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2,449 results on '"Ling, X."'

351. Requirements for enhanced transgene expression by untranslated sequences from the human cytomegalovirus immediate-early gene

Author

Simari, R. D., Yang, Z. Y., Ling, X., Stephan, D., Perkins, N. D., Nabel, G. J., and Nabel, E. G.

Subjects
Chloramphenicol O-Acetyltransferase, Swine, Gene Transfer Techniques, Cytomegalovirus, Gene Expression, Transfection, Muscle, Smooth, Vascular, Genes, Reporter, Untranslated Regions, Animals, Humans, Promoter Regions, Genetic, Genes, Immediate-Early, Cells, Cultured, Research Article, Plasmids
Abstract

BACKGROUND: The cytomegalovirus immediate early (CMV IE) promoter has been widely used for heterologous expression. Further enhancements of gene expression from this potent promoter may allow for the development of improved gene transfer strategies. We aimed to determine whether inclusion of the first exon (5' untranslated) and first intron of the CMV IE gene would increase heterologous transgene expression in primary target cells and to determine the sequences required for any observed increases. MATERIALS AND METHODS: Comparisons of reporter gene expression were made following transient transfection of vascular smooth muscle cells (VSMCs) with plasmids containing the first exon and intron from the CMV IE gene or deletional mutations. Comparisons were also made using a heterologous promoter (RSV). RESULTS: Gene expression from the CMV IE promoter was increased 5.7-fold in VSMC with the inclusion of the first exon and intron. Similar increases were seen with other target cells and from the heterologous RSV promoter. This increase was associated with an increase in steady-state mRNA. Deletion analyses demonstrated that the enhancement was dependent on the presence of the 5' portion of the first exon while deletion of large segments within the intron was associated with similar levels of expression compared with the parental plasmid. CONCLUSIONS: Inclusion of the first exon and intron from the CMV IE gene increases expression from the CMV IE promoter. This enhancement is seen with the heterologous RSV promoter and is associated with an increase in steady-state mRNA. Deletion analyses suggest that this enhancement is associated with inclusion of sequences within the 5' portion of the first exon and inclusion of an intron.

Published
1998

352. A Mild and Efficient Solid-Support Synthesis of Novel Oligonucleotide Conjugates

Author

Jin Xie, Wen Qiang Zhou, Ivan Habus, Sudhir Agrawal, Ling X Shen, and Radhakrishnan P. Iyer

Subjects
Biomedical Engineering, Pharmaceutical Science, Succinimides, Bioengineering, Antineoplastic Agents, Tretinoin, High-performance liquid chromatography, Mass Spectrometry, Polyethylene Glycols, chemistry.chemical_compound, Folic Acid, Hydroxides, Organic chemistry, Polyacrylamide gel electrophoresis, Chromatography, High Pressure Liquid, Pharmacology, Arachidonic Acid, Base Sequence, Molecular Structure, Oligonucleotide, Organic Chemistry, Oligonucleotide conjugate synthesis, Oligonucleotides, Antisense, Thionucleotides, Combinatorial chemistry, Cyclic AMP-Dependent Protein Kinases, Ammonium hydroxide, chemistry, Spectrophotometry, Ammonium Hydroxide, Arachidonic acid, Electrophoresis, Polyacrylamide Gel, Propionates, Nucleoside, Ethylene glycol, Biotechnology, Conjugate
Abstract

Conjugates of oligodeoxyribonucleotide phosphorothioate (ODN-PS) with folic acid, retinoic acid, arachidonic acid, and methoxypoly(ethylene glycol)propionic acid have been synthesized. The procedure involved the initial solid-phase preparation of 5'-amino-functionalized ODN-PS using N-pent-4-enoyl-derived (PNT) nucleoside phosphoramidites followed by conjugation of the oligonucleotide either to the ligand acids, using 1-[3-(dimethylamino)propyl]-3-ethylcarbodiimide as a coupling reagent, or to their corresponding succinimidyl derivatives. Subsequent exposure of the support to aqueous ammonium hydroxide (28%, 2 h, 55 degrees C) resulted in the release of the fully deprotected ODN conjugates, which were purified by reversed-phase HPLC or by preparative polyacrylamide gel electrophoresis. The identity of the oligonucleotide conjugates was confirmed by MALDI-TOF mass spectral analysis.

Published
1998

353. Equilibrium and Driven Vortex Phases in the Anomalous Peak Effect

Author

Berger, J. E., Smullin, S. J., Karlin, W. L., Ling, X. S., and Prober, D. E.

Subjects
Superconductivity (cond-mat.supr-con), Condensed Matter - Superconductivity, Condensed Matter::Superconductivity, FOS: Physical sciences
Abstract

We report a crucial experimental test of the present models of the peak effect in weakly disordered type-II superconductors. Our results favor the scenario in which the peak effect arises from a crossover between the Larkin pinning length and a rapidly falling elastic length in a vortex phase populated with thermally excited topological defects. A thickness dependence study of the onset of the peak effect at varying driving currents suggests that both screw and edge dislocations are involved in the vortex lattice disordering. The driven dynamics in 3D samples are drastically different from those in 2D samples. We suggest that this may be a consequence of the absence of a Peierls potential for screw dislocations in a vortex line lattice., Comment: 5 pages, 5 figures

Published
1998
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357. IMMUNOLOGY RESEARCH

Author

Barish, M., primary, Weng, L., additional, D'Apuzzo, M., additional, Forman, S., additional, Brown, C., additional, Ben Horin, I., additional, Volovitz, I., additional, Ram, Z., additional, Chang, A., additional, Wainwright, D., additional, Dey, M., additional, Han, Y., additional, Lesniak, M., additional, Chow, K., additional, Yi, J., additional, Shaffer, D., additional, Gottschalk, S., additional, Clark, A., additional, Safaee, M., additional, Oh, T., additional, Ivan, M., additional, Kaur, R., additional, Sun, M., additional, Lu, Y.-J., additional, Ozawa, T., additional, James, C. D., additional, Bloch, O., additional, Parsa, A., additional, Debinski, W., additional, Choi, Y. A., additional, Gibo, D. M., additional, Herold-Mende, C., additional, Mossemann, J., additional, Jungk, C., additional, Ahmadi, R., additional, Capper, D., additional, von Deimling, A., additional, Unterberg, A., additional, Beckhove, P., additional, Jiang, H., additional, Klein, S. R., additional, Piya, S., additional, Vence, L., additional, Yung, W. K. A., additional, Sawaya, R., additional, Heimberger, A., additional, Conrad, C., additional, Lang, F., additional, Gomez-Manzano, C., additional, Fueyo, J., additional, Jung, T.-Y., additional, Choi, Y.-D., additional, Kim, Y.-H., additional, Lee, J.-J., additional, Kim, H.-S., additional, Kim, J.-S., additional, Kim, S.-K., additional, Jung, S., additional, Cho, D., additional, Kosaka, A., additional, Ohkuri, T., additional, Okada, H., additional, Erickson, K., additional, Malone, C., additional, Ha, E., additional, Soto, H., additional, Hickey, M., additional, Owens, G., additional, Liau, L., additional, Prins, R., additional, Minev, B., additional, Kruse, C., additional, Lee, J., additional, Dang, X., additional, Borboa, A., additional, Coimbra, R., additional, Baird, A., additional, Eliceiri, B., additional, Mathios, D., additional, Lim, M., additional, Ruzevick, J., additional, Nicholas, S., additional, Polanczyk, M., additional, Jackson, C., additional, Taube, J., additional, Burger, P., additional, Martin, A., additional, Xu, H., additional, Ochs, K., additional, Sahm, F., additional, Opitz, C. A., additional, Lanz, T. V., additional, Oezen, I., additional, Couraud, P.-O., additional, Wick, W., additional, Platten, M., additional, Ghosh, A., additional, Zhu, J., additional, Ikeura, M., additional, Watkins, S., additional, Sarkar, S., additional, Pellegatta, S., additional, Pessina, S., additional, Cantini, G., additional, Kapetis, D., additional, Finocchiaro, G., additional, Avril, T., additional, Vauleon, E., additional, Hamlat, A., additional, Mosser, J., additional, Quillien, V., additional, Raychaudhuri, B., additional, Rayman, P., additional, Huang, P., additional, Grabowski, M., additional, Hamburdzumyan, D., additional, Finke, J., additional, Vogelbaum, M., additional, Renner, D., additional, Litterman, A., additional, Balgeman, A., additional, Jin, F., additional, Hanson, L., additional, Gamez, J., additional, Carlson, B., additional, Sarkaria, J., additional, Parney, I., additional, Ohlfest, J., additional, Pirko, I., additional, Pavelko, K., additional, Johnson, A., additional, Sims, J., additional, Grinshpun, B., additional, Feng, Y., additional, Amendolara, B., additional, Shen, Y., additional, Canoll, P., additional, Sims, P., additional, Bruce, J., additional, Lee, S. X., additional, Wong, E., additional, Swanson, K., additional, Balyasnikova, I., additional, Cheng, Y., additional, Wang, F., additional, Wei, J., additional, Xu, S., additional, Ling, X., additional, Yaghi, N., additional, Kong, L.-Y., additional, Doucette, T., additional, Weinberg, J., additional, DeMonte, F., additional, Prabhu, S., additional, Wiencke, J., additional, Accomando, W., additional, Houseman, E. A., additional, Nelson, H., additional, Wrensch, M., additional, Wiemels, J., additional, Zheng, S., additional, Hsuang, G., additional, Bracci, P., additional, and Kelsey, K., additional

Published
2013
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367. First use of a neutral cluster and air ion spectrometer in Australia.

Author

Jayaratne, E. R., Pushpawela, B., Ling, X., and Morawska, L.

Subjects
AEROSOLS, AIR pollution
Abstract

Aerosol particles form from molecular clusters at a size of about 1.6 nm. Conventional aerosol measuring instruments such as the scanning mobility particle sizer (SMPS) cannot monitor particles smaller than about 5 nm. The neutral cluster and air ion spectrometer (NAIS) is a recently developed instrument that is designed to measure airborne ions and particles down to a size of 0.8 nm, which is smaller than the size boundary between clusters and particles. It is, therefore, able to observe and measure aerosols at the very sizes that they are formed, permitting more reliable identification and characterisation of new particle formation (NPF) events in the atmosphere than has been possible so far. The Queensland University of Technology purchased a NAIS in 2011. Although, it had been used in several locations around the world, at the time it was the very first NAIS in the Southern Hemisphere and is still the only such instrument in Australia and New Zealand. Since then, the instrument has provided a wealth of data in Australia. For example, for the very first time, it has enabled us to monitor charged particle concentrations near busy roads and overhead powerlines and to reliably identify NPF and determine formation and growth rates of particles in various environments. In this article, we will provide a summary of our findings from the various projects that were conducted over the last five years and discuss the future directions of this research. [ABSTRACT FROM AUTHOR]

Published
2016

368. Lab-on-a-CD.

Author

Kong, Ling X., Perebikovsky, Alexandra, Moebius, Jacob, Kulinsky, Lawrence, and Madou, Marc

Subjects
EXPERIMENTAL design, LABORATORIES, NANOPARTICLES, NUCLEIC acids, RELIABILITY (Personality trait), STATISTICAL sampling, SYSTEM analysis, TECHNOLOGY, QUANTITATIVE research, MILLENNIALS, THREE-dimensional printing, MICROARRAY technology, NUCLEIC acid amplification techniques
Abstract

The field of centrifugal microfluidics has experienced tremendous growth during the past 15 years, especially in applications such as lab-on-a-disc (LoD) diagnostics. The strength of LoD systems lies in its potential for development into fully integrated sample-to-answer analysis systems. This review highlights the technologies necessary to develop the next generation of these systems. In addition to outlining valving and other fluid-handling operations, we discuss the recent advances and future outlook in four categories of LoD processes: reagent storage, sample preparation, nucleic acid amplification, and analyte detection strategies. [ABSTRACT FROM AUTHOR]

Published
2016
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369. HDAC Inhibition Elicits Myocardial Protective Effect through Modulation of MKK3/Akt-1

Author

Jianfeng Du, Paul Y. Liu, Ting C. Zhao, Shougang Zhuang, and Ling X. Zhang

Subjects
Male, Mouse, MAP Kinase Kinase 3, Immunofluorescence, Myocardial Infarction, lcsh:Medicine, Gene Expression, Fluorescent Antibody Technique, Stimulation, 030204 cardiovascular system & hematology, Pharmacology, Cardiovascular, Hydroxamic Acids, Ventricular Function, Left, Immunoenzyme Techniques, Mice, Phosphatidylinositol 3-Kinases, 0302 clinical medicine, Molecular Cell Biology, Myocardial infarction, lcsh:Science, Mice, Knockout, Cardioprotection, 0303 health sciences, Multidisciplinary, Chemistry, Statistics, Histone Modification, Acetylation, Animal Models, Signaling Cascades, Medicine, Phosphorylation, Epigenetics, Research Article, Signal Transduction, medicine.drug, Immunology, Blotting, Western, Ischemia, Biostatistics, Histone Deacetylases, 03 medical and health sciences, Model Organisms, Genetics, Akt Signaling Cascade, medicine, Animals, Immunoprecipitation, Immunoassays, Biology, Protein kinase B, 030304 developmental biology, lcsh:R, medicine.disease, Molecular biology, Histone Deacetylase Inhibitors, Trichostatin A, Immunologic Techniques, lcsh:Q, Proto-Oncogene Proteins c-akt, Reperfusion injury, Mathematics
Abstract

We and others have demonstrated that HDAC inhibition protects the heart against myocardial injury. It is known that Akt-1 and MAP kinase play an essential role in modulation of myocardial protection and cardiac preconditioning. Our recent observations have shown that Akt-1 was activated in post-myocardial infarction following HDAC inhibition. However, it remains unknown whether MKK3 and Akt-1 are involved in HDAC inhibition-induced myocardial protection in acute myocardial ischemia and reperfusion injury. We sought to investigate whether the genetic disruption of Akt-1 and MKK3 eliminate cardioprotection elicited by HDAC inhibition and whether Akt-1 is associated with MKK3 to ultimately achieve protective effects. Adult wild type and MKK3⁻/⁻, Akt-1⁻/⁻ mice received intraperitoneal injections of trichostatin A (0.1 mg/kg), a potent inhibitor of HDACs. The hearts were subjected to 30 min myocardial ischemia/30 min reperfusion in the Langendorff perfused heart after twenty four hours to elicit pharmacologic preconditioning. Left ventricular function was measured, and infarct size was determined. Acetylation and phosphorylation of MKK3 were detected and disruption of Akt-1 abolished both acetylation and phosphorylation of MKK3. HDAC inhibition produces an improvement in left ventricular functional recovery, but these effects were abrogated by disruption of either Akt-1 or MKK3. Disruption of Akt-1 or MKK3 abolished the effects of HDAC inhibition-induced reduction of infarct size. Trichostatin A treatment resulted in an increase in MKK3 phosphorylation or acetylation in myocardium. Taken together, these results indicate that stimulation of the MKK3 and Akt-1 pathway is a novel approach to HDAC inhibition -induced cardioprotection.

Published
2013
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372. Irisin deficiency exacerbates diet-induced insulin resistance and cardiac dysfunction in type II diabetes in mice.

Author

Wang, Jianguo, Zhao, Yu Tina, Zhang, Ling X., Dubielecka, Patrycja M., Qin, Gangjian, Chin, Y. Eugene, Gower, Adam C., Zhuang, Shougang, Liu, Paul Y., and Zhao, Ting C.

Abstract

Irisin is involved in the regulation of a variety of physiological conditions, metabolism, and survival. We and others have demonstrated that irisin contributes critically to modulation of insulin resistance and the improvement of cardiac function. However, whether the deletion of irisin will regulate cardiac function and insulin sensitivity in type II diabetes remains unclear. We utilized the CRISPR/ Cas-9 genome-editing system to delete irisin globally in mice and high-fat diet (HFD)-induced type II diabetes model. We found that irisin deficiency did not result in developmental abnormality during the adult stage, which illustrates normal cardiac function and insulin sensitivity assessed by glucose tolerance test in the absence of stress. The ultrastructural analysis of the transmission electronic microscope (TEM) indicated that deletion of irisin did not change the morphology of mitochondria in myocardium. Gene expression profiling showed that several key signaling pathways related to integrin signaling, extracellular matrix, and insulin-like growth factors signaling were coordinately downregulated by deletion of irisin. However, when mice were fed a high-fat diet and chow food for 16 wk, ablation of irisin in mice exposed to HFD resulted in much more severe insulin resistance, metabolic derangements, profound cardiac dysfunction, and hypertrophic response and remodeling as compared with wild-type control mice. Taken together, our results indicate that the loss of irisin exacerbates insulin resistance, metabolic disorders, and cardiac dysfunction in response to HFD and promotes myocardial remodeling and hypertrophic response. This evidence reveals the molecular evidence and the critical role of irisin in modulating insulin resistance and cardiac function in type II diabetes. NEW & NOTEWORTHY By utilizing the CRISPR/Cas-9 genome-editing system and high-fat diet (HFD)-induced type II diabetes model, our results provide direct evidence showing that the loss of irisin exacerbates cardiac dysfunction and insulin resistance while promoting myocardial remodeling and a hypertrophic response in HFD-induced diabetes. This study provides new insight into understanding the molecular evidence and the critical role of irisin in modulating insulin resistance and cardiac function in type II diabetes. [ABSTRACT FROM AUTHOR]

Published
2023
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378. Synthesis and NMR of RNA with selective isotopic enrichment in the bases

Author

Ling X. Shen, Zhuoping Cai, John SantaLucia, Hal Lewis, and Ignacio Tinoco

Subjects
chemistry.chemical_classification, Magnetic Resonance Spectroscopy, Pyrimidine, Guanosine, Stereochemistry, Adenine, RNA, Cytidine, Purine Nucleosides, Biology, Pyrimidine Nucleosides, Uridine, chemistry.chemical_compound, Heteronuclear molecule, chemistry, Biochemistry, Genetics, Nucleotide, Uracil, Nucleoside
Abstract

Efficient syntheses of pyrimidine and purine nucleosides and nucleotides with selective 13C enrichment in the base moieties are described. Uridine and cytidine are labeled at position C6 and adenosine and guanosine are labeled at position C8. The selectively labeled nucleosides were converted to nucleoside triphosphates and used with in vitro transcription to synthesize labeled RNA. Isotope-edited 12C and 13C sub-spectra of a omega 1-1/2-X-filtered NOESY experiment are demonstrated to be useful for making resonance assignments and for deriving structural information in large (> 20 nt) RNA molecules. The labeled RNAs also allow heteronuclear J-couplings and relaxation parameters to be measured without complications from 13C-13C J-couplings.

Published
1995

379. RNA structure at high resolution

Author

Ling X. Shen, Zhuoping Cai, and Ignacio Tinoco

Subjects
Models, Molecular, Conformational change, Magnetic Resonance Spectroscopy, Base Sequence, Chemistry, Base pair, RNA Conformation, Molecular Sequence Data, Stacking, RNA, Nuclear magnetic resonance spectroscopy, Crystallography, X-Ray, Biochemistry, Genes, env, Genetics, Biophysics, Nucleic Acid Conformation, RNA, Viral, Nucleic acid structure, Structural motif, Molecular Biology, Biotechnology
Abstract

Studies of RNA structural motifs at high resolution by NMR and X-ray crystallographic methods have provided many insights into the fundamental forces that give rise to the unique structural characteristics of RNA. Non-Watson-Crick purine-pyrimidine, purine-purine, and pyrimidine-pyrimidine base pairing, as well as base-phosphate and base-ribose hydrogen bonding, are important forces for folding and stabilizing RNA structures. Base stacking is as important in determining RNA conformations as hydrogen bonding interactions. With the noncanonical interactions, many single-stranded loop regions such as hairpin loops, bulge loops, and internal loops fold into well-defined secondary structures. Loop-loop and loop-helix interactions can produce tertiary structures such as pseudoknots. Also, single strands adjacent to helical regions can form tertiary contacts with base-paired nucleotides of the helices. As we learn more about the structures of the important motifs we can ask more specific questions about the mechanisms of RNA-mediated functions. Conformational flexibility rather than a specific shape of the RNA may be important for some biological reactions. However, knowledge of the structures and the ease of conformational change of the molecules involved in any process are essential for understanding and eventually controlling the process.

Published
1995

380. The structure of an RNA pseudoknot that causes efficient frameshifting in mouse mammary tumor virus

Author

Ling X. Shen and Ignacio Tinoco

Subjects
Models, Molecular, Reading Frames, Magnetic Resonance Spectroscopy, viruses, Molecular Sequence Data, Biology, Slippery sequence, Ribosome, Structural Biology, Nucleotide, Computer Simulation, RNA, Messenger, Molecular Biology, chemistry.chemical_classification, Messenger RNA, Base Sequence, Mouse mammary tumor virus, RNA, Translation (biology), biology.organism_classification, Molecular biology, Fusion Proteins, gag-pol, chemistry, Mammary Tumor Virus, Mouse, Protein Biosynthesis, Biophysics, Nucleic Acid Conformation, RNA, Viral, Imines, Protons, Pseudoknot
Abstract

The structure of a 34-nucleotide RNA pseudoknot that causes efficient −1 frameshifting in the messenger RNA of mouse mammary tumor virus has been investigated by NMR. Spectral assignment of the pseudoknot was facilitated by comparative NMR studies on the pseudoknot and on two smaller hairpin RNAs, and by using selective 1 3 C labeling and 1 3 C-edited NMR techniques. The three-dimensional structure of the pseudoknot has been determined. The frameshifter pseudoknot possesses structural features not observed in previously reported model pseudoknots. It has a compact structure with a pronounced bend at the junction of its two G-C-rich stems. A single adenylate residue is intercalated between the two stems so that direct coaxial staking of the stems is not possible. The lack of an opposing nucleotide for the stacked, intervening adenylate creates a hinge in the pseudoknot. Most of the loop nucleotides are restrained by base staking interactions which keep the loops from adopting extended conformations. The sterically constrained loops direct the bending of the pseudoknot at the stem-stem junction. The roles of the intercalacted adenylate and loop lengths in causing bending can explain their requirement for efficient frameshifting. Our NMR data also indicate that there are internal dynamics associated with the pseudoknot. The unique, compact structure and conformational flexibility of the pseudoknot may be required for recognition and favourable interaction with the translating ribosome, or with translation factors associated with the ribosome.

Published
1995

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