Your search keyword '"Xiu-Ling Xu"' showing total 6 results

1. A convenient cell fusion assay for the study of SARS‐CoV entry and inhibition

Author

Ying Zhu, Da He Jiang, Wen Lan Wu, Xin Mao, Rui Gong, Zhi Jian Cao, Wenxin Li, Ying Liang Wu, Hui Liu, Xiu Ling Xu, and Yong Gang Sha

Subjects

fusion inhibition, Time Factors, viruses, Clinical Biochemistry, Green Fluorescent Proteins, ACE2, Biology, Peptidyl-Dipeptidase A, Severe Acute Respiratory Syndrome, Biochemistry, Article, Flow cytometry, S protein, Cell Fusion, Viral Envelope Proteins, Viral entry, Chlorocebus aethiops, Genetics, medicine, Escherichia coli, Animals, Trypsin, cell‐to‐cell fusion assay, Molecular Biology, Fluorescent Dyes, Glutathione Transferase, Syncytium, COS cells, Cell fusion, Membrane Glycoproteins, medicine.diagnostic_test, Ligand binding assay, SARS‐CoV, Cell Biology, Articles, Molecular biology, Coculture Techniques, Recombinant Proteins, Cell biology, Luminescent Proteins, Severe acute respiratory syndrome-related coronavirus, Cell culture, COS Cells, Spike Glycoprotein, Coronavirus, Biological Assay, Angiotensin-Converting Enzyme 2, Peptides, Fusion mechanism

Abstract

SARS‐CoV spike (S) protein‐mediated cell fusion is important for the viral entry mechanism and identification of SARS‐CoV entry inhibitors. In order to avoid the high risks involved in handling SARS‐CoV and to facilitate the study of viral fusion mechanism, we established the cell lines: SR‐COS7 cells that stably express both SARS‐CoV S protein and red fluorescence protein, R‐COS7 cells that stably express red fluorescence protein, and AG‐COS7 cells that stably express both ACE2 and green fluorescence protein, respectively. When SR‐COS7 cells or R‐COS7 cells were cocultured with AG‐COS7 cells, syncytia with yellow fluorescence were conveniently observed after 12 h in SR‐COS7 cells plus AG‐COS7 cells, but not in R‐COS7 cells plus AG‐COS7 cells. The cell‐to‐cell fusion efficiency was simply determined for quantitative analysis based on the number of syncytium detected by flow cytometry. Such new cell‐to‐cell fusion model was further assessed by the potent HR2 peptide inhibitor, which led to the obvious decrease of the cell‐to‐cell fusion efficiency. The successful fusion and inhibition of cell‐based binding assay shows that it can be well used for the study of SARS‐CoV entry and inhibition. iubmb Life, 58: 480 ‐ 486, 2006

Published

2008

2. Synthesis and nonlinear optical absorption properties of two new conjugated ferrocene-bridge-pyridinium compounds

Author

Fan Yang, Xiu-Ling Xu, Wen-Wei Qiu, Jin-Wei Zhou, Yong-Hua Gong, Jie Tang, Pierre Audebert, and Zhen-Rong Sun

Subjects

chemistry.chemical_classification, Pyridinium Compounds, Organic Chemistry, Electron donor, Electron, Conjugated system, Electron acceptor, Photochemistry, Biochemistry, chemistry.chemical_compound, Ferrocene, chemistry, Drug Discovery, Pyridinium, Absorption (electromagnetic radiation)

Abstract

Two electron donor–π-acceptor (D–π-A) chromospheres, with ferrocene as the electron donor and pyridinium as the electron acceptor, were synthesized. The nonlinear optical absorption (NOA) properties in the solution state were investigated by the Z-scan technique. Both compounds exhibited reverse saturable absorption (RSA) and optical limiting effect under nanosecond pulse irradiation.

Published

2007

3. A Red/Green Cyanobacteriochrome Sustains Its Color Despite a Change in the Bilin Chromophore's Protonation State

Author

Francisco Velazquez Escobar, Xiu-ling Xu, Jörg Matysik, Rei Narikawa, Friedrich Siebert, Wolfgang Gärtner, Chen Song, Peter Hildebrandt, and Masahiko Ikeuchi

Subjects

Models, Molecular, Protein Folding, Spectrophotometry, Infrared, Protein Conformation, Color, Protonation, Photochemistry, Biochemistry, chemistry.chemical_compound, Deprotonation, Protein structure, Bacterial Proteins, Phycocyanobilin, Phycobilins, Bile Pigments, Bilin, Nuclear Magnetic Resonance, Biomolecular, Phytochrome, Chemistry, Phycocyanin, Chromophore, Anabaena, Spectrophotometry, Ultraviolet, Cyanobacteriochrome, Protons, Protein Binding

Abstract

The second GAF domain of AnPixJ, AnPixJg2, a bilin-binding protein from the cyanobacterium Anabaena PCC 7120, undergoes a photoinduced interconversion between a red-absorbing state, Pr, and a green-absorbing state, Pg. Combining ultraviolet-vis (UV-vis), infrared, resonance Raman (RR), and magic-angle spinning (MAS) nuclear magnetic resonance (NMR) spectroscopy, we have studied this cyanobacteriochrome (CBCR) assembled with phycocyanobilin (PCB) either in vivo or in vitro. In both assembly routes, the spectroscopic data of the Pr state reveal nearly identical chromophore structures with a protonated (cationic) bilin. However, unlike the native (in vivo assembly) Pg photoproduct, in which the bilin retains protonation, the Pg generated from the in vitro-assembled AnPixJg2 harbors a deprotonated (neutral) bilin chromophore at pH 7.8. IR difference spectroscopy further reveals the transfer of a proton from the bilin to a side-chain carboxylate on an amino acid, probably Asp291. Besides the change in protonation state, the bilin structure is very similar in the in vitro- and in vivo-assembled Pg photoproducts. The chromophore of the in vitro Pg becomes protonated when the pH is increased to 10, presumably because of a partial reversal of protein misfolding. Most remarkably, the electronic transitions remain unchanged and are very similar to those of the native Pg. Thus, bilin protonation is not a key parameter for controlling the energies of the electronic transitions in AnPixJg2. Possible alternative molecular mechanisms for color tuning are discussed.

Published

2015

4. Genomic Sequence Analysis and Organization of BmKαTx11 and BmKαTx15 from Buthus martensii Karsch: Molecular Evolution of α-toxin genes

Author

Xin Mao, Wen Lan Wu, Wenxin Li, Da He Jiang, Hui Liu, Xiu Ling Xu, Yong Gang Sha, Zhi Jian Cao, Feng Luo, and Ji Qun Sheng

Subjects

DNA, Complementary, Sequence analysis, Molecular Sequence Data, Scorpion Venoms, Locus (genetics), Biology, Biochemistry, Evolution, Molecular, Scorpions, Gene Duplication, Sequence Homology, Nucleic Acid, Complementary DNA, Gene duplication, Animals, Gene family, Amino Acid Sequence, Molecular Biology, Gene, Southern blot, Genetics, Genome, Base Sequence, General Medicine, Introns, Blotting, Southern, genomic DNA, Mutation, Gene Deletion

Abstract

Based on the reported cDNA sequences of BmKalphaTxs , the genes encoding toxin BmKalphaTx11 and BmKalphaTx15 were amplified by PCR from the Chinese scorpion Buthus martensii Karsch genomic DNA employing synthetic oligonucleotides. Sequences analysis of nucleotide showed that an intron about 500 bp length interrupts signal peptide coding regions of BmKalphaTx11 and BmKalphaTx15. Using cDNA sequence of BmKalphaTx11 as probe, southern hybridization of BmK genome total DNA was performed. The result indicates that BmKalphaTx11 is multicopy genes or belongs to multiple gene family with high homology genes. The similarity of BmKalpha-toxin gene sequences and southern hybridization revealed the evolution trace of BmKalpha-toxins: BmKalpha-toxin genes evolve from a common progenitor, and the genes diversity is associated with a process of locus duplication and gene divergence.

Published

2005

5. Combined Mutagenesis and Kinetics Characterization of the Bilin-Binding GAF Domain of the Protein Slr1393 from the Cyanobacterium Synechocystis PCC6803

Author

Dan Miao, Lorena Valle, Alexander Gutt, Claudio D. Borsarelli, Sarah Raffelberg, Kun Tang, Wolfgang Gärtner, Kai-Hong Zhao, Jonas Mechelke, and Xiu Ling Xu

Subjects

Models, Molecular, Histidine Kinase, Otras Ciencias Biológicas, Protein Data Bank (RCSB PDB), Molecular Conformation, PHYCOCYANOBILIN, Biochemistry, Absorbance, Ciencias Biológicas, chemistry.chemical_compound, GLOBAL FIT, Phycocyanobilin, Bacterial Proteins, PAS domain, Phycobilins, TIME RESOLVED, Molecular Biology, MUTAGENESIS, Phytochrome, biology, Organic Chemistry, Synechocystis, Phycocyanin, Chromophore, biology.organism_classification, Protein Structure, Tertiary, PHYTOCHROMES, Crystallography, Kinetics, chemistry, Mutagenesis, Site-Directed, Molecular Medicine, Cyanobacteriochrome, CHROMOPHORES, Protein Kinases, CIENCIAS NATURALES Y EXACTAS

Abstract

The gene slr1393 from Synechocystis sp. PCC6803 encodes a protein composed of three GAF domains, a PAS domain, and a histidine kinase domain. GAF3 is the sole domain able to bind phycocyanobilin (PCB) as chromophore and to accomplish photochemistry: switching between a red-absorbing parental and a green-absorbing photoproduct state (lmax=649 and 536 nm, respectively). Conversions in both directions were followed by time-resolved absorption spectroscopy with the separately expressed GAF3 domain of Slr1393. Global fit analysis of the recorded absorbance changes yielded three lifetimes (3.2 ms, 390 ms, and 1.5 ms) for the red-to-green conversion, and 1.2 ms, 340 ms, and 1 ms for the green-to-red conversion. In addition to the wild-type (WT) protein, 24 mutated proteins were studied spectroscopically. The design of these site-directed mutations was based on sequence alignments with related proteins and by employing the crystal structure of AnPixJg2 (PDB ID: 3W2Z), a Slr1393 orthologous from Anabaena sp.PCC7120. The structure of AnPixJg2 was also used as template for model building, thus confirming the strong structural similarity between the proteins, and for identifying amino acids to target for mutagenesis. Only amino acids in close proximity to the chromophore were exchanged, as these were considered likely to have an impact on the spectral and dynamic properties. Three groups of mutants were found: some showed absorption features similar to the WT protein, a second group showed modified absorbance properties, and the third group had lost the ability to bind the chromophore. The most unexpected result was obtained for the exchange at residue 532 (N532Y). In vivo assembly yielded a red-absorbing, WT-like protein. Irradiation, however, not only converted it into the greenabsorbing form, but also produced a 660 nm, further-red-shifted absorbance band. This photoproduct was fully reversible to the parental form upon green light irradiation. Fil: Xu, Xiu Ling. Max-Planck-Institute for Chemical Energy Conversion; Alemania Fil: Gutt, Alexander. Max-Planck-Institute for Chemical Energy Conversion; Alemania Fil: Mechelke, Jonas. Max-Planck-Institute for Chemical Energy Conversion; Alemania Fil: Raffelberg, Sarah. Max-Planck-Institute for Chemical Energy Conversion; Alemania Fil: Tang, Kun. Max-Planck-Institute for Chemical Energy Conversion; Alemania. Huazhong Agricultural University; República de China Fil: Miao, Dan. Huazhong Agricultural University; República de China Fil: Valle, Lorena. Consejo Nacional de Investigaciones Científicas y Técnicas. Centro de Investigaciones y Transferencia de Santiago del Estero. Universidad Nacional de Santiago del Estero. Centro de Investigaciones y Transferencia de Santiago del Estero; Argentina. Universidad Nacional de Santiago del Estero. Facultad de Agronomía y Agroindustrias; Argentina Fil: Borsarelli, Claudio Darío. Consejo Nacional de Investigaciones Científicas y Técnicas. Centro de Investigaciones y Transferencia de Santiago del Estero. Universidad Nacional de Santiago del Estero. Centro de Investigaciones y Transferencia de Santiago del Estero; Argentina. Universidad Nacional de Santiago del Estero. Facultad de Agronomía y Agroindustrias; Argentina Fil: Zhao, Kai Hong. Huazhong Agricultural University; República de China Fil: Gärtner, Wolfgang. Max-Planck-Institute for Chemical Energy Conversion; Alemania

Published

2014

6. Rapid identification of Quox-1 homeodomain DNA-binding sequence using SAAB

Author

Fan Zhu, Zhongchun Liu, Xiu-Ling Xu, and Wenxin Li

Subjects

Genetics, Homeodomain Proteins, Mutation, Binding Sites, Base Sequence, Oligonucleotides, Electrophoretic Mobility Shift Assay, Nerve Tissue Proteins, General Medicine, Biology, medicine.disease_cause, Biochemistry, Binding, Competitive, DNA binding site, DNA-Binding Proteins, medicine, Consensus sequence, Homeobox, Humans, Protein–DNA interaction, Electrophoretic mobility shift assay, Binding site, Hox gene, Protein Binding

Abstract

Quox-1 is the only gene in the hox family whose expression occurs throughout the development of the central nervous system. Using the Quox-1 homeodomain produced in a bacterial expression system, we were able to identify DNA-binding targets of the Quox-1 protein from a library of randomly generated oligonucleotides by the selection and amplification binding (SAAB) technique. The results indicated that the Quox-1 protein recognizes a new consensus sequence, 5'-CAATC-3', which has not been reported for any other Hox family homeoprotein. In addition, electromobility shift assay further confirmed that the Quox-1 homeoprotein preferentially binds to the 5'-CAATC-3' sequence, but not to the binding sites for other Hox class homeoprotein (TAAT) or NKX class homeoprotein (CAAG). Based on mutation analyses of the DNA sequences, we found that the 5'-CAATC-3' core sequences are required for high affinity binding by the Quox-1 protein. Furthermore, mutation analyses of the Quox-1 homeodomain showed that one of the major determinants participating in recognition of a minor groove is the Gln6 and Thr7 in the N-terminal arm of the homeodomain.

Published

2005