Your search keyword '"Gloeckner C"' showing total 62 results

1. The ciliopathy-associated protein homologs RPGRIP1 and RPGRIP1L are linked to cilium integrity through interaction with Nek4 serine/threonine kinase

Author

Coene, Karlien L.M., Mans, Dorus A., Boldt, Karsten, Gloeckner, C. Johannes, van Reeuwijk, Jeroen, Bolat, Emine, Roosing, Susanne, Letteboer, Stef J.F., Peters, Theo A., Cremers, Frans P.M., Ueffing, Marius, and Roepman, Ronald

Published

2011

2. Understanding the role of genetic variability in LRRK2 in Indian population

Author

Kishore A., Ashok Kumar Sreelatha A., Sturm M., von-Zweydorf F., Pihlstrom L., Raimondi F., Russell R., Lichtner P., Banerjee M., Krishnan S., Rajan R., Puthenveedu D. K., Chung S. J., Bauer P., Riess O., Gloeckner C. J., Kruger R., Gasser T., Sharma M., Kishore, A., Ashok Kumar Sreelatha, A., Sturm, M., von-Zweydorf, F., Pihlstrom, L., Raimondi, F., Russell, R., Lichtner, P., Banerjee, M., Krishnan, S., Rajan, R., Puthenveedu, D. K., Chung, S. J., Bauer, P., Riess, O., Gloeckner, C. J., Kruger, R., Gasser, T., and Sharma, M.

Subjects

Parkinson's disease, neurodegeneration, LRRK2, nervous system diseases

Abstract

Background: Genetic variability in LRRK2 has been unequivocally established as a major risk factor for familial and sporadic forms of PD in ethnically diverse populations. Objectives: To resolve the role of LRRK2 in the Indian population. Methods: We performed targeted resequencing of the LRRK2 locus in 288 cases and 298 controls and resolved the haplotypic structure of LRRK2 in a combined cohort of 800 cases and 402 controls in the Indian population. We assessed the frequency of novel missense variants in the white and East Asian population by leveraging exome sequencing and densely genotype data, respectively. We did computational modeling and biochemical approach to infer the potential role of novel variants impacting the LRRK2 protein function. Finally, we assessed the phosphorylation activity of identified novel coding variants in the LRRK2 gene. Results: We identified four novel missense variants with frequency ranging from 0.0008% to 0.002% specific for the Indian population, encompassing armadillo and kinase domains of the LRRK2 protein. A common genetic variability within LRRK2 may contribute to increased risk, but it was nonsignificant after correcting for multiple testing, because of small cohort size. The computational modeling showed destabilizing effect on the LRRK2 function. In comparison to the wild-type, the kinase domain variant showed 4-fold increase in the kinase activity. Conclusions: Our study, for the first time, identified novel missense variants for LRRK2, specific for the Indian population, and showed that a novel missense variant in the kinase domain modifies kinase activity in vitro. © 2018 International Parkinson and Movement Disorder Society.

Published

2019

3. LRRK2 BINDS TO NEURONAL VESICLES THROUGH PROTEIN INTERACTIONS MEDIATED BY ITS C-TERMINAL WD40 DOMAIN

Author

Cirnaru, M., Onofri, Franco, Marte, Antonella, Kastenmüller, A., Pischedda, F., Zweydorf, F. Von, Jagtap, P., Giesert, F., Pan, L., Sala, C., Ueffing, M., Gloeckner, C. J., and Piccoli, G. .

Published

2014

4. Mutational dynamics between primary and relapse neuroblastomas

Author

Schramm, A. (Alexander), Köster, J. (Johannes), Assenov, Y. (Yassen), Althoff, K. (Kristina), Peifer, M. (Martin), Mahlow, E. (Ellen), Odersky, A. (Andrea), Beisser, D. (Daniela), Ernst, C. (Corinna), Henssen, A.G. (Anton), Stephan, H. (Harald), Schröder, C. (Christopher), Heukamp, L. (Lukas), Engesser, A. (Anne), Kahlert, Y. (Yvonne), Theissen, J. (Jessica), Hero, B. (Barbara), Roels, F. (Frederik), Altmüller, J. (Janine), Nürnberg, P. (Peter), Astrahantseff, K. (Kathy), Gloeckner, C. (Christian), De Preter, K. (Katleen), Plass, C. (Christoph), Lee, S. (Sangkyun), Lode, H.N. (Holger), Henrich, K.-O. (Kai-Oliver), Gartlgruber, M. (Moritz), Speleman, F. (Frank), Schmezer, P. (Peter), Westermann, F. (Frank), Rahmann, S. (Sven), Fischer, M. (Matthias), Eggert, A. (Angelika), Schulte, J.H. (Johannes), Schramm, A. (Alexander), Köster, J. (Johannes), Assenov, Y. (Yassen), Althoff, K. (Kristina), Peifer, M. (Martin), Mahlow, E. (Ellen), Odersky, A. (Andrea), Beisser, D. (Daniela), Ernst, C. (Corinna), Henssen, A.G. (Anton), Stephan, H. (Harald), Schröder, C. (Christopher), Heukamp, L. (Lukas), Engesser, A. (Anne), Kahlert, Y. (Yvonne), Theissen, J. (Jessica), Hero, B. (Barbara), Roels, F. (Frederik), Altmüller, J. (Janine), Nürnberg, P. (Peter), Astrahantseff, K. (Kathy), Gloeckner, C. (Christian), De Preter, K. (Katleen), Plass, C. (Christoph), Lee, S. (Sangkyun), Lode, H.N. (Holger), Henrich, K.-O. (Kai-Oliver), Gartlgruber, M. (Moritz), Speleman, F. (Frank), Schmezer, P. (Peter), Westermann, F. (Frank), Rahmann, S. (Sven), Fischer, M. (Matthias), Eggert, A. (Angelika), and Schulte, J.H. (Johannes)

Abstract

Neuroblastoma is a malignancy of the developing sympathetic nervous system that is often lethal when relapse occurs. We here used whole-exome sequencing, mRNA expression profiling, array CGH and DNA methylation analysis to characterize 16 paired samples at diagnosis and relapse from individuals with neuroblastoma. The mutational burden significantly increased in relapsing tumors, accompanied by altered mutational signatures and reduced subclonal heterogeneity. Global allele frequencies at relapse indicated clonal mutation selection durin

Published

2015

5. RT XFEL structure of Photosystem II 500 ms after the 2nd illumination (2F) at 4.5 A resolution

Author

Kern, J., primary, Tran, R., additional, Alonso-Mori, R., additional, Koroidov, S., additional, Echols, N., additional, Hattne, J., additional, Ibrahim, M., additional, Gul, S., additional, Laksmono, H., additional, Sierra, R.G., additional, Gildea, R.J., additional, Han, G., additional, Hellmich, J., additional, Lassalle-Kaiser, B., additional, Chatterjee, R., additional, Brewster, A., additional, Stan, C.A., additional, Gloeckner, C., additional, Lampe, A., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Seibert, M.M., additional, Koglin, J.E., additional, Gallo, E., additional, Uhlig, J., additional, Sokaras, D., additional, Weng, T.-C., additional, Zwart, P.H., additional, Skinner, D.E., additional, Bogan, M.J., additional, Messerschmidt, M., additional, Glatzel, P., additional, Williams, G.J., additional, Boutet, S., additional, Adams, P.D., additional, Zouni, A., additional, Messinger, J., additional, Sauter, N.K., additional, Bergmann, U., additional, Yano, J., additional, and Yachandra, V.K., additional

Published

2014

6. 1.8 A resolution room temperature structure of Thermolysin recorded using an XFEL

Author

Kern, J., primary, Tran, R., additional, Alonso-Mori, R., additional, Koroidov, S., additional, Echols, N., additional, Hattne, J., additional, Ibrahim, M., additional, Gul, S., additional, Laksmono, H., additional, Sierra, R.G., additional, Gildea, R.J., additional, Han, G., additional, Hellmich, J., additional, Lassalle-Kaiser, B., additional, Chatterjee, R., additional, Brewster, A., additional, Stan, C.A., additional, Gloeckner, C., additional, Lampe, A., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Seibert, M.M., additional, Koglin, J.E., additional, Gallo, E., additional, Uhlig, J., additional, Sokaras, D., additional, Weng, T.-C., additional, Zwart, P.H., additional, Skinner, D.E., additional, Bogan, M.J., additional, Messerschmidt, M., additional, Glatzel, P., additional, Williams, G.J., additional, Boutet, S., additional, Adams, P.D., additional, Zouni, A., additional, Messinger, J., additional, Sauter, N.K., additional, Bergmann, U., additional, Yano, J., additional, and Yachandra, V.K., additional

Published

2014

7. RT XFEL structure of Photosystem II in the dark state at 4.9 A resolution

Author

Kern, J., primary, Tran, R., additional, Alonso-Mori, R., additional, Koroidov, S., additional, Echols, N., additional, Hattne, J., additional, Ibrahim, M., additional, Gul, S., additional, Laksmono, H., additional, Sierra, R.G., additional, Gildea, R.J., additional, Han, G., additional, Hellmich, J., additional, Lassalle-Kaiser, B., additional, Chatterjee, R., additional, Brewster, A., additional, Stan, C.A., additional, Gloeckner, C., additional, Lampe, A., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Seibert, M.M., additional, Koglin, J.E., additional, Gallo, E., additional, Uhlig, J., additional, Sokaras, D., additional, Weng, T.-C., additional, Zwart, P.H., additional, Skinner, D.E., additional, Bogan, M.J., additional, Messerschmidt, M., additional, Glatzel, P., additional, Williams, G.J., additional, Boutet, S., additional, Adams, P.D., additional, Zouni, A., additional, Messinger, J., additional, Sauter, N.K., additional, Bergmann, U., additional, Yano, J., additional, and Yachandra, V.K., additional

Published

2014

8. RT XFEL structure of Photosystem II 250 microsec after the third illumination at 5.2 A resolution

Author

Kern, J., primary, Tran, R., additional, Alonso-Mori, R., additional, Koroidov, S., additional, Echols, N., additional, Hattne, J., additional, Ibrahim, M., additional, Gul, S., additional, Laksmono, H., additional, Sierra, R.G., additional, Gildea, R.J., additional, Han, G., additional, Hellmich, J., additional, Lassalle-Kaiser, B., additional, Chatterjee, R., additional, Brewster, A., additional, Stan, C.A., additional, Gloeckner, C., additional, Lampe, A., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Seibert, M.M., additional, Koglin, J.E., additional, Gallo, E., additional, Uhlig, J., additional, Sokaras, D., additional, Weng, T.-C., additional, Zwart, P.H., additional, Skinner, D.E., additional, Bogan, M.J., additional, Messerschmidt, M., additional, Glatzel, P., additional, Williams, G.J., additional, Boutet, S., additional, Adams, P.D., additional, Zouni, A., additional, Messinger, J., additional, Sauter, N.K., additional, Bergmann, U., additional, Yano, J., additional, and Yachandra, V.K., additional

Published

2014

9. RT XFEL structure of Photosystem II 500 ms after the third illumination at 4.6 A resolution

Author

Kern, J., primary, Tran, R., additional, Alonso-Mori, R., additional, Koroidov, S., additional, Echols, N., additional, Hattne, J., additional, Ibrahim, M., additional, Gul, S., additional, Laksmono, H., additional, Sierra, R.G., additional, Gildea, R.J., additional, Han, G., additional, Hellmich, J., additional, Lassalle-Kaiser, B., additional, Chatterjee, R., additional, Brewster, A., additional, Stan, C.A., additional, Gloeckner, C., additional, Lampe, A., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Seibert, M.M., additional, Koglin, J.E., additional, Gallo, E., additional, Uhlig, J., additional, Sokaras, D., additional, Weng, T.-C., additional, Zwart, P.H., additional, Skinner, D.E., additional, Bogan, M.J., additional, Messerschmidt, M., additional, Glatzel, P., additional, Williams, G.J., additional, Boutet, S., additional, Adams, P.D., additional, Zouni, A., additional, Messinger, J., additional, Sauter, N.K., additional, Bergmann, U., additional, Yano, J., additional, and Yachandra, V.K., additional

Published

2014

10. 1176P - Hybrid-capture based sequencing assays to detect novel alterations in BRAF from tissue and liquid biopsies

Author

Müller, J., Lakis, S., Mariotti, E., Schneider, P., Glöckner, C., Leenders, F., Hube, A., Gullo, G., Crown, J., Griesinger, F., Heuckmann, J., Heukamp, L., and Menon, R.

Published

2016

11. RT fs X-ray diffraction of Photosystem II, first illuminated state

Author

Kern, J., primary, Alonso-Mori, R., additional, Tran, R., additional, Hattne, J., additional, Gildea, R.J., additional, Echols, N., additional, Gloeckner, C., additional, Hellmich, J., additional, Laksmono, H., additional, Sierra, R.G., additional, Lassalle-Kaiser, B., additional, Koroidov, S., additional, Lampe, A., additional, Han, G., additional, Gul, S., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Miahnahri, A., additional, Schafer, D.W., additional, Messerschmidt, M., additional, Seibert, M.M., additional, Koglin, J.E., additional, Sokaras, D., additional, Weng, T.-C., additional, Sellberg, J., additional, Latimer, M.J., additional, Grosse-Kunstleve, R.W., additional, Zwart, P.H., additional, White, W.E., additional, Glatzel, P., additional, Adams, P.D., additional, Bogan, M.J., additional, Williams, G.J., additional, Boutet, S., additional, Messinger, J., additional, Zouni, A., additional, Sauter, N.K., additional, Yachandra, V.K., additional, Bergmann, U., additional, and Yano, J., additional

Published

2013

12. RT fs X-ray diffraction of Photosystem II, dark state

Author

Kern, J., primary, Alonso-Mori, R., additional, Tran, R., additional, Hattne, J., additional, Gildea, R.J., additional, Echols, N., additional, Gloeckner, C., additional, Hellmich, J., additional, Laksmono, H., additional, Sierra, R.G., additional, Lassalle-Kaiser, B., additional, Koroidov, S., additional, Lampe, A., additional, Han, G., additional, Gul, S., additional, DiFiore, D., additional, Milathianaki, D., additional, Fry, A.R., additional, Miahnahri, A., additional, Schafer, D.W., additional, Messerschmidt, M., additional, Seibert, M.M., additional, Koglin, J.E., additional, Sokaras, D., additional, Weng, T.-C., additional, Sellberg, J., additional, Latimer, M.J., additional, Grosse-Kunstleve, R.W., additional, Zwart, P.H., additional, White, W.E., additional, Glatzel, P., additional, Adams, P.D., additional, Bogan, M.J., additional, Williams, G.J., additional, Boutet, S., additional, Messinger, J., additional, Zouni, A., additional, Sauter, N.K., additional, Yachandra, V.K., additional, Bergmann, U., additional, and Yano, J., additional

Published

2013

13. fs X-ray diffraction of Photosystem II

Author

Kern, J., primary, Alonso-Mori, R., additional, Hellmich, J., additional, Tran, R., additional, Hattne, J., additional, Laksmono, H., additional, Gloeckner, C., additional, Echols, N., additional, Sierra, R.G., additional, Sellberg, J., additional, Lassalle-Kaiser, B., additional, Gildea, R.J., additional, Glatzel, P., additional, Grosse-Kunstleve, R.W., additional, Latimer, M.J., additional, Mcqueen, T.A., additional, Difiore, D., additional, Fry, A.R., additional, Messerschmidt, M.M., additional, Miahnahri, A., additional, Schafer, D.W., additional, Seibert, M.M., additional, Sokaras, D., additional, Weng, T.-C., additional, Zwart, P.H., additional, White, W.E., additional, Adams, P.D., additional, Bogan, M.J., additional, Boutet, S., additional, Williams, G.J., additional, Messinger, J., additional, Sauter, N.K., additional, Zouni, A., additional, Bergmann, U., additional, Yano, J., additional, and Yachandra, V.K., additional

Published

2012

14. Chemical Biology of DNA Polymerases: From Selectivity to New Functions

Author

Marx, A., primary, Summerer, D., additional, Sauter, K. B. M., additional, Gloeckner, C., additional, and Rudinger, N. Z., additional

Published

2007

15. The AIDS challenge.

Author

Gloeckner, C.

Subjects

*HIV

Abstract

Explains how the human immunodeficiency virus (HIV) invades the body, attacks the immune system and eventually causes acquired immunodeficiency syndrome (AIDS). How HIV is spread; Recent retirement of basketball star Earvin `Magic' Johnson; Helper T, or T4, cells; The CD4 receptor; The six stages of HIV infection; Vaccine research; Drugs such as zidovudine (AZT) and dideoxyinosine (DDI); AIDS prevention and education; Where to obtain more information.

Published

1992

16. The human eye.

Author

Gloeckner, C.

Subjects

*EYE

Abstract

Describes the parts of the human eye and the function of each part. General characteristics; Function of tears; How eye movement is accomplished; How the brain translates light into images; Vision problems; Suggestions for protecting vision. INSET: Shopping for shades (sunglasses).;Myopia blues (how....

Published

1991

17. What a pain!!! Understanding the causes and treatments of pain.

Author

Gloeckner, C.

Subjects

*PAIN

Abstract

Examines the mechanisms of pain. The pain process; Pain as a warning to the body; Psychology of pain; Painkillers; Pain therapy. INSET: The pain process (diagram).;Pain clinics; A glossary of pain....

Published

1991

18. Antagonist-induced transient down-regulation of delta-opioid receptors in NG108-15 cells.

Author

Belcheva, M M, Barg, J, Gloeckner, C, Gao, X M, Chuang, D M, and Coscia, C J

Abstract

According to current concepts, agonists can effect the down-regulation of cell surface receptors, whereas antagonists can cause their up-regulation. We have discovered that the opioid antagonists naltrexone, naloxone, and ICI174864 induce a transient down-regulation of delta-opioid receptors before up-regulation, in NG108-15 cells. The possibility of an apparent loss of sites due to blockade by residual antagonist was ruled out by several lines of evidence. The reduction in delta receptors was time, temperature, and antagonist concentration dependent. This down-regulation could not be induced by either the highly mu-selective opioid antagonist cyclic D-Phe-Cys-Try-D-Trp-Arg-Thr-Pen-Thr-amide or the muscarinic antagonist atropine. In the same neurohybrid cells, the opioid agonist [D-Ala2,D-Leu5]enkephalin (0.1 microM, 60 min) effected a greater down-regulation of delta-opioid receptors. Similar qualitative changes in opioid binding of subcellular fractions were elicited with [D-Ala2,D-Leu5]enkephalin and naltrexone. However, the agonist was 2-fold more effective in reducing the heavy membrane population of receptors and 4-fold more potent in increasing the light membrane sites. Because heavy membranes are enriched in plasma membrane, whereas light membranes contain intracellular sites, these findings indicate that internalization occurs in both instances. Naltrexone and the delta-specific antagonists ICI174864 and naltrindole also diminished specific activities of two lysosomal enzymes, whereas opioid agonist-induced down-regulation was accompanied by an increase in their specific activities. Pretreatment of cell cultures with concanavalin A blocked both down-regulation and alterations in the lysosomal enzyme activities elicited by agonists and antagonists, suggesting that the latter is an opioid receptor-mediated process. The up-regulation of delta-opioid receptors by antagonists appears, then, to entail down-regulation that differs from that of agonists.

Published

1992

19. From drinking to disease.

Author

Gloeckner, C.

Subjects

*ALCOHOLISM

Abstract

Looks at diseases caused by alcohol abuse. Toxic hepatitis; Cirrhosis of the liver; Gastritis, stroke and hypoglycemia; Malnutrition and fetal alcohol syndrome; Effects on the brain. INSET: Alcoholism.;Oh, my aching head..

Published

1990

20. Helping teens who have problems.

Author

Gloeckner, C.

Subjects

*YOUTH

Abstract

Encourages teens to empathize with each other. Being friendly; Practical help; Being a good listener; Sources of help. INSET: Be a peer counselor..

Published

1991

21. When one date leads (happily) to another.

Author

Gloeckner, C.

Subjects

*DATING (Social customs)

Abstract

Outlines eight aspects of a healthy dating relationship. Attraction and honest communication; Compatibility and trust; Commitment and mutual nurture; Constructive fighting and independence. INSET: Trouble ahead!.

Published

1990

22. Where there's smoke, there's disease.

Author

Gloeckner, C.

Subjects

*PHYSIOLOGICAL effects of tobacco

Abstract

Warns against diseases caused by smoking. Cancer; Chronic obstructive pulmonary disease (COPD); Heart disease; Fetal damage and sick children; Passive smoking; Toward a smoke-free society.

Published

1990

23. Lead, the deadly metal.

Author

Gloeckner, C.

Subjects

*PHYSIOLOGICAL effects of lead

Abstract

Discusses the health hazards posed by contact with lead. Effects of lead poisoning; How lead gets into the human body; Efforts to reduce the incidence of lead poisoning.

Published

1990

24. Life with asthma.

Author

Gloeckner, C.

Subjects

*ASTHMA

Abstract

Discusses asthma, a disease in which the tubes that carry air to the lungs cease to function effectively. Causes; Who has it; Treatment. INSET: How can you help?.

Published

1989

25. Auto-regulation of Rab5 GEF activity in Rabex5 by allosteric structural changes, catalytic core dynamics and ubiquitin binding

Author

Michael Habeck, Christian Johannes Gloeckner, Andrei N. Lupas, Francesco Raimondi, Vikram Alva, Yannis Kalaidzidis, Alice Cezanne, Marius Ueffing, Sandra Segeletz, Marino Zerial, Giambattista Guaitoli, Marc Gentzel, Janelle L. Lauer, Lauer, J., Segeletz, S., Cezanne, A., Guaitoli, G., Raimondi, F., Gentzel, M., Alva, V., Habeck, M., Kalaidzidis, Y., Ueffing, M., Lupas, A. N., Gloeckner, C. J., and Zerial, M.

Subjects

metabolism [Guanine Nucleotide Exchange Factors], Ubiquitin binding, QH301-705.5, Structural Biology and Molecular Biophysics, Science, Allosteric regulation, GTPase, General Biochemistry, Genetics and Molecular Biology, Cell Line, 03 medical and health sciences, 0302 clinical medicine, Rab5, guanine nucleotide exchange factor (GEF), Catalytic Domain, metabolism [Ubiquitin], Animals, Guanine Nucleotide Exchange Factors, Humans, structural biology, Biology (General), hydrogen deuterium exchange mass spectrometry (HDX-MS), 030304 developmental biology, rab5 GTP-Binding Proteins, 0303 health sciences, General Immunology and Microbiology, Chemistry, Ubiquitin, General Neuroscience, General Medicine, Protein Transport, Structural biology, molecular biophysic, metabolism [rab5 GTP-Binding Proteins], Biophysics, Medicine, Hydrogen–deuterium exchange, Rab, Other, Linker, ddc:600, 030217 neurology & neurosurgery, Function (biology), Research Article, Protein Binding

Abstract

Intracellular trafficking depends on the function of Rab GTPases, whose activation is regulated by guanine exchange factors (GEFs). The Rab5 GEF, Rabex5, was previously proposed to be auto-inhibited by its C-terminus. Here, we studied full-length Rabex5 and Rabaptin5 proteins as well as domain deletion Rabex5 mutants using hydrogen deuterium exchange mass spectrometry. We generated a structural model of Rabex5, using chemical cross-linking mass spectrometry and integrative modeling techniques. By correlating structural changes with nucleotide exchange activity for each construct, we uncovered new auto-regulatory roles for the ubiquitin binding domains and the Linker connecting those domains to the catalytic core of Rabex5. We further provide evidence that enhanced dynamics in the catalytic core are linked to catalysis. Our results suggest a more complex auto-regulation mechanism than previously thought and imply that ubiquitin binding serves not only to position Rabex5 but to also control its Rab5 GEF activity through allosteric structural alterations.

Published

2019

26. Structural model of the dimeric Parkinson’s protein LRRK2 reveals a compact architecture involving distant interdomain contacts

Author

Wim Versées, Zhenyu Yue, Giambattista Guaitoli, Alex B. Burgin, Christian Johannes Gloeckner, Egon Deyaert, Felix von Zweydorf, Francesco Raimondi, Fabiana Renzi, Pravin Kumar Ankush Jagtap, Arjan Kortholt, Katja Gotthardt, Adam Schaffner, Karsten Boldt, Xianting Li, Iban Ubarretxena-Belandia, Yacob Gomez-Llorente, Donald D. Lorimer, Nebojsa Janjic, Bernd K Gilsbach, Michael Sattler, Marius Ueffing, Cell Biochemistry, Guaitoli, G., Raimondi, F., Gilsbach, B. K., Gomez-Llorente, Y., Deyaert, E., Renzi, F., Li, X., Schaffner, A., Jagtap, P. K. A., Boldt, K., Von Zweydorf, F., Gotthardt, K., Lorimer, D. D., Yue, Z., Burgin, A., Janjic, N., Sattler, M., Versees, W., Ueffing, M., Ubarretxena-Belandia, I., Kortholt, A., Gloeckner, C. J., Department of Bio-engineering Sciences, and Structural Biology Brussels

Subjects

0301 basic medicine, Models, Molecular, CROSS-LINKING, Parkinson's disease, metabolism [Leucine-Rich Repeat Serine-Threonine Protein Kinase-2], Crystallography, X-Ray, DISEASE, genetics [Parkinson Disease], Catalytic Domain, Ankyrin, Structural modeling, Peptide sequence, Protein secondary structure, Genetics, chemistry.chemical_classification, ELECTRON-MICROSCOPY, Multidisciplinary, SECONDARY STRUCTURE, Kinase, Parkinson Disease, LRRK2, SMALL-ANGLE SCATTERING, PNAS Plus, KINASE-ACTIVITY, ddc:500, STRUCTURE PREDICTION, Protein domain, chemistry [Leucine-Rich Repeat Serine-Threonine Protein Kinase-2], metabolism [Parkinson Disease], Computational biology, Biology, Protein Serine-Threonine Kinases, Leucine-Rich Repeat Serine-Threonine Protein Kinase-2, 03 medical and health sciences, Protein Domains, Leucine, Humans, Amino Acid Sequence, Kinase activity, ROC DOMAIN, CL-MS, Sequence Homology, Amino Acid, structural modeling, Reproducibility of Results, MASS-SPECTROMETRY, nervous system diseases, 030104 developmental biology, HEK293 Cells, Protein kinase domain, chemistry, EM, Mutation, genetics [Leucine-Rich Repeat Serine-Threonine Protein Kinase-2], Protein Multimerization, HIGH-RESOLUTION

Abstract

Leucine-rich repeat kinase 2 (LRRK2) is a large, multidomain protein containing two catalytic domains: a Ras of complex proteins (Roc) G-domain and a kinase domain. Mutations associated with familial and sporadic Parkinson's disease (PD) have been identified in both catalytic domains, as well as in several of its multiple putative regulatory domains. Several of these mutations have been linked to increased kinase activity. Despite the role of LRRK2 in the pathogenesis of PD, little is known about its overall architecture and how PD-linked mutations alter its function and enzymatic activities. Here, we have modeled the 3D structure of dimeric, full-length LRRK2 by combining domain-based homology models with multiple experimental constraints provided by chemical cross-linking combined with mass spectrometry, negative-stain EM, and small-angle X-ray scattering. Our model reveals dimeric LRRK2 has a compact overall architecture with a tight, multidomain organization. Close contacts between the N-terminal ankyrin and C-terminal WD40 domains, and their proximity-together with the LRR domain-to the kinase domain suggest an intramolecular mechanism for LRRK2 kinase activity regulation. Overall, our studies provide, to our knowledge, the first structural framework for understanding the role of the different domains of full-length LRRK2 in the pathogenesis of PD.

Published

2016

27. First model of dimeric LRRK2: the challenge of unrevealing the structure of a multidomain Parkinson's-associated protein

Author

Bernd K Gilsbach, Giambattista Guaitoli, Christian Johannes Gloeckner, Francesco Raimondi, Guaitoli, G., Gilsbach, B. K., Raimondi, F., and Gloeckner, C. J.

Subjects

0301 basic medicine, Models, Molecular, genetics [GTP Phosphohydrolases], Protein family, genetics [Binding Sites], chemistry [Leucine-Rich Repeat Serine-Threonine Protein Kinase-2], metabolism [Leucine-Rich Repeat Serine-Threonine Protein Kinase-2], Drug design, GTPase, Biology, Leucine-Rich Repeat Serine-Threonine Protein Kinase-2, Biochemistry, metabolism [GTP Phosphohydrolases], GTP Phosphohydrolases, Gene product, 03 medical and health sciences, chemistry [GTP Phosphohydrolases], genetics [Parkinson Disease], Humans, LRRK2 protein, human, Kinase activity, Phosphorylation, Gene, Genetics, Binding Sites, Parkinson Disease, LRRK2, nervous system diseases, Protein Structure, Tertiary, 030104 developmental biology, Protein kinase domain, ddc:540, Mutation, genetics [Leucine-Rich Repeat Serine-Threonine Protein Kinase-2], Protein Multimerization, enzymology [Parkinson Disease]

Abstract

Mutations within the leucine-rich repeat kinase 2 (LRRK2) gene represent the most common cause of Mendelian forms of Parkinson's disease, among autosomal dominant cases. Its gene product, LRRK2, is a large multidomain protein that belongs to the Roco protein family exhibiting GTPase and kinase activity, with the latter activity increased by pathogenic mutations. To allow rational drug design against LRRK2 and to understand the cross-regulation of the G- and the kinase domain at a molecular level, it is key to solve the three-dimensional structure of the protein. We review here our recent successful approach to build the first structural model of dimeric LRRK2 by an integrative modeling approach.

Published

2016

28. High In-Hospital Mortality in SARS-CoV-2-Infected Patients with Active Cancer Disease during Omicron Phase of the Pandemic: Insights from the CORONA Germany Study.

Author

Konermann FM, Gessler N, Wohlmuth P, Behr J, Feldhege J, Gloeckner C, Gunawardene MA, Herrlinger KR, Hoelting T, Pape UF, Reinmuth N, Stang A, Sheikhzadeh S, Arnold D, and Wesseler C

Subjects

Adult, Humans, SARS-CoV-2, Hospital Mortality, Pandemics, Cohort Studies, Germany epidemiology, COVID-19, Neoplasms

Abstract

Introduction: SARS-CoV-2 infected patients with cancer have a worse outcome including a significant higher mortality, compared to non-cancer patients. However, limited data are available regarding in-hospital mortality during the Omicron phase of the pandemic. Therefore, the aim of the study was the comparison of mortality in patients with history of cancer and patients with active cancer disease during the different phases of the COVID-19 pandemic, focusing on the current Omicron variant of concern., Methods: We conducted a multicenter, observational, epidemiological cohort study at 45 hospitals in Germany. Until July 20, 2022, all adult hospitalized SARS-CoV-2 positive patients were included. The primary endpoint was in-hospital mortality regarding cancer status (history of cancer and active cancer disease) and SARS-CoV-2 virus type., Results: From March 11, 2020, to July 20, 2022, a total of 27,490 adult SARS-CoV-2 positive patients were included in the study. 2,578 patients (9.4%) had diagnosis of cancer, of whom 1,065 (41.3%) had history of cancer, whereas 1,513 (58.7%) had active cancer disease. Overall 3,749 out of the total of 27,490 patients (13.6%) died during the hospital stay. Patients with active cancer disease had a significantly higher mortality compared to patients without cancer diagnosis, in both phases of the pandemic (wild-type to Delta: OR 1.940 [1.646-2.285]); Omicron: 2.864 [2.354-3.486]). After adjustment to co-variables, SARS-CoV-2 infected patients with active cancer disease had the highest risk for in-hospital mortality compared to the other groups, in both phases of the pandemic., Conclusion: The CORONA Germany study indicates that hospitalized patients with active cancer disease are at high risk of death during a SARS-CoV-2 infection. Mortality of patients with history of cancer improved to nearly the level of non-cancer patients during Omicron phase., (© 2023 S. Karger AG, Basel.)

Published

2023

29. Comparison of machine learning methods with logistic regression analysis in creating predictive models for risk of critical in-hospital events in COVID-19 patients on hospital admission.

Author

Sievering AW, Wohlmuth P, Geßler N, Gunawardene MA, Herrlinger K, Bein B, Arnold D, Bergmann M, Nowak L, Gloeckner C, Koch I, Bachmann M, Herborn CU, and Stang A

Subjects

Humans, Logistic Models, Cohort Studies, Prospective Studies, Machine Learning, Hospitals, COVID-19

Abstract

Background: Machine learning (ML) algorithms have been trained to early predict critical in-hospital events from COVID-19 using patient data at admission, but little is known on how their performance compares with each other and/or with statistical logistic regression (LR). This prospective multicentre cohort study compares the performance of a LR and five ML models on the contribution of influencing predictors and predictor-to-event relationships on prediction model´s performance., Methods: We used 25 baseline variables of 490 COVID-19 patients admitted to 8 hospitals in Germany (March-November 2020) to develop and validate (75/25 random-split) 3 linear (L1 and L2 penalty, elastic net [EN]) and 2 non-linear (support vector machine [SVM] with radial kernel, random forest [RF]) ML approaches for predicting critical events defined by intensive care unit transfer, invasive ventilation and/or death (composite end-point: 181 patients). Models were compared for performance (area-under-the-receiver-operating characteristic-curve [AUC], Brier score) and predictor importance (performance-loss metrics, partial-dependence profiles)., Results: Models performed close with a small benefit for LR (utilizing restricted cubic splines for non-linearity) and RF (AUC means: 0.763-0.731 [RF-L1]); Brier scores: 0.184-0.197 [LR-L1]). Top ranked predictor variables (consistently highest importance: C-reactive protein) were largely identical across models, except creatinine, which exhibited marginal (L1, L2, EN, SVM) or high/non-linear effects (LR, RF) on events., Conclusions: Although the LR and ML models analysed showed no strong differences in performance and the most influencing predictors for COVID-19-related event prediction, our results indicate a predictive benefit from taking account for non-linear predictor-to-event relationships and effects. Future efforts should focus on leveraging data-driven ML technologies from static towards dynamic modelling solutions that continuously learn and adapt to changes in data environments during the evolving pandemic., Trial Registration Number: NCT04659187., (© 2022. The Author(s).)

Published

2022

30. Cell-free tumor DNA, CA125 and HE4 for the objective assessment of tumor burden in patients with advanced high-grade serous ovarian cancer.

Author

Heitz F, Lakis S, Harter P, Heikaus S, Sehouli J, Talwar J, Menon R, Ataseven B, Bertrand M, Schneider S, Mariotti E, Bommert M, Müller JN, Prader S, Leenders F, Hengsbach A, Gloeckner C, Braicu EI, Heukamp LC, du Bois A, and Heuckmann JM

Subjects

Humans, Female, Middle Aged, Aged, Prospective Studies, Tumor Burden, Circulating Tumor DNA blood, Circulating Tumor DNA genetics, Proteins genetics, Tumor Suppressor Protein p53 genetics, Adult, Mutation, Biomarkers, Tumor blood, Biomarkers, Tumor genetics, Membrane Proteins genetics, Membrane Proteins blood, Neoplasm Grading, Cystadenocarcinoma, Serous genetics, Cystadenocarcinoma, Serous pathology, Cystadenocarcinoma, Serous blood, Ascites genetics, Ascites pathology, Ascites blood, Carcinoma, Ovarian Epithelial blood, Carcinoma, Ovarian Epithelial genetics, Carcinoma, Ovarian Epithelial pathology, Cell-Free Nucleic Acids blood, Cell-Free Nucleic Acids genetics, CA-125 Antigen blood, Ovarian Neoplasms genetics, Ovarian Neoplasms blood, Ovarian Neoplasms pathology, WAP Four-Disulfide Core Domain Protein 2 analysis, WAP Four-Disulfide Core Domain Protein 2 metabolism

Abstract

Background: The present prospective study aimed at determining the impact of cell-free tumor DNA (ct-DNA), CA125 and HE4 from blood and ascites for quantification of tumor burden in patients with advanced high-grade serous epithelial ovarian cancer (EOC)., Methods: Genomic DNA was extracted from tumor FFPE and ct-DNA from plasma before surgery and on subsequent post-surgical days. Extracted DNA was subjected to hybrid-capture based next generation sequencing. Blood and ascites were sampled before surgery and on subsequent post-surgical days. 20 patients (10 undergoing complete resection (TR0), 10 undergoing incomplete resection (TR>0)) were included., Results: The minor allele frequency (MAF) of TP53 mutations in ct-DNA of all patients with TR0 decreased significantly, compared to only one patient with TR>0. It was not possible to distinguish between patients with TR0 and patients with TR>0, using CA125 and HE4 from blood and ascites., Conclusions: Based upon the present findings, ct-DNA assessment in patients with high-grade serous EOC might help to better determine disease burden compared to standard tumor markers. Further studies should prospectively evaluate whether this enhancement of accuracy can help to optimize management of patients with EOC., Competing Interests: FH: Travel grants: AstraZeneca, Tesaro, Roche; Honoraria: Roche, AstraZeneca; Clovis, Advisory: Roche; SL: personal fees from NEO New Oncology GmbH, personal fees from BioNTech Diagnostics, personal fees from Definiens GmbH; PH: Honoraria: Roche, AstraZeneca, Tesaro; Advisory: Roche, AstraZeneca, Tesaro, PharmaMar, Lilly; SH: none; JS: HONORARIA: Astra Zeneca, Eisai, Clovis, Olympus, Johnsons and Johnson, PharmaMar, Pfizer, TEVA, TESARO, MSD; CONSULTING OR ADVISORY ROLE: Astra Zeneca, Clovis, Lilly, PharmaMar, Pfizer, Roche, TESARO, MSD; RESEARCH FUNDING: Astra Zeneca, Clovis, Merck, Bayer, PharmaMar, Pfizer, TESARO, MSD; TRAVEL, ACCOMODATIONS, EXPENSES: Astra Zeneca, Clovis, PharmaMar, Roche, Pfizer, TESARO, MSD; JT: employed at New Oncology; RM: employed at New Oncology; BA: reports receiving honoraria from Roche, Tesaro, Clovis, AstraZeneca, and Celgene for lectures, and is an unpaid consultant/advisory board member for Roche and Amgen; MB employed at New Oncology; SS: none; EM: employed at New Oncology; MB: Travel support from prIME Oncology; JNM: employed at New Oncology; SP: none; FL: employed at New Oncology; AH: none; CG: employed at New Oncology; EIB: reports receiving honoraria for advisory board and educational activities from AstraZeneca, Clovis, Tesaro, GSK, Roche Pharma, Incyte, Eisai, MSD, Abbvie; reports receiving travel costs from Clovis, Tesaro, Roche Pharma; LCH: employed at New Oncology; AdB: reports honorary for advisory board and educational activities for Roche, Astra Zeneca, Tesaro, Clovis, Biocad, and Genmab; JMH: employed at New Oncology. That the competing interests does not alter our adherence to PLOS ONE policies on sharing data and materials.

Published

2022

31. Clinical outcome, risk assessment, and seasonal variation in hospitalized COVID-19 patients-Results from the CORONA Germany study.

Author

Gessler N, Gunawardene MA, Wohlmuth P, Arnold D, Behr J, Gloeckner C, Herrlinger K, Hoelting T, Pape UF, Schreiber R, Stang A, Wesseler C, Willems S, Arms C, and Herborn CU

Subjects

Aged, Aged, 80 and over, COVID-19 epidemiology, COVID-19 mortality, Female, Geography, Germany epidemiology, Hospital Mortality, Humans, Male, Middle Aged, Outcome Assessment, Health Care methods, Pandemics, Prospective Studies, Risk Assessment methods, Risk Factors, SARS-CoV-2 physiology, Severity of Illness Index, COVID-19 prevention & control, Hospitalization statistics & numerical data, Outcome Assessment, Health Care statistics & numerical data, Risk Assessment statistics & numerical data, SARS-CoV-2 isolation & purification, Seasons

Abstract

Background: After one year of the pandemic and hints of seasonal patterns, temporal variations of in-hospital mortality in COVID-19 are widely unknown. Additionally, heterogeneous data regarding clinical indicators predicting disease severity has been published. However, there is a need for a risk stratification model integrating the effects on disease severity and mortality to support clinical decision-making., Methods: We conducted a multicenter, observational, prospective, epidemiological cohort study at 45 hospitals in Germany. Until 1 January 2021, all hospitalized SARS CoV-2 positive patients were included. A comprehensive data set was collected in a cohort of seven hospitals. The primary objective was disease severity and prediction of mild, severe, and fatal cases. Ancillary analyses included a temporal analysis of all hospitalized COVID-19 patients for the entire year 2020., Findings: A total of 4704 COVID-19 patients were hospitalized with a mortality rate of 19% (890/4704). Rates of mortality, need for ventilation, pneumonia, and respiratory insufficiency showed temporal variations, whereas age had a strong influence on the course of mortality. In cohort conducting analyses, prognostic factors for fatal/severe disease were: age (odds ratio (OR) 1.704, CI:[1.221-2.377]), respiratory rate (OR 1.688, CI:[1.222-2.333]), lactate dehydrogenase (LDH) (OR 1.312, CI:[1.015-1.695]), C-reactive protein (CRP) (OR 2.132, CI:[1.533-2.965]), and creatinine values (OR 2.573, CI:[1.593-4.154]., Conclusions: Age, respiratory rate, LDH, CRP, and creatinine at baseline are associated with all cause death, and need for ventilation/ICU treatment in a nationwide series of COVID 19 hospitalized patients. Especially age plays an important prognostic role. In-hospital mortality showed temporal variation during the year 2020, influenced by age., Trial Registration Number: NCT04659187., Competing Interests: The authors have declared that no competing interests exist that could be perceived to bias this work. The commercial affiliation does not alter our adherence to PLOS ONE policies on sharing data and materials. SW reports grants and personal fees from Abbott and personal feels from Abbott, Boston Scientific, Boehringer Ingelheim, Bristol Myers Squibb, Bayer Vital, Acutus, and Daiichi Sankyo, outside the submitted work.

Published

2021

32. Concordance between Comprehensive Cancer Genome Profiling in Plasma and Tumor Specimens.

Author

Müller JN, Falk M, Talwar J, Neemann N, Mariotti E, Bertrand M, Zacherle T, Lakis S, Menon R, Gloeckner C, Tiemann M, Heukamp LC, Thomas RK, Griesinger F, and Heuckmann JM

Subjects

Female, Humans, Male, Neoplasms genetics, Proto-Oncogene Mas, Genomics methods, Liquid Biopsy methods, Neoplasms blood, Neoplasms diagnosis

Abstract

Introduction: Detection of somatic genomic alterations in the plasma of patients with cancer ("liquid biopsy") are increasingly being used in the clinic. However, the concordance of alterations identified in liquid biopsies with those detected in cancer specimens is not routinely being determined., Methods: We sought to systematically compare alterations found by a massively parallel sequencing liquid biopsy assay covering 39 genes (NEOliquid [NEO New Oncology GmbH, Köln, Germany]) with those identified through routine diagnostic testing in a certified central pathology laboratory in a cohort of patients with nonsquamous NSCLC. NEOliquid is based on enrichment of the genomic territory of interest by hybrid capture and is thus capable of detecting point mutations, small insertions and deletions, copy number alterations, and gene rearrangements/fusions in a single assay., Results: In a cohort of 82 patients with matched blood/tissue samples, the concordance between NEOliquid and tissue-based routine testing was 98%, the sensitivity of NEOliquid was higher than 70%, and the specificity was 100%. Discordant cases included those with insufficient amounts of circulaating tumor DNA in plasma and cases in which known driver mutations (e.g., isocitrate dehydrogenase (NADP(+)), 1 systolic gene [IDH1] R132H, kinesin family member 5B gene [KIF5b-ret proto-oncogene [RET], or MNNG HOS Transforming gene [MET] exon 14) were found in the plasma but were not interrogated by routine tissue analyses., Conclusions: In summary, NEOliquid offers accurate and reliable detection of clinically relevant driver alterations in plasma of patients with cancer., (Copyright © 2017 International Association for the Study of Lung Cancer. Published by Elsevier Inc. All rights reserved.)

Published

2017

33. Improved genome sequencing using an engineered transposase.

Author

Kia A, Gloeckner C, Osothprarop T, Gormley N, Bomati E, Stephenson M, Goryshin I, and He MM

Subjects

AT Rich Sequence genetics, Reproducibility of Results, Sensitivity and Specificity, Chromosome Mapping methods, DNA genetics, High-Throughput Nucleotide Sequencing methods, Protein Engineering, Sequence Analysis, DNA methods, Transposases genetics

Abstract

Background: Next-generation sequencing (NGS) has transformed genomic research by reducing turnaround time and cost. However, no major breakthrough has been made in the upstream library preparation methods until the transposase-based Nextera method was invented. Nextera combines DNA fragmentation and barcoding in a single tube reaction and therefore enables a very fast workflow to sequencing-ready DNA libraries within a couple of hours. When compared to the traditional ligation-based methods, transposed-based Nextera has a slight insertion bias., Results: Here we present the discovery of a mutant transposase (Tn5-059) with a lowered GC insertion bias through protein engineering. We demonstrate Tn5-059 reduces AT dropout and increases uniformity of genome coverage in both bacterial genomes and human genome. We also observe higher library diversity generated by Tn5-059 when compared to Nextera v2 for human exomes, which leads to less sequencing and lower cost per genome. In addition, when used for human exomes, Tn5-059 delivers consistent library insert size over a range of input DNA, allowing up to a tenfold variance from the 50 ng input recommendation., Conclusions: Enhanced DNA input tolerance of Tn5-059 can translate to flexibility and robustness of workflow. DNA input tolerance together with superior uniformity of coverage and lower AT dropouts extend the applications of transposase based library preps. We discuss possible mechanisms of improvements in Tn5-059, and potential advantages of using the new mutant in varieties of applications including microbiome sequencing and chromatin profiling.

Published

2017

34. Telomerase activation by genomic rearrangements in high-risk neuroblastoma.

Author

Peifer M, Hertwig F, Roels F, Dreidax D, Gartlgruber M, Menon R, Krämer A, Roncaioli JL, Sand F, Heuckmann JM, Ikram F, Schmidt R, Ackermann S, Engesser A, Kahlert Y, Vogel W, Altmüller J, Nürnberg P, Thierry-Mieg J, Thierry-Mieg D, Mariappan A, Heynck S, Mariotti E, Henrich KO, Gloeckner C, Bosco G, Leuschner I, Schweiger MR, Savelyeva L, Watkins SC, Shao C, Bell E, Höfer T, Achter V, Lang U, Theissen J, Volland R, Saadati M, Eggert A, de Wilde B, Berthold F, Peng Z, Zhao C, Shi L, Ortmann M, Büttner R, Perner S, Hero B, Schramm A, Schulte JH, Herrmann C, O'Sullivan RJ, Westermann F, Thomas RK, and Fischer M

Subjects

Cell Line, Tumor, Cell Transformation, Neoplastic genetics, Chromatin genetics, Chromatin metabolism, Chromosomes, Human, Pair 5 genetics, DNA Helicases genetics, DNA Methylation, Enhancer Elements, Genetic genetics, Enzyme Activation genetics, Gene Amplification genetics, Gene Silencing, Humans, Infant, N-Myc Proto-Oncogene Protein, Neuroblastoma classification, Neuroblastoma enzymology, Nuclear Proteins genetics, Oncogene Proteins genetics, Prognosis, RNA, Messenger analysis, RNA, Messenger genetics, Risk, Translocation, Genetic genetics, Up-Regulation genetics, X-linked Nuclear Protein, Gene Expression Regulation, Neoplastic genetics, Genome, Human genetics, Neuroblastoma genetics, Neuroblastoma pathology, Recombination, Genetic genetics, Telomerase genetics, Telomerase metabolism

Abstract

Neuroblastoma is a malignant paediatric tumour of the sympathetic nervous system. Roughly half of these tumours regress spontaneously or are cured by limited therapy. By contrast, high-risk neuroblastomas have an unfavourable clinical course despite intensive multimodal treatment, and their molecular basis has remained largely elusive. Here we have performed whole-genome sequencing of 56 neuroblastomas (high-risk, n = 39; low-risk, n = 17) and discovered recurrent genomic rearrangements affecting a chromosomal region at 5p15.33 proximal of the telomerase reverse transcriptase gene (TERT). These rearrangements occurred only in high-risk neuroblastomas (12/39, 31%) in a mutually exclusive fashion with MYCN amplifications and ATRX mutations, which are known genetic events in this tumour type. In an extended case series (n = 217), TERT rearrangements defined a subgroup of high-risk tumours with particularly poor outcome. Despite a large structural diversity of these rearrangements, they all induced massive transcriptional upregulation of TERT. In the remaining high-risk tumours, TERT expression was also elevated in MYCN-amplified tumours, whereas alternative lengthening of telomeres was present in neuroblastomas without TERT or MYCN alterations, suggesting that telomere lengthening represents a central mechanism defining this subtype. The 5p15.33 rearrangements juxtapose the TERT coding sequence to strong enhancer elements, resulting in massive chromatin remodelling and DNA methylation of the affected region. Supporting a functional role of TERT, neuroblastoma cell lines bearing rearrangements or amplified MYCN exhibited both upregulated TERT expression and enzymatic telomerase activity. In summary, our findings show that remodelling of the genomic context abrogates transcriptional silencing of TERT in high-risk neuroblastoma and places telomerase activation in the centre of transformation in a large fraction of these tumours.

Published

2015

35. Mutational dynamics between primary and relapse neuroblastomas.

Author

Schramm A, Köster J, Assenov Y, Althoff K, Peifer M, Mahlow E, Odersky A, Beisser D, Ernst C, Henssen AG, Stephan H, Schröder C, Heukamp L, Engesser A, Kahlert Y, Theissen J, Hero B, Roels F, Altmüller J, Nürnberg P, Astrahantseff K, Gloeckner C, De Preter K, Plass C, Lee S, Lode HN, Henrich KO, Gartlgruber M, Speleman F, Schmezer P, Westermann F, Rahmann S, Fischer M, Eggert A, and Schulte JH

Subjects

Adaptor Proteins, Signal Transducing genetics, Cell Line, Tumor, Comparative Genomic Hybridization, DNA Copy Number Variations, DNA Helicases genetics, Exome genetics, Gene Expression Profiling methods, Gene Frequency, Guanine Nucleotide Exchange Factors genetics, Hippo Signaling Pathway, Humans, In Situ Hybridization, Fluorescence, Nerve Tissue Proteins genetics, Neuroblastoma pathology, Oligonucleotide Array Sequence Analysis, Phosphoproteins genetics, Protein Serine-Threonine Kinases genetics, Protein Tyrosine Phosphatases, Non-Receptor genetics, Sequence Analysis, DNA methods, Signal Transduction genetics, Transcription Factors, YAP-Signaling Proteins, Gene Expression Regulation, Neoplastic, Mutation, Neoplasm Recurrence, Local genetics, Neuroblastoma genetics

Abstract

Neuroblastoma is a malignancy of the developing sympathetic nervous system that is often lethal when relapse occurs. We here used whole-exome sequencing, mRNA expression profiling, array CGH and DNA methylation analysis to characterize 16 paired samples at diagnosis and relapse from individuals with neuroblastoma. The mutational burden significantly increased in relapsing tumors, accompanied by altered mutational signatures and reduced subclonal heterogeneity. Global allele frequencies at relapse indicated clonal mutation selection during disease progression. Promoter methylation patterns were consistent over disease course and were patient specific. Recurrent alterations at relapse included mutations in the putative CHD5 neuroblastoma tumor suppressor, chromosome 9p losses, DOCK8 mutations, inactivating mutations in PTPN14 and a relapse-specific activity pattern for the PTPN14 target YAP. Recurrent new mutations in HRAS, KRAS and genes mediating cell-cell interaction in 13 of 16 relapse tumors indicate disturbances in signaling pathways mediating mesenchymal transition. Our data shed light on genetic alteration frequency, identity and evolution in neuroblastoma.

Published

2015

36. The role of professional knowledge in case-based reasoning in practical ethics.

Author

Pinkus RL, Gloeckner C, and Fortunato A

Subjects

Humans, Bioengineering ethics, Curriculum, Ethics, Professional education, Ethics, Research education, Knowledge, Learning, Thinking

Abstract

The use of case-based reasoning in teaching professional ethics has come of age. The fields of medicine, engineering, and business all have incorporated ethics case studies into leading textbooks and journal articles, as well as undergraduate and graduate professional ethics courses. The most recent guidelines from the National Institutes of Health recognize case studies and face-to-face discussion as best practices to be included in training programs for the Responsible Conduct of Research. While there is a general consensus that case studies play a central role in the teaching of professional ethics, there is still much to be learned regarding how professionals learn ethics using case-based reasoning. Cases take many forms, and there are a variety of ways to write them and use them in teaching. This paper reports the results of a study designed to investigate one of the issues in teaching case-based ethics: the role of one's professional knowledge in learning methods of moral reasoning. Using a novel assessment instrument, we compared case studies written and analyzed by three groups of students whom we classified as: (1) Experts in a research domain in bioengineering. (2) Novices in a research domain in bioengineering. (3) The non-research group--students using an engineering domain in which they were interested but had no in-depth knowledge. This study demonstrates that a student's level of understanding of a professional knowledge domain plays a significant role in learning moral reasoning skills.

Published

2015

37. DNA sequencing using polymerase substrate-binding kinetics.

Author

Previte MJ, Zhou C, Kellinger M, Pantoja R, Chen CY, Shi J, Wang B, Kia A, Etchin S, Vieceli J, Nikoomanzar A, Bomati E, Gloeckner C, Ronaghi M, and He MM

Subjects

Bacteriophage phi X 174 genetics, Base Pair Mismatch, Base Sequence, DNA chemistry, Equipment Design, Genome, Viral, Genomics, Kinetics, Molecular Sequence Data, Polymers, DNA-Directed DNA Polymerase chemistry, High-Throughput Nucleotide Sequencing instrumentation, High-Throughput Nucleotide Sequencing methods, Nucleotides genetics, Sequence Analysis, DNA

Abstract

Next-generation sequencing (NGS) has transformed genomic research by decreasing the cost of sequencing. However, whole-genome sequencing is still costly and complex for diagnostics purposes. In the clinical space, targeted sequencing has the advantage of allowing researchers to focus on specific genes of interest. Routine clinical use of targeted NGS mandates inexpensive instruments, fast turnaround time and an integrated and robust workflow. Here we demonstrate a version of the Sequencing by Synthesis (SBS) chemistry that potentially can become a preferred targeted sequencing method in the clinical space. This sequencing chemistry uses natural nucleotides and is based on real-time recording of the differential polymerase/DNA-binding kinetics in the presence of correct or mismatch nucleotides. This ensemble SBS chemistry has been implemented on an existing Illumina sequencing platform with integrated cluster amplification. We discuss the advantages of this sequencing chemistry for targeted sequencing as well as its limitations for other applications.

Published

2015

38. Computational modeling of pedunculopontine nucleus deep brain stimulation.

Author

Zitella LM, Mohsenian K, Pahwa M, Gloeckner C, and Johnson MD

Subjects

Animals, Computer Simulation, Humans, Primates, Species Specificity, Action Potentials physiology, Deep Brain Stimulation methods, Evoked Potentials physiology, Models, Neurological, Nerve Net physiology, Neurons physiology

Abstract

Objective: Deep brain stimulation (DBS) near the pedunculopontine nucleus (PPN) has been posited to improve medication-intractable gait and balance problems in patients with Parkinson's disease. However, clinical studies evaluating this DBS target have not demonstrated consistent therapeutic effects, with several studies reporting the emergence of paresthesia and oculomotor side effects. The spatial and pathway-specific extent to which brainstem regions are modulated during PPN-DBS is not well understood., Approach: Here, we describe two computational models that estimate the direct effects of DBS in the PPN region for human and translational non-human primate (NHP) studies. The three-dimensional models were constructed from segmented histological images from each species, multi-compartment neuron models and inhomogeneous finite element models of the voltage distribution in the brainstem during DBS., Main Results: The computational models predicted that: (1) the majority of PPN neurons are activated with -3 V monopolar cathodic stimulation; (2) surgical targeting errors of as little as 1 mm in both species decrement activation selectivity; (3) specifically, monopolar stimulation in caudal, medial, or anterior PPN activates a significant proportion of the superior cerebellar peduncle (up to 60% in the human model and 90% in the NHP model at -3 V); (4) monopolar stimulation in rostral, lateral or anterior PPN activates a large percentage of medial lemniscus fibers (up to 33% in the human model and 40% in the NHP model at -3 V) and (5) the current clinical cylindrical electrode design is suboptimal for isolating the modulatory effects to PPN neurons., Significance: We show that a DBS lead design with radially-segmented electrodes may yield improved functional outcome for PPN-DBS.

Published

2013

39. The use of small molecule probes to study spatially separated stimulus-induced signaling pathways.

Author

Kravchenko VV, Gloeckner C, Stowe GN, Kang YJ, Tobias PS, Mathison JC, Ulevitch RJ, Kaufmann GF, and Janda KD

Subjects

Animals, Cells, Cultured, Immunity, Innate drug effects, Lipopolysaccharides immunology, Macrophages drug effects, Macrophages immunology, Mice, Mice, Inbred C57BL, Small Molecule Libraries chemistry, NF-kappa B immunology, Signal Transduction drug effects, Small Molecule Libraries pharmacology, p38 Mitogen-Activated Protein Kinases immunology

Abstract

Simultaneous activation of signaling pathways requires dynamic assembly of higher-order protein complexes at the cytoplasmic domains of membrane-associated receptors in a stimulus-specific manner. Here, using the paradigm of cellular activation through cytokine and innate immune receptors, we demonstrate the proof-of-principle application of small molecule probes for the dissection of receptor-proximal signaling processes, such as activation of the transcription factor NF-κB and the protein kinase p38., (Copyright © 2012 Elsevier Ltd. All rights reserved.)

Published

2012

40. Targeting the Wolbachia cell division protein FtsZ as a new approach for antifilarial therapy.

Author

Li Z, Garner AL, Gloeckner C, Janda KD, and Carlow CK

Subjects

Animals, Bacterial Proteins genetics, Bacterial Proteins metabolism, Cytoskeletal Proteins genetics, Cytoskeletal Proteins metabolism, DNA, Bacterial chemistry, DNA, Bacterial genetics, Enzyme Inhibitors pharmacology, GTP Phosphohydrolases genetics, GTP Phosphohydrolases metabolism, Molecular Sequence Data, Sequence Analysis, DNA, Anti-Bacterial Agents pharmacology, Bacterial Proteins antagonists & inhibitors, Berberine pharmacology, Brugia malayi microbiology, Cytoskeletal Proteins antagonists & inhibitors, Filaricides pharmacology, GTP Phosphohydrolases antagonists & inhibitors, Wolbachia drug effects

Abstract

The use of antibiotics targeting the obligate bacterial endosymbiont Wolbachia of filarial parasites has been validated as an approach for controlling filarial infection in animals and humans. Availability of genomic sequences for the Wolbachia (wBm) present in the human filarial parasite Brugia malayi has enabled genome-wide searching for new potential drug targets. In the present study, we investigated the cell division machinery of wBm and determined that it possesses the essential cell division gene ftsZ which was expressed in all developmental stages of B. malayi examined. FtsZ is a GTPase thereby making the protein an attractive Wolbachia drug target. We described the molecular characterization and catalytic properties of Wolbachia FtsZ. We also demonstrated that the GTPase activity was inhibited by the natural product, berberine, and small molecule inhibitors identified from a high-throughput screen. Furthermore, berberine was also effective in reducing motility and reproduction in B. malayi parasites in vitro. Our results should facilitate the discovery of selective inhibitors of FtsZ as a novel anti-symbiotic approach for controlling filarial infection. NOTE: The nucleotide sequences reported in this paper are available in GenBank™ Data Bank under the accession number wAlB-FtsZ (JN616286).

Published

2011

41. Learning from directed evolution: Thermus aquaticus DNA polymerase mutants with translesion synthesis activity.

Author

Obeid S, Schnur A, Gloeckner C, Blatter N, Welte W, Diederichs K, and Marx A

Subjects

Directed Molecular Evolution, Models, Molecular, Mutant Proteins chemistry, Mutant Proteins genetics, Mutant Proteins metabolism, Protein Conformation, Taq Polymerase chemistry, Thermus chemistry, DNA Damage, Mutation, Taq Polymerase genetics, Taq Polymerase metabolism, Thermus enzymology, Thermus genetics

Abstract

DNA is being constantly damaged by endo- and exogenous agents such as reactive oxygen species, chemicals, radioactivity, and ultraviolet radiation. Additionally, DNA is inherently labile, and this can result in, for example, the spontaneous hydrolysis of the glycosidic bond that connects the sugar and the nucleobase moieties in DNA; this results in abasic sites. It has long been obscure how cells achieve DNA synthesis past these lesions, and only recently has it been discovered that several specialized DNA polymerases are involved in translesion synthesis. The underlying mechanisms that render one DNA polymerase competent in translesion synthesis while another DNA polymerase fails are still indistinct. Recently two variants of Taq DNA polymerase that exhibited higher lesion bypass ability than the wild-type enzyme were identified by directed-evolution approaches. Strikingly, in both approaches it was independently found that substitution of a single nonpolar amino acid side chain by a cationic side chain increases the capability of translesion synthesis. Here, we combined both mutations in a single enzyme. We found that the KlenTaq DNA polymerase that bore both mutations superseded the wild-type as well as the respective single mutants in translesion-bypass proficiency. Further insights in the molecular basis of the detected gain of translesion-synthesis function were obtained by structural studies of DNA polymerase variants caught in processing canonical and damaged substrates. We found that increased positive charge of the surface potential in the area proximal to the negatively charged substrates promotes translesion synthesis by KlenTaq DNA polymerase, an enzyme that has very limited naturally evolved capability to perform translesion synthesis. Since expanded positively charged surface potential areas are also found in naturally evolved translesion DNA polymerases, our results underscore the impact of charge on the proficiency of naturally evolved translesion DNA polymerases., (Copyright © 2011 WILEY-VCH Verlag GmbH & Co. KGaA, Weinheim.)

Published

2011

42. Design, synthesis, and biological activities of closantel analogues: structural promiscuity and its impact on Onchocerca volvulus.

Author

Garner AL, Gloeckner C, Tricoche N, Zakhari JS, Samje M, Cho-Ngwa F, Lustigman S, and Janda KD

Subjects

Animals, Chitinases chemistry, Drug Design, Enzyme Inhibitors chemical synthesis, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology, Epithelial Cells, Filaricides chemistry, HEK293 Cells, Haplorhini, Humans, Ionophores pharmacology, Larva drug effects, Molecular Structure, Molting drug effects, Onchocerca volvulus enzymology, Onchocerca volvulus growth & development, Onchocerciasis drug therapy, Onchocerciasis parasitology, Onchocerciasis, Ocular drug therapy, Onchocerciasis, Ocular parasitology, Protons, Salicylanilides chemistry, Structure-Activity Relationship, Chitinases antagonists & inhibitors, Filaricides chemical synthesis, Filaricides pharmacology, Onchocerca volvulus drug effects, Salicylanilides chemical synthesis, Salicylanilides pharmacology

Abstract

Onchocerciasis, or river blindness, is a neglected tropical disease that affects more than 37 million people worldwide, primarily in Africa and Central and South America. We have disclosed evidence that the larval-stage-specific chitinase, OvCHT1, may be a potential biological target for affecting nematode development. On the basis of screening efforts, closantel, a known anthelmintic drug, was discovered as a potent and highly specific OvCHT1 inhibitor. Originally, closantel's anthelmintic mode of action was believed to rely solely on its role as a proton ionophore; thus, the impact of each of its biological activities on O. volvulus L3 molting was investigated. Structure-activity relationship studies on an active closantel fragment are detailed, and remarkably, by use of a simple salicylanilide scaffold, compounds acting only as protonophores or chitinase inhibitors were identified. From these data, unexpected synergistic protonophore and chitinase inhibition activities have also been found to be critical for molting in O. volvulus L3 larvae.

Published

2011

43. Directed evolution of DNA polymerases: construction and screening of DNA polymerase mutant libraries.

Author

Gloeckner C, Kranaster R, and Marx A

Abstract

The protocols in this article describe the construction of a mutant DNA polymerase library using error-prone PCR (epPCR) as a method for gene randomization, followed by screening of the library using two different approaches. The examples described use an N-terminally truncated form of the thermostable DNA polymerase I of Thermus aquaticus (Taq DNA polymerase), namely Klentaq (KTQ), and protocols are included for the identification of variants with (1) increased DNA lesion-bypass ability and (2) enhanced selectivity for DNA match/mismatch recognition. The screening assays are based on double-stranded DNA detection (using SYBR Green I) which can be carried out using standard laboratory equipment. The described assays are designed for use in a 384-well plate format to increase screening throughput and reduce material costs. For improved accuracy and ease of liquid handling, the use of an automated liquid handling device is recommended. Curr. Protoc. Chem Biol. 2:89-109. © 2010 by John Wiley & Sons, Inc.

Published

2010

44. Repositioning of an existing drug for the neglected tropical disease Onchocerciasis.

Author

Gloeckner C, Garner AL, Mersha F, Oksov Y, Tricoche N, Eubanks LM, Lustigman S, Kaufmann GF, and Janda KD

Subjects

Animals, Anthelmintics chemistry, Anthelmintics isolation & purification, Chitin metabolism, Enzyme Inhibitors chemistry, Enzyme Inhibitors isolation & purification, Humans, Inhibitory Concentration 50, Molting drug effects, Onchocerca enzymology, Onchocerca growth & development, Salicylanilides chemistry, Salicylanilides isolation & purification, Small Molecule Libraries, Anthelmintics pharmacology, Chitin antagonists & inhibitors, Chitinases antagonists & inhibitors, Drug Discovery, Enzyme Inhibitors pharmacology, Onchocerca drug effects, Onchocerciasis drug therapy, Salicylanilides pharmacology

Abstract

Onchocerciasis, or river blindness, is a neglected tropical disease caused by the filarial nematode Onchocerca volvulus that affects more than 37 million people, mainly in third world countries. Currently, the only approved drug available for mass treatment is ivermectin, however, drug resistance is beginning to emerge, thus, new therapeutic targets and agents are desperately needed to treat and cure this devastating disease. Chitin metabolism plays a central role in invertebrate biology due to the critical structural function of chitin for the organism. Taken together with its absence in mammals, targeting chitin is an appealing therapeutic avenue. Importantly, the chitinase OvCHT1 from O. volvulus was recently discovered, however, its exact role in the worm's metabolism remains unknown. A screening effort against OvCHT1 was conducted using the Johns Hopkins Clinical Compound Library that contains over 1,500 existing drugs. Closantel, a veterinary anthelmintic with known proton ionophore activities, was identified as a potent and specific inhibitor of filarial chitinases, an activity not previously reported for this compound. Notably, closantel was found also to completely inhibit molting of O. volvulus infective L3 stage larvae. Closantel appears to target two important biochemical processes essential to filarial parasites. To begin to unravel closantel's effects, a retro-fragment-based study was used to define structural elements critical for closantel's chitinase inhibitor function. As resources towards the development of new agents that target neglected tropical diseases are scant, the finding of an existing drug with impact against O. volvulus provides promise in the hunt for new therapies against river blindness.

Published

2010

45. Inhibition of tumor metastasis: functional immune modulation of the CUB domain containing protein 1.

Author

Fukuchi K, Steiniger SC, Deryugina E, Liu Y, Lowery CA, Gloeckner C, Zhou B, Kaufmann GF, Quigley JP, and Janda KD

Subjects

Amino Acid Sequence, Animals, Antibodies, Blocking administration & dosage, Antibodies, Blocking genetics, Antibodies, Monoclonal administration & dosage, Antibodies, Monoclonal genetics, Antibody-Dependent Cell Cytotoxicity, Antigens, CD genetics, Antigens, Neoplasm, Cell Adhesion Molecules genetics, Cell Line, Tumor, Chick Embryo, Female, HeLa Cells, Humans, Male, Mice, Mice, Inbred NOD, Mice, SCID, Molecular Sequence Data, Neoplasm Metastasis immunology, Neoplasm Metastasis therapy, Neoplasm Proteins genetics, Peptide Library, Prostatic Neoplasms immunology, Prostatic Neoplasms secondary, Prostatic Neoplasms therapy, Recombinant Fusion Proteins administration & dosage, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins immunology, Sequence Homology, Amino Acid, Transfection, Xenograft Model Antitumor Assays, Antigens, CD immunology, Cell Adhesion Molecules antagonists & inhibitors, Cell Adhesion Molecules immunology, Neoplasm Metastasis prevention & control, Neoplasm Proteins antagonists & inhibitors, Neoplasm Proteins immunology

Abstract

Despite significant progress and notable successes in tumor therapy, malignant disease remains an extremely difficult problem in today's health care setting. There is, however, an increasing application of new therapies targeting proteins specifically upregulated on tumor cells. These innovative therapeutic approaches are aimed at molecules that contribute to malignant development and progression but spare normal tissues. The CUB domain containing protein 1 (CDCP1) is such a tumor-associated protein and, thus, a potential candidate for targeted cancer immunotherapy. Herein, we describe the generation of function-blocking human antibodies against CDCP1 that were obtained from human scFv phage display libraries using subtractive panning protocols on CDCP1 expressing cancer cells and immunopurified CDCP1 protein. One of the isolated anti-CDCP1 antibodies, namely, C20Fc, efficiently blocked experimental metastasis of human carcinoma cells, including HeLa cells stably transfected with CDCP1 and prostate carcinoma cells PC-hi/diss naturally expressing CDCP1, in both chick embryo and mouse model systems. The C20Fc antibody also reduced colony formation of CDCP1 expressing cells in a soft agar assay for anchorage-independent cell growth. Specific targeting of CDCP1 by C20Fc mediated the delivery of a toxin-conjugated antibody complex, thus, providing evidence for antibody internalization and specific killing of CDCP1-positive tumor cells. Our findings indicate a functional role for CDCP1 in human cancer and underscore the therapeutic potential of function-blocking anti-CDCP1 antibodies targeting both primary and metastatic carcinoma cells.

Published

2010

46. Defining the mode of action of tetramic acid antibacterials derived from Pseudomonas aeruginosa quorum sensing signals.

Author

Lowery CA, Park J, Gloeckner C, Meijler MM, Mueller RS, Boshoff HI, Ulrich RL, Barry CE 3rd, Bartlett DH, Kravchenko VV, Kaufmann GF, and Janda KD

Subjects

4-Butyrolactone analogs & derivatives, 4-Butyrolactone pharmacology, Anti-Bacterial Agents biosynthesis, Anti-Bacterial Agents chemistry, Gram-Positive Bacteria drug effects, Humans, Membrane Potentials drug effects, Microbial Sensitivity Tests, Pseudomonas aeruginosa metabolism, Pyrrolidines chemistry, Pyrrolidines pharmacology, Quorum Sensing, Anti-Bacterial Agents pharmacology, Pseudomonas aeruginosa chemistry, Pyrrolidinones pharmacology

Abstract

In nature, bacteria rarely exist as single, isolated entities, but rather as communities comprised of many other species including higher host organisms. To survive in these competitive environments, microorganisms have developed elaborate tactics such as the formation of biofilms and the production of antimicrobial toxins. Recently, it was discovered that the gram-negative bacterium Pseudomonas aeruginosa , an opportunistic human pathogen, produces an antibiotic, 3-(1-hydroxydecylidene)-5-(2-hydroxyethyl)pyrrolidine-2,4-dione (C(12)-TA), derived from one of its quorum sensing molecules. Here, we present a comprehensive study of the expanded spectrum of C(12)-TA antibacterial activity against microbial competitors encountered by P. aeruginosa in nature as well as significant human pathogens. The mechanism of action of C(12)-TA was also elucidated, and C(12)-TA was found to dissipate both the membrane potential and the pH gradient of Gram-positive bacteria, correlating well with cell death. Notably, in stark contrast to its parent molecule 3-oxo-dodecanoyl homoserine lactone (3-oxo-C(12)-HSL), neither activation of cellular stress pathways nor cytotoxicity was observed in human cells treated with C(12)-TA. Our results suggest that the QS machinery of P. aeruginosa has evolved for a dual-function, both to signal others of the same species and also to defend against host immunity and competing bacteria. Because of the broad-spectrum antibacterial activity, established mode of action, lack of rapid resistance development, and tolerance by human cells, the C(12)-TA scaffold may also serve as a new lead compound for the development of antimicrobial therapeutics.

Published

2009

47. Displacement of protein-bound aptamers with small molecules screened by fluorescence polarization.

Author

Hafner M, Vianini E, Albertoni B, Marchetti L, Grüne I, Gloeckner C, and Famulok M

Subjects

Aptamers, Nucleotide metabolism, Aptamers, Nucleotide pharmacology, Drug Evaluation, Preclinical methods, Guanine Nucleotide Exchange Factors antagonists & inhibitors, Guanine Nucleotide Exchange Factors chemistry, Protein Binding, Aptamers, Nucleotide isolation & purification, Fluorescence Polarization methods, Guanine Nucleotide Exchange Factors metabolism

Abstract

Small molecule inhibitors of proteins are invaluable tools in research and as starting points for drug development. However, their screening can be tedious, as most screening methods have to be tailored to the corresponding drug target. Here, we describe a detailed protocol for a modular and generally applicable assay for the identification of small organic compounds that displace an aptamer complexed to its target protein. The method relies on fluorescence-labeled aptamers and the increase of fluorescence polarization upon their binding to the target protein. The assay has high Z'-factors, making it compatible with high-throughput screening. It allows easy automation, making fluorescence readout the time-limiting step. As aptamers can be generated for virtually any protein target, the assay allows identification of small molecule inhibitors for targets or individual protein domains for which no functional screen is available. We provide the step-by-step protocol to screen for antagonists of the cytohesin class of small guanosine exchange factors.

Published

2008

48. Directed DNA polymerase evolution: effects of mutations in motif C on the mismatch-extension selectivity of thermus aquaticus DNA polymerase.

Author

Strerath M, Gloeckner C, Liu D, Schnur A, and Marx A

Subjects

Amino Acid Motifs, Base Sequence, DNA chemistry, Molecular Sequence Data, Polymerase Chain Reaction, Taq Polymerase chemistry, Amino Acids chemistry, DNA genetics, Evolution, Molecular, Mutation genetics, Taq Polymerase genetics, Thermus enzymology

Abstract

The selectivity of DNA polymerases for processing the canonical nucleotide and DNA substrate in favor of the noncanonical ones is the key to the integrity of the genome of every living species and to many biotechnological applications. The inborn ability of most DNA polymerases to abort efficient extension of mismatched DNA substrates adds to the overall DNA polymerase selectivity. DNA polymerases have been grouped into families according to their sequence. Within family A DNA polymerases, six motifs that come into contact with the substrates and form the active site have been discovered to be evolutionary highly conserved. Here we present results obtained from amino acid randomization within one motif, motif C, of thermostable Thermus aquaticus DNA polymerase. We have identified several distinct mutation patterns that increase the selectivity of mismatch extension. These results might lead to direct applications such as allele-specific PCR, as demonstrated by real-time PCR experiments and add to our understanding of DNA polymerase selectivity.

Published

2007

49. New branched DNA constructs.

Author

Chandra M, Keller S, Gloeckner C, Bornemann B, and Marx A

Subjects

Automation, Base Sequence, Circular Dichroism, Electrophoresis, Polyacrylamide Gel, Models, Chemical, Oligonucleotides chemical synthesis, Base Pairing, Biotechnology, DNA chemical synthesis, Nanotechnology, Nucleic Acid Conformation

Abstract

The Watson-Crick base pairing of DNA is an advantageous phenomenon that can be exploited when using DNA as a scaffold for directed self-organization of nanometer-sized objects. Several reports have appeared in the literature that describe the generation of branched DNA (bDNA) with variable numbers of arms that self-assembles into predesigned architectures. These bDNA units are generated by using cleverly designed rigid crossover DNA molecules. Alternatively, bDNA can be generated by using synthetic branch points derived from either nucleoside or non-nucleoside building blocks. Branched DNA has scarcely been explored for use in nanotechnology or from self-assembling perspectives. Herein, we wish to report our results for the synthesis, characterization, and assembling properties of asymmetrical bDNA molecules that are able to generate linear and circular bDNA constructs. Our strategy for the generation of bDNA is based on a branching point that makes use of a novel protecting-group strategy. The bDNA units were generated by means of automated DNA synthesis methods and were used to generate novel objects by employing chemical and biological techniques. The entities generated might be useful building blocks for DNA-based nanobiotechnology.

Published

2007

50. An efficient method for the construction of functionalized DNA bearing amino acid groups through cross-coupling reactions of nucleoside triphosphates followed by primer extension or PCR.

Author

Capek P, Cahová H, Pohl R, Hocek M, Gloeckner C, and Marx A

Subjects

Base Sequence, Circular Dichroism, DNA-Directed DNA Polymerase metabolism, Molecular Sequence Data, Molecular Structure, Nucleosides chemistry, Amino Acids chemistry, DNA chemistry, DNA genetics, DNA Primers genetics, Nucleotides chemistry, Polymerase Chain Reaction methods

Abstract

Single-step aqueous cross-coupling reactions of nucleobase-halogenated 2'-deoxynucleosides (8-bromo-2'-deoxyadenosine, 7-iodo-7-deaza-2'-deoxyadenosine, or 5-iodo-2'-deoxy-uridine) or their 5'-triphosphates with 4-boronophenylalanine or 4-ethynylphenylalanine have been developed and used for efficient synthesis of modified 2'-deoxynucleoside triphosphates (dNTPs) bearing amino acid groups. These dNTPs were then tested as substrates for DNA polymerases for construction of functionalized DNA through primer extension and PCR. While 8-substituted adenosine triphosphates were poor substrates for DNA polymerases, the corresponding 7-substituted 7-deazaadenine and 5-substituted uracil nucleotides were efficiently incorporated in place of dATP or dTTP, respectively, by Pwo (Pyrococcus woesei) DNA polymerase. Nucleotides bearing the amino acid connected through the less bulky acetylene linker were incorporated more efficiently than those directly linked through a more bulky phenylene group. In addition, combinations of modified dATPs and dTTPs were incorporated by Pwo polymerase. Novel functionalized DNA duplexes bearing amino acid moieties were prepared by this two-step approach. PCR can be used for amplification of duplexes bearing large number of modifications, while primer extension is suitable for introduction of just one or several modifications in a single DNA strand.

Published

2007