yuxing Chen, Wen-Zhe Li, Wen-Tao Hou, Cong-Zhao Zhou, and Yong-Liang Jiang
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Ap4A phosphorylase ,chemistry.chemical_classification ,crystal structure ,HIT superfamily ,substrate specificity ,enzymatic activity ,Saccharomyces cerevisiae ,Protein Data Bank (RCSB PDB) ,computer.file_format ,Biology ,Protein Data Bank ,biology.organism_classification ,Antiparallel (biochemistry) ,Yeast ,Enzyme ,Biochemistry ,chemistry ,Structural Biology ,Transferase ,Molecular Biology ,computer ,Histidine - Abstract
The homeostasis of intracellular diadenosine 5',5″'-P(1),P(4)-tetraphosphate (Ap4A) in the yeast Saccharomyces cerevisiae is maintained by two 60% sequence-identical paralogs of Ap4A phosphorylases (Apa1 and Apa2). Enzymatic assays show that, compared to Apa1, Apa2 has a relatively higher phosphorylase activity towards Ap3A (5',5″'-P(1),P(3)-tetraphosphate), Ap4A, and Ap5A (5',5″'-P(1),P(5)-tetraphosphate), and Ap4A is the favorable substrate for both enzymes. To decipher the catalytic insights, we determined the crystal structures of Apa2 in the apo-, AMP-, and Ap4A-complexed forms at 2.30, 2.80, and 2.70A resolution, respectively. Apa2 is an α/β protein with a core domain of a twisted eight-stranded antiparallel β-sheet flanked by several α-helices, similar to the galactose-1-phosphate uridylyltransferase (GalT) members of the histidine triad (HIT) superfamily. However, a unique auxiliary domain enables an individual Apa2 monomer to possess an intact substrate-binding cleft, which is distinct from previously reported dimeric GalT proteins. This cleft is perfectly complementary to the favorable substrate Ap4A, the AMP and ATP moieties of which are perpendicular to each other, leaving the α-phosphate group exposed at the sharp turn against the catalytic residue His161. Structural comparisons combined with site-directed mutagenesis and activity assays enable us to define the key residues for catalysis. Furthermore, multiple-sequence alignment reveals that Apa2 and homologs represent canonical Ap4A phosphorylases, which could be grouped as a unique branch in the GalT family.
- Published
- 2013
71. Structural Insights into the Substrate Specificity of a 6-Phospho-β-glucosidase BglA-2 from Streptococcus pneumoniae TIGR4
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Wei-Li Yu, Andreas Pikis, Yong-Liang Jiang, John F. Thompson, Yan-Min Ren, Cong-Zhao Zhou, Xiao-Hui Bai, Wang Cheng, and Yuxing Chen
- Subjects
Stereochemistry ,Mutation, Missense ,Cellobiose ,Crystallography, X-Ray ,Biochemistry ,Protein Structure, Secondary ,Substrate Specificity ,Structure-Activity Relationship ,chemistry.chemical_compound ,Bacterial Proteins ,Catalytic Domain ,Hydrolase ,Molecular Biology ,Alanine ,chemistry.chemical_classification ,Glycoside hydrolase family 1 ,biology ,Tryptophan ,Active site ,Cell Biology ,Streptococcus pneumoniae ,Enzyme ,Amino Acid Substitution ,chemistry ,Protein Structure and Folding ,biology.protein ,Glucosidases - Abstract
The 6-phospho-β-glucosidase BglA-2 (EC 3.2.1.86) from glycoside hydrolase family 1 (GH-1) catalyzes the hydrolysis of β-1,4-linked cellobiose 6-phosphate (cellobiose-6'P) to yield glucose and glucose 6-phosphate. Both reaction products are further metabolized by the energy-generating glycolytic pathway. Here, we present the first crystal structures of the apo and complex forms of BglA-2 with thiocellobiose-6'P (a non-metabolizable analog of cellobiose-6'P) at 2.0 and 2.4 Å resolution, respectively. Similar to other GH-1 enzymes, the overall structure of BglA-2 from Streptococcus pneumoniae adopts a typical (β/α)8 TIM-barrel, with the active site located at the center of the convex surface of the β-barrel. Structural analyses, in combination with enzymatic data obtained from site-directed mutant proteins, suggest that three aromatic residues, Tyr(126), Tyr(303), and Trp(338), at subsite +1 of BglA-2 determine substrate specificity with respect to 1,4-linked 6-phospho-β-glucosides. Moreover, three additional residues, Ser(424), Lys(430), and Tyr(432) of BglA-2, were found to play important roles in the hydrolytic selectivity toward phosphorylated rather than non-phosphorylated compounds. Comparative structural analysis suggests that a tryptophan versus a methionine/alanine residue at subsite -1 may contribute to the catalytic and substrate selectivity with respect to structurally similar 6-phospho-β-galactosidases and 6-phospho-β-glucosidases assigned to the GH-1 family.
- Published
- 2013
72. Structural Analysis of the Catalytic Mechanism and Substrate Specificity of Anabaena Alkaline Invertase InvA Reveals a Novel Glucosidase
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Jin Xie, Kun Cai, Hai-Xi Hu, Yong-Liang Jiang, Feng Yang, Peng-Fei Hu, Dong-Dong Cao, Wei-Fang Li, Yuxing Chen, and Cong-Zhao Zhou
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0301 basic medicine ,Sucrose ,Fructose ,Biology ,Random hexamer ,Crystallography, X-Ray ,Biochemistry ,Enzyme catalysis ,03 medical and health sciences ,chemistry.chemical_compound ,Bacterial Proteins ,Protein Domains ,Hydrolase ,Glycoside hydrolase ,Molecular Biology ,beta-Fructofuranosidase ,Substrate (chemistry) ,Cell Biology ,biochemical phenomena, metabolism, and nutrition ,Anabaena ,030104 developmental biology ,Invertase ,Glucose ,chemistry ,Protein Structure and Folding ,biology.protein ,Glucosidases - Abstract
Invertases catalyze the hydrolysis of sucrose to glucose and fructose, thereby playing a key role in primary metabolism and plant development. According to the optimum pH, invertases are classified into acid invertases (Ac-Invs) and alkaline/neutral invertases (A/N-Invs), which share no sequence homology. Compared with Ac-Invs that have been extensively studied, the structure and catalytic mechanism of A/N-Invs remain unknown. Here we report the crystal structures of Anabaena alkaline invertase InvA, which was proposed to be the ancestor of modern plant A/N-Invs. These structures are the first in the GH100 family. InvA exists as a hexamer in both crystal and solution. Each subunit consists of an (α/α)6 barrel core structure in addition to an insertion of three helices. A couple of structures in complex with the substrate or products enabled us to assign the subsites -1 and +1 specifically binding glucose and fructose, respectively. Structural comparison combined with enzymatic assays indicated that Asp-188 and Glu-414 are putative catalytic residues. Further analysis of the substrate binding pocket demonstrated that InvA possesses a stringent substrate specificity toward the α1,2-glycosidic bond of sucrose. Together, we suggest that InvA and homologs represent a novel family of glucosidases.
- Published
- 2016
73. Structural Comparison and Simulation of Pneumococcal Peptidoglycan Hydrolase LytB
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Xiao-Hui, Bai, Qiong, Li, Yong-Liang, Jiang, Jing-Ren, Zhang, Yuxing, Chen, and Cong-Zhao, Zhou
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Models, Molecular ,Protein Conformation ,N-Acetylmuramoyl-L-alanine Amidase ,Crystallography, X-Ray ,Substrate Specificity ,Molecular Docking Simulation ,Streptococcus pneumoniae ,Bacterial Proteins ,Structural Homology, Protein ,Catalytic Domain ,Mutagenesis, Site-Directed ,Computer Simulation ,Oligopeptides ,Protein Binding - Abstract
Three-dimensional structural determination combined with comprehensive comparisons with the homologs is a straightforward strategy to decipher the molecular function of an enzyme. However, in many cases it's difficult to obtain the complex structure with the substrate/ligand. Structure-based molecular simulation provides an alternative solution to predict the binding pattern of a substrate/ligand to the enzyme. The Streptococcus pneumoniae LytB is a peptidoglycan hydrolase that cleaves the glycosidic bond and therefore involves the cell division; however, the details of catalytic mechanism remain unknown. Based on the crystal structure of the catalytic domain of LytB (termed LytBCAT), we describe here how to assign the molecular functions of three LytBCAT modules: SH3b, WW, and GH73, using structural comparisons. Moreover, we dock a putative tetrasaccharide-pentapeptide substrate of peptidoglycan onto LytBCAT to provide the details of substrate binding pattern. The tetrasaccharide-pentapeptide is well accommodated in a T-shaped substrate binding pocket formed by the three modules. The conclusions deduced from structural comparison and simulation are further proved by the hydrolytic activity assays in combination with site-directed mutagenesis.
- Published
- 2016
74. Structure of a variable lymphocyte receptor-like protein from the amphioxus Branchiostoma floridae
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Cong-Zhao Zhou, Yong-Liang Jiang, Yuxing Chen, Jun-Yuan Chen, Wang Cheng, Dong-Dong Cao, Wen-Jie Wang, Qiong Li, and Xin Liao
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Gills ,Models, Molecular ,0301 basic medicine ,Protein Conformation ,Chordate ,Peptidoglycan ,Article ,Conserved sequence ,03 medical and health sciences ,Protein structure ,Variable lymphocyte receptor ,Branchiostoma floridae ,Animals ,Amino Acid Sequence ,Peptide sequence ,Conserved Sequence ,Lancelets ,Genetics ,Multidisciplinary ,biology ,Lamprey ,T-cell receptor ,Computational Biology ,biology.organism_classification ,Receptors, Antigen ,030104 developmental biology ,Protein Binding - Abstract
Discovery of variable lymphocyte receptors (VLRs) in agnathans (jawless fish) has brought the origin of adaptive immunity system (AIS) forward to 500 million years ago accompanying with the emergence of vertebrates. Previous findings indicated that amphioxus, a representative model organism of chordate, also possesses some homologs of the basic components of TCR/BCR-based AIS, but it remains unknown if there exist any components of VLR-based AIS in amphioxus. Bioinformatics analyses revealed the amphioxus Branchiostoma floridae encodes a group of putative VLR-like proteins. Here we reported the 1.79 Å crystal structure of Bf66946, which forms a crescent-shaped structure of five leucine-rich repeats (LRRs). Structural comparisons indicated that Bf66946 resembles the lamprey VLRC. Further electrostatic potential analyses showed a negatively-charged patch at the concave of LRR solenoid structure that might be responsible for antigen recognition. Site-directed mutagenesis combined with bacterial binding assays revealed that Bf66946 binds to the surface of Gram-positive bacteria Staphylococcus aureus and Streptococcus pneumonia via a couple of acidic residues at the concave. In addition, the closest homolog of Bf66946 is highly expressed in the potential immune organ gill of Branchiostoma belcheri. Altogether, our findings provide the first structural evidence for the emergence of VLR-like molecules in the basal chordates.
- Published
- 2016
75. Structural Comparison and Simulation of Pneumococcal Peptidoglycan Hydrolase LytB
- Author
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Yong-Liang Jiang, Yuxing Chen, Jing-Ren Zhang, Cong-Zhao Zhou, Qiong Li, and Xiao-Hui Bai
- Subjects
0301 basic medicine ,chemistry.chemical_classification ,Stereochemistry ,Substrate (chemistry) ,Glycosidic bond ,Plasma protein binding ,Ligand (biochemistry) ,Molecular Docking Simulation ,03 medical and health sciences ,chemistry.chemical_compound ,030104 developmental biology ,Protein structure ,chemistry ,Peptidoglycan ,N-acetylmuramoyl-L-alanine amidase - Abstract
Three-dimensional structural determination combined with comprehensive comparisons with the homologs is a straightforward strategy to decipher the molecular function of an enzyme. However, in many cases it's difficult to obtain the complex structure with the substrate/ligand. Structure-based molecular simulation provides an alternative solution to predict the binding pattern of a substrate/ligand to the enzyme. The Streptococcus pneumoniae LytB is a peptidoglycan hydrolase that cleaves the glycosidic bond and therefore involves the cell division; however, the details of catalytic mechanism remain unknown. Based on the crystal structure of the catalytic domain of LytB (termed LytBCAT), we describe here how to assign the molecular functions of three LytBCAT modules: SH3b, WW, and GH73, using structural comparisons. Moreover, we dock a putative tetrasaccharide-pentapeptide substrate of peptidoglycan onto LytBCAT to provide the details of substrate binding pattern. The tetrasaccharide-pentapeptide is well accommodated in a T-shaped substrate binding pocket formed by the three modules. The conclusions deduced from structural comparison and simulation are further proved by the hydrolytic activity assays in combination with site-directed mutagenesis.
- Published
- 2016
76. Structural basis for receptor recognition and pore formation of a zebrafish aerolysin‐like protein
- Author
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Ning Jia, Yonghui Zhang, Gang Cai, Junhui Peng, Zhihui Zhang, Xuejuan Wang, Nan Liu, Meng-Qiu Dong, Hui Wu, Lan Lan Chen, Yuxing Chen, Yue He Ding, Cong-Zhao Zhou, Hong-Wei Wang, Hui Sun, Zhiyong Zhang, Junfeng Wang, Yong-Liang Jiang, and Wang Cheng
- Subjects
0301 basic medicine ,Pore Forming Cytotoxic Proteins ,Protein subunit ,Bacterial Toxins ,Molecular Sequence Data ,Danio ,Aerolysin ,Plasma protein binding ,Biology ,Molecular Dynamics Simulation ,Biochemistry ,Pore forming protein ,Mannans ,03 medical and health sciences ,Lectins ,Genetics ,Animals ,Amino Acid Sequence ,Molecular Biology ,Zebrafish ,Peptide sequence ,Lectin ,Articles ,Zebrafish Proteins ,biology.organism_classification ,Cell biology ,Protein Structure, Tertiary ,030104 developmental biology ,biology.protein ,Protein Binding - Abstract
Various aerolysin-like pore-forming proteins have been identified from bacteria to vertebrates. However, the mechanism of receptor recognition and/or pore formation of the eukaryotic members remains unknown. Here, we present the first crystal and electron microscopy structures of a vertebrate aerolysin-like protein from Danio rerio, termed Dln1, before and after pore formation. Each subunit of Dln1 dimer comprises a β-prism lectin module followed by an aerolysin module. Specific binding of the lectin module toward high-mannose glycans triggers drastic conformational changes of the aerolysin module in a pH-dependent manner, ultimately resulting in the formation of a membrane-bound octameric pore. Structural analyses combined with computational simulations and biochemical assays suggest a pore-forming process with an activation mechanism distinct from the previously characterized bacterial members. Moreover, Dln1 and its homologs are ubiquitously distributed in bony fishes and lamprey, suggesting a novel fish-specific defense molecule.
- Published
- 2015
77. Assessments of different kinds of sham acupuncture applied in randomized controlled trials
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Yong-Qing Yang, Chun-Xiao Shan, Ying Wei, Xiao-Yan Liu, Jun Ran, Yu-Dong Xu, Yu Wang, Lei-Miao Yin, Yong-Liang Jiang, and Yan-Yan Liu
- Subjects
medicine.medical_specialty ,business.industry ,Therapeutic effect ,Placebo ,law.invention ,Physical medicine and rehabilitation ,Complementary and alternative medicine ,Randomized controlled trial ,law ,Acupuncture ,Physical therapy ,medicine ,Acupuncture therapy ,Sham acupuncture ,business - Abstract
Objective Different kinds of sham acupuncture are widely applied in randomized controlled trials (RCTs) to explore whether acupuncture has intrinsic therapeutic effects beyond the placebo effects for certain indication. To make conclusions of trials more comparable and convincing, it is of great necessity to unify the sham acupuncture procedure.
- Published
- 2011
78. Structural and Biochemical Characterization of Yeast Monothiol Glutaredoxin Grx6
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Yuxing Chen, Cong-Zhao Zhou, Yong-Xing He, Yajun Tang, Jiang Yu, Xiao-Xiao Ma, Rongguang Zhang, Yong-Liang Jiang, and Ming Luo
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Models, Molecular ,Signal peptide ,Saccharomyces cerevisiae Proteins ,Molecular Sequence Data ,Saccharomyces cerevisiae ,Biology ,Crystallography, X-Ray ,chemistry.chemical_compound ,symbols.namesake ,Structural Biology ,Glutaredoxin ,Humans ,Amino Acid Sequence ,Protein Structure, Quaternary ,Molecular Biology ,Glutaredoxins ,Glutathione Disulfide ,Endoplasmic reticulum ,Glutathione ,Golgi apparatus ,biology.organism_classification ,Protein Structure, Tertiary ,Glutathione S-transferase ,chemistry ,Biochemistry ,biology.protein ,symbols ,Glutathione-disulfide reductase activity ,Dimerization ,Oxidation-Reduction ,Sequence Alignment - Abstract
Glutaredoxins (Grxs) are a ubiquitous family of proteins that reduce disulfide bonds in substrate proteins using electrons from reduced glutathione (GSH). The yeast Saccharomyces cerevisiae Grx6 is a monothiol Grx that is localized in the endoplasmic reticulum and Golgi compartments. Grx6 consists of three segments, a putative signal peptide (M1-I36), an N-terminal domain (K37-T110), and a C-terminal Grx domain (K111-N231, designated Grx6C). Compared to the classic dithiol glutaredoxin Grx1, Grx6 has a lower glutathione disulfide reductase activity but a higher glutathione S-transferase activity. In addition, similar to human Grx2, Grx6 binds GSH via an iron–sulfur cluster in vitro. The N-terminal domain is essential for noncovalent dimerization, but not required for either of the above activities. The crystal structure of Grx6C at 1.5 A resolution revealed a novel two-strand antiparallel β-sheet opposite the GSH binding groove. This extra β-sheet might also exist in yeast Grx7 and in a group of putative Grxs in lower organisms, suggesting that Grx6 might represent the first member of a novel Grx subfamily.
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- 2010
79. Structures of yeast glutathione‐ S ‐transferase Gtt2 reveal a new catalytic type of GST family
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Yuxing Chen, Rui Bao, Yong-Xing He, Xiao-Xiao Ma, Yong-Liang Jiang, and Cong-Zhao Zhou
- Subjects
Models, Molecular ,Scientific Report ,Molecular Sequence Data ,Saccharomyces cerevisiae ,Crystallography, X-Ray ,Biochemistry ,Catalysis ,Protein Structure, Secondary ,Serine ,chemistry.chemical_compound ,Cytosol ,Protein structure ,Sequence Analysis, Protein ,Genetics ,Transferase ,Amino Acid Sequence ,Site-directed mutagenesis ,Molecular Biology ,Glutathione Transferase ,Alanine ,Sequence Homology, Amino Acid ,biology ,Glutathione ,biology.organism_classification ,Glutathione S-transferase ,chemistry ,Multigene Family ,biology.protein ,Mutant Proteins - Abstract
Glutathione-S-transferases (GSTs) are ubiquitous detoxification enzymes that catalyse the conjugation of electrophilic substrates to glutathione. Here, we present the crystal structures of Gtt2, a GST of Saccharomyces cerevisiae, in apo and two ligand-bound forms, at 2.23 A, 2.20 A and 2.10 A, respectively. Although Gtt2 has the overall structure of a GST, the absence of the classic catalytic essential residues--tyrosine, serine and cysteine--distinguishes it from all other cytosolic GSTs of known structure. Site-directed mutagenesis in combination with activity assays showed that instead of the classic catalytic residues, a water molecule stabilized by Ser129 and His123 acts as the deprotonator of the glutathione sulphur atom. Furthermore, only glycine and alanine are allowed at the amino-terminus of helix-alpha1 because of stereo-hindrance. Taken together, these results show that yeast Gtt2 is a novel atypical type of cytosolic GST.
- Published
- 2009
80. Crystal structure ofArabidopsistranslation initiation factor eIF-5A2
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Xiao-Xiao Ma, Yan-Bin Teng, Yuxing Chen, Yong-Xing He, Cheng-Bin Xiang, Jin Du, Cong-Zhao Zhou, and Yong-Liang Jiang
- Subjects
eIF2 ,biology ,Chemistry ,EIF4A1 ,biology.organism_classification ,Biochemistry ,Eukaryotic translation initiation factor 4 gamma ,Cell biology ,Internal ribosome entry site ,Eukaryotic translation ,Structural Biology ,Eukaryotic initiation factor ,Arabidopsis ,Initiation factor ,Molecular Biology - Published
- 2009
81. [Therapeutic effect and safety of microendoscopic discectomy versus conventional open discectomy for the treatment of lumbar disc herniation: a Meta analysis]
- Author
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Xiao-Ming, Ying, Yong-Liang, Jiang, Peng, Xu, Peng, Wang, Bo, Zhu, and Shao-Qing, Guo
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China ,Microsurgery ,Lumbar Vertebrae ,Postoperative Complications ,Treatment Outcome ,Incidence ,Blood Loss, Surgical ,Humans ,Endoscopy ,Length of Stay ,Intervertebral Disc Displacement ,Diskectomy - Abstract
To conduct a meta analysis of studies comparing theapeutic effect and safety of microendoscopic discectomy to conventional open discectomy in the treatment of lumbar disc herniation in China.A systematic literature retrieval was conducted in the Chinese Bio medicine Database, CNKI database, Chongqin VIP database and Wangfang database. The statistical analysis was performed using a RevMan 4.2 software. The comparison included excellent rate, operation times, blood loss, periods of bed rest and resuming daily activities, hospital stay or hospital stay after surgery, and complications of microendoscopic discectomy versus conventional open discectomy.The search yielded 20 reports, which included 2 957 cases treated by microendoscopic discectomy and 2 130 cases treated by conventional open discectomy. There were 12, 11, 7, 5, 4 and 4 reports which had comparison of operation times, blood loss, period of bed rest, periods of resuming daily activities, hospital stay and hospital stay after surgery respectively. Complications were mentioned in 10 reports. Compared to patients treated by open discectomy, patients treated by microendoscopic discectomy had a higher excellent rates [OR=1.29, 95%CI (1.03, 1.62)], less blood loss[OR=-63.67, 95%CI (-86.78, -40.55)], less period of bed rest[OR=-15.33, 95%CI (-17.76, -12.90)], less period of resumption of daily activities [OR=-24.41, 95%CI (-36.86, -11.96)], less hospital stay [OR=-5.00, 95%CI (-6.94, -3.06)] or hospital stay after surgery [OR=-7.47, 95%CI (-9.17, -5.77) respectively. However, incidence of complications and operation times were proved no significant different between microendoscopic discectomy and open discectomy.Microendoscopic discectomy and conventional open discectomy in treatment of lumbar disc herniation are both safe, effective; incidence of complications are nearly. Patients with lumbar disc herniation treated by microendoscopic discectomy have fewer blood loss, shorter periods of bed rest and hospital stay, and resume daily activities faster. Techniques are selected according to indications, microendoscopic discectomy should be carried out when conjunct indications occur.
- Published
- 2015
82. Structural insights into HetR−PatS interaction involved in cyanobacterial pattern formation
- Author
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Yan-Min Ren, Cong-Zhao Zhou, Changlin Tian, Junhui Peng, Cheng-Cai Zhang, Zhiyong Zhang, Yuxing Chen, Pei Lv, Hong-Mei Yu, Bin Wen, Hai-Xi Hu, Kun Cai, Sanling Liu, Meng-Xi Zhao, Yonghui Zhang, Hui Zhong, Yong-Liang Jiang, Qingfa Wu, Mikael Oliveberg, Key Laboratory of Tropical Forest Ecology, Xishuangbanna Tropical Botanical Garden, Shanghai public Health Clinical Center, Shanghai Medical College of Fudan University, Department of Plant Pathology & Microbiology [Riverside], University of California [Riverside] ( UCR ), Laboratoire de chimie bactérienne ( LCB ), Aix Marseille Université ( AMU ) -Centre National de la Recherche Scientifique ( CNRS ), Institut de Microbiologie de la Méditerranée ( IMM ), Laboratoire des Sciences du Climat et de l'Environnement [Gif-sur-Yvette] ( LSCE ), Université de Versailles Saint-Quentin-en-Yvelines ( UVSQ ) -Commissariat à l'énergie atomique et aux énergies alternatives ( CEA ) -Université Paris-Saclay-Centre National de la Recherche Scientifique ( CNRS ), Institut de biochimie et biophysique moléculaire et cellulaire ( IBBMC ), Université Paris-Sud - Paris 11 ( UP11 ) -Centre National de la Recherche Scientifique ( CNRS ), University of Science and Technology of China [Hefei] (USTC), Stockholm University, Laboratoire de chimie bactérienne (LCB), Aix Marseille Université (AMU)-Centre National de la Recherche Scientifique (CNRS), and Institut de Microbiologie de la Méditerranée (IMM)
- Subjects
Models, Molecular ,HMG-box ,Protein Conformation ,Protein subunit ,Plasma protein binding ,Biology ,Article ,[ SDE ] Environmental Sciences ,Structure-Activity Relationship ,03 medical and health sciences ,0302 clinical medicine ,Protein structure ,Bacterial Proteins ,Transcription (biology) ,Nucleotide Motifs ,Binding site ,Promoter Regions, Genetic ,[ SDV.BBM ] Life Sciences [q-bio]/Biochemistry, Molecular Biology ,Transcription factor ,030304 developmental biology ,Heterocyst ,Genetics ,0303 health sciences ,Binding Sites ,Multidisciplinary ,Base Sequence ,[SDV.BBM.BS]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Structural Biology [q-bio.BM] ,[ SDV.BC ] Life Sciences [q-bio]/Cellular Biology ,Anabaena ,[SDV.MP.BAC]Life Sciences [q-bio]/Microbiology and Parasitology/Bacteriology ,Cell biology ,Nucleic Acid Conformation ,[ SDV.GEN ] Life Sciences [q-bio]/Genetics ,030217 neurology & neurosurgery ,Protein Binding - Abstract
The one-dimensional pattern of heterocyst in the model cyanobacterium Anabaena sp. PCC 7120 is coordinated by the transcription factor HetR and PatS peptide. Here we report the complex structures of HetR binding to DNA and its hood domain (HetRHood) binding to a PatS-derived hexapeptide (PatS6) at 2.80 and 2.10 Å, respectively. The intertwined HetR dimer possesses a couple of novel HTH motifs, each of which consists of two canonical α-helices in the DNA-binding domain and an auxiliary α-helix from the flap domain of the neighboring subunit. Two PatS6 peptides bind to the lateral clefts of HetRHood and trigger significant conformational changes of the flap domain, resulting in dissociation of the auxiliary α-helix and eventually release of HetR from the DNA major grove. These findings provide the structural insights into a prokaryotic example of Turing model.
- Published
- 2015
83. Structural and enzymatic analyses of a glucosyltransferase Alr3699/HepE involved in Anabaena heterocyst envelop polysaccharide biosynthesis
- Author
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Cong-Zhao Zhou, Xue-Ping Wang, Yong-Liang Jiang, Yuxing Chen, Ya-Nan Dai, and Wang Cheng
- Subjects
0301 basic medicine ,chemistry.chemical_classification ,Uridine Diphosphate Glucose ,biology ,Operon ,Polysaccharides, Bacterial ,Biochemistry ,Anabaena ,03 medical and health sciences ,chemistry.chemical_compound ,Heterocyst differentiation ,030104 developmental biology ,Enzyme ,Biosynthesis ,chemistry ,Bacterial Proteins ,Protein Domains ,Glucosyltransferases ,Multigene Family ,Glycosyltransferase ,biology.protein ,Transferase ,Glucosyltransferase ,Heterocyst - Abstract
Formation of the heterocyst envelope polysaccharide (HEP) is a key process for cyanobacterial heterocyst differentiation. The maturation of HEP in Anabaena sp. strain PCC 7120 is controlled by a gene cluster termed HEP island in addition to an operon alr3698-alr3699, which encodes two putative proteins termed Alr3698/HepD and Alr3699/HepE. Here we report the crystal structures of HepE in the apo-form and three complex forms that bind to UDP-glucose (UDPG), UDP&glucose, and UDP, respectively. The overall structure of HepE displays a typical GT-B fold of glycosyltransferases, comprising two separate β/α/β Rossmann-fold domains that form an inter-domain substrate-binding crevice. Structural analyses combined with enzymatic assays indicate that HepE is a glucosyltransferase using UDPG as a sugar donor. Further site-directed mutageneses enable us to assign the key residues that stabilize the sugar donor and putative acceptor. Based on the comparative structural analyses, we propose a putative catalytic cycle of HepE, which undergoes "open-closed-open" conformational changes upon binding to the substrates and release of products. These findings provide structural and catalytic insights into the first enzyme involved in the HEP biosynthesis pathway.
- Published
- 2015
84. Structural and enzymatic characterization of the choline kinase LicA from Streptococcus pneumoniae
- Author
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Yuxing Chen, Cong-Zhao Zhou, Yong-Liang Jiang, Lei Wang, and Jing-Ren Zhang
- Subjects
chemistry.chemical_classification ,Conformational change ,Multidisciplinary ,Choline kinase ,biology ,Phosphorylcholine ,lcsh:R ,Rational design ,Active site ,lcsh:Medicine ,Crystallography, X-Ray ,Enzyme structure ,Protein Structure, Secondary ,Protein Structure, Tertiary ,Enzyme ,Streptococcus pneumoniae ,chemistry ,Biochemistry ,Bacterial Proteins ,biology.protein ,Transferase ,Choline Kinase ,lcsh:Q ,lcsh:Science ,Research Article - Abstract
LicA plays a key role in the cell-wall phosphorylcholine biosynthesis of Streptococcus pneumonia. Here we determined the crystal structures of apo-form LicA at 1.94 A and two complex forms LicA-choline and LicA-AMP-MES, at 2.01 and 1.45 A resolution, respectively. The overall structure adopts a canonical protein kinase-like fold, with the active site located in the crevice of the N- and C- terminal domains. The three structures present distinct poses of the active site, which undergoes an open-closed-open conformational change upon substrate binding and product release. The structure analyses combined with mutageneses and enzymatic assays enabled us to figure out the key residues for the choline kinase activity of LicA. In addition, structural comparison revealed the loop between helices α7 and α8 might modulate the substrate specificity and catalytic activity. These findings shed light on the structure and mechanism of the prokaryotic choline kinase LicA, and might direct the rational design of novel anti-pneumococcal drugs.
- Published
- 2015
85. Full-length structure of the major autolysin LytA
- Author
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David I. Roper, Cécile Morlot, Xiao-Hui Bai, Yuxing Chen, Wen-Jia Wang, Wang Cheng, Thierry Vernet, Yuhui Dong, Yong-Liang Jiang, Cong-Zhao Zhou, Qiong Li, University of Science and Technology of China [Hefei] (USTC), Institut de biologie structurale (IBS - UMR 5075 ), Université Grenoble Alpes [2016-2019] (UGA [2016-2019])-Institut de Recherche Interdisciplinaire de Grenoble (IRIG), Direction de Recherche Fondamentale (CEA) (DRF (CEA)), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Direction de Recherche Fondamentale (CEA) (DRF (CEA)), Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Centre National de la Recherche Scientifique (CNRS), Beijing Synchrotron Radiation Facility, Institute of High Energy Physics, University of Warwick [Coventry], Centre National de la Recherche Scientifique (CNRS)-Université Grenoble Alpes [2016-2019] (UGA [2016-2019])-Institut de Recherche Interdisciplinaire de Grenoble (IRIG), and Commissariat à l'énergie atomique et aux énergies alternatives (CEA)-Commissariat à l'énergie atomique et aux énergies alternatives (CEA)
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chemistry.chemical_classification ,Autolysis (biology) ,Protein Conformation ,Protein subunit ,[SDV]Life Sciences [q-bio] ,Autolysin ,Streptococcus ,General Medicine ,N-Acetylmuramoyl-L-alanine Amidase ,Biology ,Amidase ,chemistry.chemical_compound ,Enzyme ,Biochemistry ,chemistry ,Bacterial Proteins ,Structural Biology ,Cleave ,Hydrolase ,Peptidoglycan - Abstract
LytA is responsible for the autolysis of manyStreptococcusspecies, including pathogens such asS. pneumoniae,S. pseudopneumoniaeandS. mitis. However, how this major autolysin achieves full activity remains unknown. Here, the full-length structure of theS. pneumoniaeLytA dimer is reported at 2.1 Å resolution. Each subunit has an N-terminal amidase domain and a C-terminal choline-binding domain consisting of six choline-binding repeats, which form five canonical and one single-layered choline-binding sites. Site-directed mutageneses combined with enzymatic activity assays indicate that dimerization and binding to choline are two independent requirements for the autolytic activity of LytAin vivo. Altogether, it is suggested that dimerization and full occupancy of all choline-binding sites through binding to choline-containing TA chains enable LytA to adopt a fully active conformation which allows the amidase domain to cleave two lactyl-amide bonds located about 103 Å apart on the peptidoglycan.
- Published
- 2014
86. Multi-functional regulator MapZ controls both positioning and timing of FtsZ polymerization.
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Zhang Feng, Jiahai Zhang, Da Xu, Yong-Liang Jiang, Cong-Zhao Zhou, and Yuxing Chen
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POLYMERIZATION ,NUCLEAR magnetic resonance ,MEMBRANE proteins ,STREPTOCOCCUS pneumoniae ,CELL division - Abstract
The tubulin-like GTPase protein FtsZ, which forms a discontinuous cytokinetic ring at mid-cell, is a central player to recruit the division machinery to orchestrate cell division. To guarantee the production of two identical daughter cells, the assembly of FtsZ, namely Z-ring, and its precise positioning should be finely regulated. In Streptococcus pneumoniae, the positioning of Z-ring at the division site is mediated by a bitopic membrane protein MapZ (mid-cell-anchored protein Z) through direct interactions between the intracellular domain (termed MapZ-N (the intracellular domain of MapZ)) and FtsZ. Using nuclear magnetic resonance titration experiments, we clearly assigned the key residues involved in the interactions. In the presence of MapZ-N, FtsZ gains a shortened activation delay, a lower critical concentration for polymerization and a higher cooperativity towards GTP hydrolysis. On the other hand, MapZ-N antagonizes the lateral interactions of singlestranded filaments of FtsZ, thus slows down the formation of highly bundled FtsZ polymers and eventually maintains FtsZ at a dynamic state. Altogether, we conclude that MapZ is not only an accelerator to trigger the polymerization of FtsZ, but also a brake to tune the velocity to form the end-product, FtsZ bundles. These findings suggest that MapZ is a multi-functional regulator towards FtsZ that controls both the precise positioning and proper timing of FtsZ polymerization. [ABSTRACT FROM AUTHOR]
- Published
- 2019
- Full Text
- View/download PDF
87. Two-stage segment optimal packing of single size rectangles
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Zhi-qiang Yang, Yong-liang Jiang, and Cheng-yi Zhang
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Combinatorics ,Stage (hydrology) ,Mathematics - Published
- 2012
88. Attitudes Toward Advance Directives Among Patients and Their Family Members in China
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Yu Feng Du, Ou Bian, Fan Lin, Jie Ping Wang, Bao Cheng Yu, Xiao Hong Liu, Ye Shi, Hong Lian Zhou, Zhong Wang, Ting Gong, Ming Lei Zhu, Liang Kung Chen, Huai Hong Chen, Pei Yan Shan, Fang Liang, Lu Rong Hong, Hui Su, Jun Nan Yang, Huai Cong Long, Nan Wei, Xiao Hong Du, Yong Liang Jiang, Jing Ning, Hui Ling Lou, Lin Kang, Ping Zhong, Jing Zhang, Zhi Jun Chen, Wen He, and Xiao Hong Ning
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Male ,Advance care planning ,Mainland China ,China ,medicine.medical_specialty ,Patients ,media_common.quotation_subject ,Affect (psychology) ,Advance Care Planning ,03 medical and health sciences ,0302 clinical medicine ,Quality of life (healthcare) ,Surveys and Questionnaires ,Health care ,Humans ,Medicine ,Family ,030212 general & internal medicine ,General Nursing ,Aged ,media_common ,Aged, 80 and over ,business.industry ,Health Policy ,Do not resuscitate ,General Medicine ,Middle Aged ,Chinese people ,Cross-Sectional Studies ,Attitude ,030220 oncology & carcinogenesis ,Family medicine ,Female ,Geriatrics and Gerontology ,Advance Directives ,business ,Autonomy - Abstract
Objectives Chinese people are generally unfamiliar with the concept of advance care planning or advance directives (ACP/ADs), which raises dilemmas in life-support choice and can even affect clinical decision making. To understand and address the issues involved better, we investigated the awareness of ACP/ADs in China, as well as people's attitudes toward medical autonomy and end-of-life care. Design A multicenter cross-sectional survey, conducted from August 1 to December 31, 2016. Setting Twenty-five hospitals located in 15 different provinces throughout mainland China. Participants Pairs of adult patients without dementia or malignancies, and a family member. Measurements Participants self-filled anonymous questionnaires, and the data collected were analyzed to relate patients' sociodemographic characteristics to their awareness of ACP/ADs and attitudes to health care autonomy and end-of-life care. Results Among 1084 patients who completed the questionnaire, 415 (38.3%) had heard about ACP/ADs. Having been informed about ACP/ADs, 995 (91.8%) were willing to find out their true health status and decide for themselves; 549 (50.6%) wanted to institute ACP/ADs. Regarding end-of-life care, 473 (43.6%) chose Do Not Resuscitate, and 435 (40.1%) wished to forgo life-support treatment if irreversibly moribund. Patients predominantly (481, 44.4%) chose general hospital as their preferred place to spend their last days of life; only 114 (10.5%) favored a special hospice facility. Patients' main concerns during end-of-life care were symptom control (35.1%), followed by functional maintenance and quality of life (29.8%), and prolonging life (18.9%). More highly educated patients had significantly greater awareness of ACP/ADs than less well educated ones (χ 2 = 59.22, P 2 = 58.30, P ≤ .001) and make medical decisions in advance (χ 2 = 55.92, P 2 = 38.23, P = .001) and make medical decisions in advance (χ 2 = 18.42, P = .018), and were also more likely to wish to die at home (χ 2 = 96.25, P Conclusions Awareness about ACP/ADs in China is still low. Providing culturally sensitive knowledge, education, and communication regarding ACP/ADs is a feasible first step to promoting this sociomedical practice.
- Published
- 2017
89. Structure of the adenylation-peptidyl carrier protein didomain of the Microcystis aeruginosa microcystin synthetase McyG
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Yong-Liang Jiang, Yuxing Chen, Yan-Min Ren, Cong-Zhao Zhou, Kang Zhou, Ya-Nan Dai, and Xiao-Feng Tan
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Models, Molecular ,Microcystis ,Microcystins ,Stereochemistry ,Protein Conformation ,Molecular Sequence Data ,Peptide ,Microcystin ,Crystallography, X-Ray ,Ligases ,chemistry.chemical_compound ,Polyketide ,Biosynthesis ,Structural Biology ,Nonribosomal peptide ,Microcystis aeruginosa ,Amino Acid Sequence ,Adenylylation ,chemistry.chemical_classification ,biology ,General Medicine ,biology.organism_classification ,Protein Structure, Tertiary ,Catalytic cycle ,chemistry ,Biochemistry ,Sequence Alignment - Abstract
Microcystins, which are the most common cause of hepatotoxicity associated with cyanobacterial water blooms, are assembledin vivoon a large multienzyme complexviaa mixed nonribosomal peptide synthetase/polyketide synthetase (NRPS/PKS). The biosynthesis of microcystin inMicrocystis aeruginosaPCC 7806 starts with the enzyme McyG, which contains an adenylation–peptidyl carrier protein (A–PCP) didomain for loading the starter unit to assemble the side chain of an Adda residue. However, the catalytic mechanism remains unclear. Here, the 2.45 Å resolution crystal structure of the McyG A–PCP didomain complexed with the catalytic intermediate L-phenylalanyl-adenylate (L-Phe-AMP) is reported. Each asymmetric unit contains two protein molecules, one of which consists of the A–PCP didomain and the other of which comprises only the A domain. Structural analyses suggest that Val227 is likely to be critical for the selection of hydrophobic substrates. Moreover, two distinct interfaces demonstrating variable crosstalk between the PCP domain and the A domain were observed. A catalytic cycle for the adenylation and peptide transfer of the A–PCP didomain is proposed.
- Published
- 2014
90. Structure of pneumococcal peptidoglycan hydrolase LytB reveals insights into the bacterial cell wall remodeling and pathogenesis
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Wang Cheng, Zhensong Wen, Hui-Jie Chen, Lei Qi, Xiao-Hui Bai, Yuxing Chen, Jing-Ren Zhang, Cong-Zhao Zhou, Yubin Huang, Yong-Liang Jiang, and Qiong Li
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Protein Conformation ,Biology ,Biochemistry ,Polymerase Chain Reaction ,Microbiology ,Bacterial cell structure ,Bacterial Adhesion ,Cell wall ,chemistry.chemical_compound ,Protein structure ,Cell Wall ,Hydrolase ,N-acetylmuramoyl-L-alanine amidase ,Molecular Biology ,Choline binding ,Lung ,DNA Primers ,Base Sequence ,Cell Biology ,N-Acetylmuramoyl-L-alanine Amidase ,Enzyme structure ,digestive system diseases ,Streptococcus pneumoniae ,chemistry ,Mutagenesis, Site-Directed ,Peptidoglycan - Abstract
Streptococcus pneumoniae causes a series of devastating infections in humans. Previous studies have shown that the endo-β-N-acetylglucosaminidase LytB is critical for pneumococcal cell division and nasal colonization, but the biochemical mechanism of LytB action remains unknown. Here we report the 1.65 A crystal structure of the catalytic domain (residues Lys-375-Asp-658) of LytB (termed LytBCAT), excluding the choline binding domain. LytBCAT consists of three structurally independent modules: SH3b, WW, and GH73. These modules form a "T-shaped" pocket that accommodates a putative tetrasaccharide-pentapeptide substrate of peptidoglycan. Structural comparison and simulation revealed that the GH73 module of LytB harbors the active site, including the catalytic residue Glu-564. In vitro assays of hydrolytic activity indicated that LytB prefers the peptidoglycan from the lytB-deficient pneumococci, suggesting the existence of a specific substrate of LytB in the immature peptidoglycan. Combined with in vitro cell-dispersing and in vivo cell separation assays, we demonstrated that all three modules are necessary for the optimal activity of LytB. Further functional analysis showed that the full catalytic activity of LytB is required for pneumococcal adhesion to and invasion into human lung epithelial cells. Structure-based alignment indicated that the unique modular organization of LytB is highly conserved in its orthologs from Streptococcus mitis group and Gemella species. These findings provided structural insights into the pneumococcal cell wall remodeling and novel hints for the rational design of therapeutic agents against pneumococcal growth and thereby the related diseases.
- Published
- 2014
91. Crystal structure of juvenile hormone epoxide hydrolase from the silkworm Bombyx mori
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Kang, Zhou, Ning, Jia, Chen, Hu, Yong-Liang, Jiang, Jie-Pin, Yang, Yuxing, Chen, Sheng, Li, Wei-Fang, Li, and Cong-Zhao, Zhou
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Epoxide Hydrolases ,Models, Molecular ,Binding Sites ,Protein Conformation ,Molecular Sequence Data ,Animals ,Amino Acid Sequence ,Bombyx ,Crystallography, X-Ray - Published
- 2014
92. Structural and biochemical analyses of the Streptococcus pneumonia L,D-carboxypeptidase DacB
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Juan Zhang, Yong-Liang Jiang, Cong-Zhao Zhou, Yi-Hu Yang, and Yuxing Chen
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Subfamily ,Metallopeptidase ,Carboxypeptidases ,Peptidoglycan ,Crystallography, X-Ray ,Pneumococcal Infections ,Microbiology ,Substrate Specificity ,chemistry.chemical_compound ,Structural Biology ,Humans ,Enzyme kinetics ,Amino Acid Sequence ,Peptide sequence ,chemistry.chemical_classification ,biology ,Tetrapeptide ,General Medicine ,Carboxypeptidase ,Molecular Docking Simulation ,Enzyme ,Streptococcus pneumoniae ,chemistry ,Biochemistry ,biology.protein - Abstract
The L,D-carboxypeptidase DacB plays a key role in the remodelling ofStreptococcus pneumoniaepeptidoglycan during cell division. In order to decipher its substrate-binding properties and catalytic mechanism, the 1.71 Å resolution crystal structure of DacB fromS. pneumoniaeTIGR4 is reported. Structural analyses in combination with comparisons with the recently reported structures of DacB fromS. pneumoniaeD39 and R6 clearly demonstrate that DacB adopts a zinc-dependent carboxypeptidase fold and belongs to the metallopeptidase M15B subfamily. In addition, enzymatic activity assays further confirm that DacB indeed acts as an L,D-carboxypeptidase towards the tetrapeptide L-Ala-D-iGln-L-Lys-D-Ala of the peptidoglycan stem, withKmandkcatvalues of 2.84 ± 0.37 mMand 91.49 ± 0.05 s−1, respectively. Subsequent molecular docking and site-directed mutagenesis enable the assignment of the key residues that bind to the tetrapeptide. Altogether, these findings provide structural insights into substrate recognition in the metallopeptidase M15B subfamily.
- Published
- 2014
93. Crystal structures and catalytic mechanism of the C-methyltransferase Coq5 provide insights into a key step of the yeast coenzyme Q synthesis pathway
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Fei Meng, Yuxing Chen, Chang-Biao Chi, Yong-Liang Jiang, Kang Zhou, Ya-Nan Dai, Yan-Min Ren, Cong-Zhao Zhou, and Dong-Dong Cao
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Methionine ,Methyltransferase ,Saccharomyces cerevisiae Proteins ,biology ,Stereochemistry ,Ubiquinone ,Saccharomyces cerevisiae ,Substrate (chemistry) ,General Medicine ,Methyltransferases ,biology.organism_classification ,Crystallography, X-Ray ,Yeast ,Catalysis ,Substrate Specificity ,chemistry.chemical_compound ,Biosynthesis ,chemistry ,Structural Biology ,Coenzyme Q – cytochrome c reductase ,Transferase - Abstract
Saccharomyces cerevisiaeCoq5 is anS-adenosyl methionine (SAM)-dependent methyltransferase (SAM-MTase) that catalyzes the onlyC-methylation step in the coenzyme Q (CoQ) biosynthesis pathway, in which 2-methoxy-6-polyprenyl-1,4-benzoquinone (DDMQH2) is converted to 2-methoxy-5-methyl-6-polyprenyl-1,4-benzoquinone (DMQH2). Crystal structures of Coq5 were determined in the apo form (Coq5-apo) at 2.2 Å resolution and in the SAM-bound form (Coq5-SAM) at 2.4 Å resolution, representing the first pair of structures for the yeast CoQ biosynthetic enzymes. Coq5 displays a typical class I SAM-MTase structure with two minor variations beyond the core domain, both of which are considered to participate in dimerization and/or substrate recognition. Slight conformational changes at the active-site pocket were observed upon binding of SAM. Structure-based computational simulation using an analogue of DDMQH2enabled us to identify the binding pocket and entrance tunnel of the substrate. Multiple-sequence alignment showed that the residues contributing to the dimeric interface and the SAM- and DDMQH2-binding sites are highly conserved in Coq5 and homologues from diverse species. A putative catalytic mechanism of Coq5 was proposed in which Arg201 acts as a general base to initiate catalysis with the help of a water molecule.
- Published
- 2014
94. Structural insights into the neutralization mechanism of monoclonal antibody 6C2 against ricin
- Author
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Huajing Wang, Maikun Teng, Xu Li, Xiaojie Yu, Liwen Niu, Jianxin Dai, Yong-Liang Jiang, Yajun Guo, Pengfei Fang, Tiancheng Zhang, Tian Xia, and Yuwei Zhu
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endocrine system ,Complementarity determining region ,Ricin ,Biology ,Biochemistry ,Ribosome ,Neutralization ,Epitope ,Protein Structure, Secondary ,chemistry.chemical_compound ,Antibodies, Monoclonal, Murine-Derived ,Mice ,Ribosomal protein ,Animals ,Protein Structure, Quaternary ,Molecular Biology ,Cell Biology ,Molecular biology ,Antibodies, Neutralizing ,Complementarity Determining Regions ,carbohydrates (lipids) ,enzymes and coenzymes (carbohydrates) ,Structural biology ,chemistry ,Protein Structure and Folding ,Depurination ,Additions and Corrections ,Binding Sites, Antibody - Abstract
Ricin belongs to the type II ribosome-inactivating proteins that depurinate the universally conserved α-sarcin loop of rRNA. The RNA N-glycosidase activity of ricin also largely depends on the ribosomal proteins that play an important role during the process of rRNA depurination. Therefore, the study of the interaction between ricin and the ribosomal elements will be better to understand the catalysis mechanism of ricin. The antibody 6C2 is a mouse monoclonal antibody exhibiting unusually potent neutralizing ability against ricin, but the neutralization mechanism remains unknown. Here, we report the 2.8 Å crystal structure of 6C2 Fab in complex with the A-chain of ricin (RTA), which reveals an extensive antigen-antibody interface that contains both hydrogen bonds and van der Waals contacts. The complementarity-determining region loops H1, H2, H3, and L3 form a pocket to accommodate the epitope on the RTA (residues Asp(96)-Thr(116)). ELISA results show that Gln(98), Glu(99), Glu(102), and Thr(105) (RTA) are the key residues that play an important role in recognizing 6C2. With the perturbation of the 6C2 Fab-RTA interface, 6C2 loses its neutralization ability, measured based on the inhibition of protein synthesis in a cell-free system. Finally, we propose that the neutralization mechanism of 6C2 against ricin is that the binding of 6C2 hinders the interaction between RTA and the ribosome and the surface plasmon resonance and pulldown results confirm our hypothesis. In short, our data explain the neutralization mechanism of mAb 6C2 against ricin and provide a structural basis for the development of improved antibody drugs with better specificity and higher affinity.
- Published
- 2013
95. Structure and catalytic mechanism of yeast 4-amino-4-deoxychorismate lyase
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Ke Ruan, Chang-Biao Chi, Yuxing Chen, Ya-Nan Dai, Wang Cheng, Yan-Min Ren, Cong-Zhao Zhou, Yong-Liang Jiang, and Kang Zhou
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Saccharomyces cerevisiae Proteins ,Saccharomyces cerevisiae ,Molecular Dynamics Simulation ,Crystallography, X-Ray ,Biochemistry ,Cofactor ,chemistry.chemical_compound ,Residue (chemistry) ,Structure-Activity Relationship ,Escherichia coli ,Pyridoxal phosphate ,Molecular Biology ,Schiff base ,biology ,Escherichia coli Proteins ,Active site ,Oxo-Acid-Lyases ,Cell Biology ,Lyase ,biology.organism_classification ,Yeast ,Protein Structure, Tertiary ,body regions ,chemistry ,Protein Structure and Folding ,biology.protein - Abstract
Saccharomyces cerevisiae Abz2 is a pyridoxal 5′-phosphate (PLP)-dependent lyase that converts 4-amino-4-deoxychorismate (ADC) to para-aminobenzoate and pyruvate. To investigate the catalytic mechanism, we determined the 1.9 A resolution crystal structure of Abz2 complexed with PLP, representing the first eukaryotic ADC lyase structure. Unlike Escherichia coli ADC lyase, whose dimerization is critical to the formation of the active site, the overall structure of Abz2 displays as a monomer of two domains. At the interdomain cleft, a molecule of cofactor PLP forms a Schiff base with residue Lys-251. Computational simulations defined a basic clamp to orientate the substrate ADC in a proper pose, which was validated by site-directed mutageneses combined with enzymatic activity assays. Altogether, we propose a putative catalytic mechanism of a unique class of monomeric ADC lyases led by yeast Abz2.
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- 2013
96. Structures of yeast Apa2 reveal catalytic insights into a canonical AP₄A phosphorylase of the histidine triad superfamily
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Wen-Tao, Hou, Wen-Zhe, Li, Yuxing, Chen, Yong-Liang, Jiang, and Cong-Zhao, Zhou
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Models, Molecular ,Protein Conformation ,DNA Mutational Analysis ,Molecular Sequence Data ,Saccharomyces cerevisiae ,Crystallography, X-Ray ,Nucleotidyltransferases ,Adenosine Monophosphate ,Adenosine Triphosphate ,Catalytic Domain ,Mutagenesis, Site-Directed ,Mutant Proteins ,Amino Acid Sequence ,Sequence Alignment ,Dinucleoside Phosphates ,Protein Binding - Abstract
The homeostasis of intracellular diadenosine 5',5″'-P(1),P(4)-tetraphosphate (Ap4A) in the yeast Saccharomyces cerevisiae is maintained by two 60% sequence-identical paralogs of Ap4A phosphorylases (Apa1 and Apa2). Enzymatic assays show that, compared to Apa1, Apa2 has a relatively higher phosphorylase activity towards Ap3A (5',5″'-P(1),P(3)-tetraphosphate), Ap4A, and Ap5A (5',5″'-P(1),P(5)-tetraphosphate), and Ap4A is the favorable substrate for both enzymes. To decipher the catalytic insights, we determined the crystal structures of Apa2 in the apo-, AMP-, and Ap4A-complexed forms at 2.30, 2.80, and 2.70Å resolution, respectively. Apa2 is an α/β protein with a core domain of a twisted eight-stranded antiparallel β-sheet flanked by several α-helices, similar to the galactose-1-phosphate uridylyltransferase (GalT) members of the histidine triad (HIT) superfamily. However, a unique auxiliary domain enables an individual Apa2 monomer to possess an intact substrate-binding cleft, which is distinct from previously reported dimeric GalT proteins. This cleft is perfectly complementary to the favorable substrate Ap4A, the AMP and ATP moieties of which are perpendicular to each other, leaving the α-phosphate group exposed at the sharp turn against the catalytic residue His161. Structural comparisons combined with site-directed mutagenesis and activity assays enable us to define the key residues for catalysis. Furthermore, multiple-sequence alignment reveals that Apa2 and homologs represent canonical Ap4A phosphorylases, which could be grouped as a unique branch in the GalT family.
- Published
- 2013
97. Coordinating carbon and nitrogen metabolic signaling through the cyanobacterial global repressor NdhR.
- Author
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Yong-Liang Jiang, Xue-Ping Wang, Hui Sun, Shu-Jing Han, Wei-Fang Li, Ning Cui, Gui-Ming Lin, Ju-Yuan Zhang, Wang Cheng, Dong-Dong Cao, Zhi-Yong Zhang, Cheng-Cai Zhang, Yuxing Chen, and Cong-Zhao Zhou
- Subjects
- *
CARBON metabolism , *NITROGEN metabolism , *GENE expression , *GENETIC transcription , *CYANOBACTERIA , *OXYGENASE regulation - Abstract
The coordination of carbon and nitrogen metabolism is essential for bacteria to adapt to nutritional variations in the environment, but the underlying mechanism remains poorly understood. In autotrophic cyanobacteria, high CO2 levels favor the carboxylase activity of ribulose 1,5 bisphosphate carboxylase/oxygenase (RuBisCO) to produce 3-phosphoglycerate, whereas low CO2 levels promote the oxygenase activity of RuBisCO, leading to 2-phosphoglycolate (2-PG) production. Thus, the 2-PG level is reversely correlated with that of 2-oxoglutarate (2-OG), which accumulates under a high carbon/nitrogen ratio and acts as a nitrogen-starvation signal. The LysR-type transcriptional repressor NAD(P)H dehydrogenase regulator (NdhR) controls the expression of genes related to carbon metabolism. Based on genetic and biochemical studies, we report here that 2-PG is an inducer of NdhR, while 2-OG is a corepressor, as found previously. Furthermore, structural analyses indicate that binding of 2-OG at the interface between the two regulatory domains (RD) allows the NdhR tetramer to adopt a repressor conformation, whereas 2-PG binding to an intradomain cleft of each RD triggers drastic conformational changes leading to the dissociation of NdhR from its target DNA. We further confirmed the effect of 2-PG or 2-OG levels on the transcription of the NdhR regulon. Together with previous findings, we propose that NdhR can sense 2-OG from the Krebs cycle and 2-PG from photorespiration, two key metabolites that function together as indicators of intracellular carbon/nitrogen status, thus representing a fine sensor for the coordination of carbon and nitrogen metabolism in cyanobacteria. [ABSTRACT FROM AUTHOR]
- Published
- 2018
- Full Text
- View/download PDF
98. Proteomic Analysis Reveals the Deregulation of Inflammation-Related Proteins in Acupuncture-Treated Rats with Asthma Onset
- Author
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Chun-Xiao Shan, Yu Wang, Lei-Miao Yin, Yong-Qing Yang, Xiao-Yan Liu, Ying Wei, Chang-Ke Gao, Jian-mei Cui, Yu-Dong Xu, Yong-Liang Jiang, and Yan-Yan Liu
- Subjects
Article Subject ,Effector ,business.industry ,Inflammation ,lcsh:Other systems of medicine ,medicine.disease ,lcsh:RZ201-999 ,Proinflammatory cytokine ,Complementary and alternative medicine ,Immunology ,Proteome ,medicine ,Acupuncture ,Respiratory function ,Signal transduction ,medicine.symptom ,business ,Asthma ,Research Article - Abstract
Although the beneficial effects of acupuncture in asthma treatment have been well documented, little is known regarding the biological basis of this treatment. Changes in the lung proteome of acupuncture-treated rats with asthma onset were comparatively analyzed using a two-dimensional gel electrophoresis (2DE) and mass-spectrometry- (MS-) based proteomic approach. Acupuncture on specific acupuncture points appeared to improve respiratory function and reduce the total number of leukocytes and eosinophils in bronchoalveolar lavage fluid in OVA-induced asthma onset. Image analysis of 2DE gels revealed 32 differentially expressed acupuncture-specific protein spots in asthma onset; 30 of which were successfully identified as 28 unique proteins using LC-MS/MS. Bioinformatic analyses indicated that these altered proteins are most likely involved in inflammation-related biological functions, and the functional associations of these proteins result in an inflammation signaling pathway. Acupuncture regulates the pathway at different levels by regulating several key nodal proteins, including downregulating of proinflammatory proteins (e.g., S100A8, RAGE, and S100A11) and upregulating of anti-inflammatory proteins (e.g., CC10, ANXA5, and sRAGE). These deregulated inflammation-related proteins may mediate, at least in part, the antiasthmatic effect of acupuncture. Further functional investigation of these acupuncture-specific effector proteins could identify new drug candidates for the prophylaxis and treatment of asthma.
- Published
- 2012
99. Structure of Yeast Sulfhydryl Oxidase Erv1 Reveals Electron Transfer of the Disulfide Relay System in the Mitochondrial Intermembrane Space*
- Author
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Yuxing Chen, Zhang-Zhi Bao, Jin-Di Ma, Xiao-Jie Yu, Shu-Jie Wang, Pengchao Guo, Yong-Liang Jiang, and Cong-Zhao Zhou
- Subjects
Protein Folding ,Saccharomyces cerevisiae Proteins ,Mitochondrial intermembrane space ,Amino Acid Motifs ,Mutation, Missense ,Saccharomyces cerevisiae ,Biology ,Crystallography, X-Ray ,Biochemistry ,Mitochondrial Membrane Transport Proteins ,Electron Transport ,Mitochondrial Proteins ,Electron transfer ,Protein structure ,Oxidoreductase ,Mitochondrial Precursor Protein Import Complex Proteins ,Oxidoreductases Acting on Sulfur Group Donors ,Disulfides ,Molecular Biology ,chemistry.chemical_classification ,Oxidative folding ,Cell Biology ,Mitochondria ,Protein Structure, Tertiary ,Crystallography ,chemistry ,Amino Acid Substitution ,Helix ,Protein Structure and Folding ,Biophysics ,Protein folding ,CTD - Abstract
The disulfide relay system in the mitochondrial intermembrane space drives the import of proteins with twin CX(9)C or twin CX(3)C motifs by an oxidative folding mechanism. This process requires disulfide bond transfer from oxidized Mia40 to a substrate protein. Reduced Mia40 is reoxidized/regenerated by the FAD-linked sulfhydryl oxidase Erv1 (EC 1.8.3.2). Full-length Erv1 consists of a flexible N-terminal shuttle domain (NTD) and a conserved C-terminal core domain (CTD). Here, we present crystal structures at 2.0 Å resolution of the CTD and at 3.0 Å resolution of a C30S/C133S double mutant of full-length Erv1 (Erv1FL). Similar to previous homologous structures, the CTD exists as a homodimer, with each subunit consisting of a conserved four-helix bundle that accommodates the isoalloxazine ring of FAD and an additional single-turn helix. The structure of Erv1FL enabled us to identify, for the first time, the three-dimensional structure of the Erv1NTD, which is an amphipathic helix flanked by two flexible loops. This structure also represents an intermediate state of electron transfer from the NTD to the CTD of another subunit. Comparative structural analysis revealed that the four-helix bundle of the CTD forms a wide platform for the electron donor NTD. Moreover, computational simulation combined with multiple-sequence alignment suggested that the amphipathic helix close to the shuttle redox enter is critical for the recognition of Mia40, the upstream electron donor. These findings provide structural insights into electron transfer from Mia40 via the shuttle domain of one subunit of Erv1 to the CTD of another Erv1 subunit.
- Published
- 2012
100. Structural insights into the substrate specificity of Streptococcus pneumoniae β(1,3)-galactosidase BgaC
- Author
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Qiong Li, Ge Yu, Qiu-Ling Liang, Jun Chu, Yuxing Chen, Xiao-Hui Bai, Cong-Zhao Zhou, Wang Cheng, Yong-Liang Jiang, and Lei Wang
- Subjects
Stereochemistry ,Virulence Factors ,Protein subunit ,Biochemistry ,Acetylglucosamine ,Substrate Specificity ,chemistry.chemical_compound ,Structure-Activity Relationship ,Protein structure ,Bacterial Proteins ,Catalytic Domain ,TIM barrel ,Hydrolase ,Beta-galactosidase ,Molecular Biology ,Crystallography ,biology ,Galactosidases ,Virulence ,Active site ,Galactose ,Cell Biology ,beta-Galactosidase ,Protein Structure, Tertiary ,Streptococcus pneumoniae ,chemistry ,Mutagenesis ,Protein Structure and Folding ,biology.protein ,Dimerization - Abstract
The surface-exposed β-galactosidase BgaC from Streptococcus pneumoniae was reported to be a virulence factor because of its specific hydrolysis activity toward the β(1,3)-linked galactose and N-acetylglucosamine (Galβ(1,3)NAG) moiety of oligosaccharides on the host molecules. Here we report the crystal structure of BgaC at 1.8 A and its complex with galactose at 1.95 A. At pH 5.5-8.0, BgaC exists as a stable homodimer, each subunit of which consists of three distinct domains: a catalytic domain of a classic (β/α)(8) TIM barrel, followed by two all-β domains (ABDs) of unknown function. The side walls of the TIM β-barrel and a loop extended from the first ABD constitute the active site. Superposition of the galactose-complexed structure to the apo-form revealed significant conformational changes of residues Trp-243 and Tyr-455. Simulation of a putative substrate entrance tunnel and modeling of a complex structure with Galβ(1,3)NAG enabled us to assign three key residues to the specific catalysis. Site-directed mutagenesis in combination with activity assays further proved that residues Trp-240 and Tyr-455 contribute to stabilizing the N-acetylglucosamine moiety, whereas Trp-243 is critical for fixing the galactose ring. Moreover, we propose that BgaC and other galactosidases in the GH-35 family share a common domain organization and a conserved substrate-determinant aromatic residue protruding from the second domain.
- Published
- 2012
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