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1. Integrated multi-omics reveals anaplerotic rewiring in methylmalonyl-CoA mutase deficiency

Author

Forny, Patrick, Bonilla, Ximena, Lamparter, David, Shao, Wenguang, Plessl, Tanja, Frei, Caroline, Bingisser, Anna, Goetze, Sandra, van Drogen, Audrey, Harshman, Keith, Pedrioli, Patrick G. A., Howald, Cedric, Poms, Martin, Traversi, Florian, Bürer, Céline, Cherkaoui, Sarah, Morscher, Raphael J., Simmons, Luke, Forny, Merima, Xenarios, Ioannis, Aebersold, Ruedi, Zamboni, Nicola, Rätsch, Gunnar, Dermitzakis, Emmanouil T., Wollscheid, Bernd, Baumgartner, Matthias R., and Froese, D. Sean

Published
2023
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2. Quantification of the spread of SARS-CoV-2 variant B.1.1.7 in Switzerland

Author

Chen, Chaoran, Nadeau, Sarah Ann, Topolsky, Ivan, Manceau, Marc, Huisman, Jana S., Jablonski, Kim Philipp, Fuhrmann, Lara, Dreifuss, David, Jahn, Katharina, Beckmann, Christiane, Redondo, Maurice, Noppen, Christoph, Risch, Lorenz, Risch, Martin, Wohlwend, Nadia, Kas, Sinem, Bodmer, Thomas, Roloff, Tim, Stange, Madlen, Egli, Adrian, Eckerle, Isabella, Kaiser, Laurent, Denes, Rebecca, Feldkamp, Mirjam, Nissen, Ina, Santacroce, Natascha, Burcklen, Elodie, Aquino, Catharine, de Gouvea, Andreia Cabral, Moccia, Maria Domenica, Grüter, Simon, Sykes, Timothy, Opitz, Lennart, White, Griffin, Neff, Laura, Popovic, Doris, Patrignani, Andrea, Tracy, Jay, Schlapbach, Ralph, Dermitzakis, Emmanouil T., Harshman, Keith, Xenarios, Ioannis, Pegeot, Henri, Cerutti, Lorenzo, Penet, Deborah, Blin, Anthony, Elies, Melyssa, Althaus, Christian L., Beisel, Christian, Beerenwinkel, Niko, Ackermann, Martin, and Stadler, Tanja

Published
2021
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3. Gene expression across mammalian organ development

Author

Cardoso-Moreira, Margarida, Halbert, Jean, Valloton, Delphine, Velten, Britta, Chen, Chunyan, Shao, Yi, Liechti, Angélica, Ascenção, Kelly, Rummel, Coralie, Ovchinnikova, Svetlana, Mazin, Pavel V., Xenarios, Ioannis, Harshman, Keith, Mort, Matthew, Cooper, David N., Sandi, Carmen, Soares, Michael J., Ferreira, Paula G., Afonso, Sandra, Carneiro, Miguel, Turner, James M. A., VandeBerg, John L., Fallahshahroudi, Amir, Jensen, Per, Behr, Rüdiger, Lisgo, Steven, Lindsay, Susan, Khaitovich, Philipp, Huber, Wolfgang, Baker, Julie, Anders, Simon, Zhang, Yong E., and Kaessmann, Henrik

Published
2019
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4. The genome of the fire ant Solenopsis invicta

Author

Wurm, Yannick, Wang, John, Riba-Grognuz, Oksana, Corona, Miguel, Nygaard, Sanne, Hunt, Brendan G., Ingram, Krista K., Falquet, Laurent, Nipitwattanaphon, Mingkwan, Gotzek, Dietrich, Dijkstra, Michiel B., Oettler, Jan, Comtesse, Fabien, Shih, Cheng-Jen, Wu, Wen-Jer, Yang, Chin-Cheng, Thomas, Jerome, Beaudoing, Emmanuel, Pradervand, Sylvain, Flegel, Volker, Cook, Erin D., Fabbretti, Roberto, Stockinger, Heinz, Long, Li, Farmerie, William G., Oakey, Jane, Boomsma, Jacobus J., Pamilo, Pekka, Yi, Soojin V., Heinze, Jürgen, Goodisman, Michael A. D., Farinelli, Laurent, Harshman, Keith, Hulo, Nicolas, Cerutti, Lorenzo, Xenarios, Ioannis, DeWayne Shoemaker, Keller, Laurent, and Robinson, Gene E.

Published
2011

5. Integrated multi-omics reveals anaplerotic insufficiency in methylmalonyl-CoA mutase deficiency

Author

Forny, Patrick, Bonilla Bustillo, Ximena, Lamparter, David, Shao, Wenguang, Plessl, Tanja, Frei, Caroline, Bingisser, Anna, Goetze, Sandra, van Drogen, Audrey, Harshman, Keith, Pedrioli, Patrick G.A., Howald, Cedric, Poms, Martin, Traversi, Florian, Cherkaoui, Sarah, Morscher, Raphael J., Simmons, Luke, Forny, Merima, Xenarios, Ioannis, Aebersold, Rudolf, Zamboni, Nicola, Rätsch, Gunnar, Dermitzakis, Emmanouil, Wollscheid, Bernd, Baumgartner, Matthias R., and Froese, D. Sean

Abstract

Multi-layered omics approaches can help define relationships between genetic factors, biochemical processes and phenotypes thus extending research of inherited diseases beyond identifying their monogenic cause 1. We implemented a multi-layered omics approach for the inherited metabolic disorder methylmalonic aciduria (MMA). We performed whole genome sequencing, transcriptomic sequencing, and mass spectrometry-based proteotyping from matched primary fibroblast samples of 230 individuals (210 affected, 20 controls) and related the molecular data to 105 phenotypic features. Integrative analysis identified a molecular diagnosis for 84% (177/210) of affected individuals, the majority (148) of whom had pathogenic variants in methylmalonyl-CoA mutase (MMUT). Untargeted analysis of all three omics layers revealed dysregulation of the TCA cycle and surrounding metabolic pathways, a finding that was further corroborated by multi-organ metabolomics of a hemizygous Mmut mouse model. Integration of phenotypic disease severity indicated downregulation of oxoglutarate dehydrogenase and upregulation of glutamate dehydrogenase, two proteins involved in glutamine anaplerosis of the TCA cycle. The relevance of disturbances in this pathway was supported by metabolomics and isotope tracing studies which showed decreased glutamine-derived anaplerosis in MMA. We further identified MMUT to physically interact with both, oxoglutarate dehydrogenase complex components and glutamate dehydrogenase providing evidence for a multi-protein metabolon that orchestrates TCA cycle anaplerosis. This study emphasizes the utility of a multi-modal omics approach to investigate metabolic diseases and highlights glutamine anaplerosis as a potential therapeutic intervention point in MMA.Take home message Combination of integrative multi-omics technologies with clinical and biochemical features leads to an increased diagnostic rate compared to genome sequencing alone and identifies anaplerotic rewiring as a targetable feature of the rare inborn error of metabolism methylmalonic aciduria.Competing Interest StatementThe authors have declared no competing interest.Funding StatementThis project was funded by the ETH domain strategic focus area Personalized Health and Related Technology (PHRT; https://www.sfa-phrt.ch).Author DeclarationsI confirm all relevant ethical guidelines have been followed, and any necessary IRB and/or ethics committee approvals have been obtained.YesThe details of the IRB/oversight body that provided approval or exemption for the research described are given below:The Ethics Committee of the Canton of Zurich, Switzerland gave ethical approval for this work.I confirm that all necessary patient/participant consent has been obtained and the appropriate institutional forms have been archived, and that any patient/participant/sample identifiers included were not known to anyone (e.g., hospital staff, patients or participants themselves) outside the research group so cannot be used to identify individuals.YesI understand that all clinical trials and any other prospective interventional studies must be registered with an ICMJE-approved registry, such as ClinicalTrials.gov. I confirm that any such study reported in the manuscript has been registered and the trial registration ID is provided (note: if posting a prospective study registered retrospectively, please provide a statement in the trial ID field explaining why the study was not registered in advance).YesI have followed all appropriate research reporting guidelines and uploaded the relevant EQUATOR Network research reporting checklist(s) and other pertinent material as supplementary files, if applicable.YesAll data produced in the present study are available upon reasonable request to the authors., medRxiv

Published
2022
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7. A Strong Candidate for the Breast and Ovarian Cancer Susceptibility Gene BRCA1

Author

Miki, Yoshio, Swensen, Jeff, Shattuck-Eidens, Donna, Futreal, P. Andrew, Harshman, Keith, Tavtigian, Sean, Liu, Qingyun, Cochran, Charles, Bennett, L. Michelle, Ding, Wei, Bell, Russell, Rosenthal, Judith, Hussey, Charles, Tran, Thanh, McClure, Melody, Frye, Cheryl, Hattier, Tom, Phelps, Robert, Haugen-Strano, Astrid, Katcher, Harold, Yakumo, Kazuko, Gholami, Zahra, Shaffer, Daniel, Stone, Steven, Bayer, Steven, Wray, Christian, Bogden, Robert, Dayananth, Priya, Ward, John, Tonin, Patricia, Narod, Steven, Bristow, Pam K., Norris, Frank H., Helvering, Leah, Morrison, Paul, Rosteck, Paul, Lai, Mei, Barrett, J. Carl, Lewis, Cathryn, Neuhausen, Susan, Cannon-Albright, Lisa, Goldgar, David, Wiseman, Roger, Kamb, Alexander, and Skolnick, Mark H.

Published
1994

10. Comparative genome analysis of Pseudomonas knackmussii B13, the first bacterium known to degrade chloroaromatic compounds

Author

Miyazaki, Ryo, Bertelli, Claire, Benaglio, Paola, Canton, Jonas, De Coi, Nicoló, Gharib, Walid H., Gjoksi, Bebeka, Goesmann, Alexander, Greub, Gilbert, Harshman, Keith, Linke, Burkhard, Mikulic, Josip, Mueller, Linda, Nicolas, Damien, Robinson-Rechavi, Marc, Rivolta, Carlo, Roggo, Clémence, Roy, Shantanu, Sentchilo, Vladimir, Siebenthal, Alexandra Von, Falquet, Laurent, and van der Meer, Jan Roelof

Published
2015
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11. Differential gene expression in the pathogenic dermatophyte Arthroderma benhamiae in vitro versus during infection

Author

Staib, Peter, Zaugg, Christophe, Mignon, Bernard, Weber, Johann, Grumbt, Maria, Pradervand, Sylvain, Harshman, Keith, and Monod, Michel

Subjects
DNA microarrays -- Usage, Dermatophytes -- Health aspects, Dermatophytes -- Genetic aspects, Dermatophytes -- Research, Gene expression -- Research, Virulence (Microbiology) -- Genetic aspects, Virulence (Microbiology) -- Research, Biological sciences
Abstract

Although dermatophytes are the most common agents of superficial mycoses in humans and animals, the molecular basis of the pathogenicity of these fungi is largely unknown. In vitro digestion of keratin by dermatophytes is associated with the secretion of multiple proteases, which are assumed to be responsible for their particular specialization to colonize and degrade keratinized host structures during infection. To investigate the role of individual secreted proteases in dermatophytosis, a guinea pig infection model was established for the zoophilic dermatophyte Arthroderma benhamiae, which causes highly inflammatory cutaneous infections in humans and rodents. By use of a cDNA microarray covering approximately 20-25% of the A. benhamiae genome and containing sequences of at least 23 protease genes, we revealed a distinct in vivo protease gene expression profile in the fungal cells, which was surprisingly different from the pattern elicited during in vitro growth on keratin. Instead of the major in vitro-expressed proteases, others were activated specifically during infection. These enzymes are therefore suggested to fulfil important functions that are not exclusively associated with the degradation of keratin. Most notably, the gene encoding the serine protease subtilisin 6, which is a known major allergen in the related dermatophyte Trichophyton rubrum and putatively linked to host inflammation, was found to be the most strongly upregulated gene during infection. In addition, our approach identified other candidate pathogenicity-related factors in A. benhamiae, such as genes encoding key enzymes of the glyoxylate cycle and an opsin-related protein. Our work provides what we believe to be the first broad-scale gene expression profile in human pathogenic dermatophytes during infection, and points to putative virulence-associated mechanisms that make these micro-organisms the most successful aetiological agents of superficial mycoses. DOI 10.1099/mic.0.033464-0

Published
2010

13. Activation of the epidermal growth factor signalling pathway by tissue plasminogen activator in pancreas cancer cells

Author

Hurtado, Mariano, Lozano, Juan Jose, Castellanos, Elisabeth, Lopez-Fernandez, Luis A., Harshman, Keith, Martinez-A, Carlos, Ortiz, Angel R., Thomson, Timothy M., and Paciucci, Rosanna

Subjects
Epidermal growth factor -- Research, Epidermal growth factor -- Physiological aspects, Tissue plasminogen activator -- Research, Tissue plasminogen activator -- Physiological aspects, Pancreatic cancer -- Research, Pancreatic cancer -- Physiological aspects, Cancer cells -- Research, Cancer cells -- Physiological aspects, Health
Published
2007

17. Rates of p16 (MTS1) Mutations in Primary Tumors with 9p Loss

Author

Cairns, Paul, Mao, Li, Merlo, Adrian, Lee, Daniel J., Schwab, Donna, Eby, Yolanda, Tokino, Kaori, van der Riet, Peter, Blaugrund, James E., Sidransky, David, Kamb, Alexander, Liu, Qingyun, Harshman, Keith, Tavtigian, Sean, Cordon-Cardo, Carlos, and Skolnick, Mark H.

Published
1994

18. BRCA1 Mutations in Primary Breast and Ovarian Carcinomas

Author

Futreal, P. Andrew, Liu, Qingyun, Shattuck-Eidens, Donna, Cochran, Charles, Harshman, Keith, Tavtigian, Sean, Bennett, L. Michelle, Haugen-Strano, Astrid, Swensen, Jeff, Miki, Yoshio, Eddington, Ken, McClure, Melody, Frye, Cheryl, Weaver-Feldhaus, Jane, Ding, Wei, Gholami, Zahra, Söderkvist, Peter, Terry, Lori, Jhanwar, Suresh, Berchuck, Andrew, Iglehart, J. Dirk, Marks, Jeff, Ballinger, Dennis G., Barrett, J. Carl, Skolnick, Mark H., Kamb, Alexander, and Wiseman, Roger

Published
1994

20. INTEGRATED MULTI-OMIC ANALYSIS OF A RARE INBORN ERROR OF METABOLISM

Author

Forny, Patrick, Bonilla, Ximena, Lamparter, David, Shao, Wenguang, Plessl, Tanja, Frei, Caroline, Bingisser, Anna, Goetze, Sandra, van Drogen, Audrey, Harshman, Keith, Pedrioli, Patrick, Traversi, Florian, Xenarios, Ioannis, Aebersold, Ruedi, Zamboni, Nicola, Rätsch, Gunnar, Dermitzakis, Emmanouil, Wollscheid, Bernd, Froese, D. Sean, and Baumgartner, Matthias R.

Published
2022
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21. BRCA 1 Mutations in Primary Breast and Ovarian Carcinomas

Author

Futreal, P. Andrew, Liu, Qingyun, Shattuck-Eidens, Donna, Cochran, Charles, Harshman, Keith, Tavtigian, Sean, Bennett, L. Michelle, Haugen-Strano, Astrid, Swensen, Jeff, Miki, Yoshio, Eddington, Ken, McClure, Melody, Frye, Cheryl, Weaver-Feldhaus, Jane, Ding, Wei, Gholami, Zahra, Soederkvist, Peter, Terry, Lori, Jhanwar, Suresh, Berchuck, Andrew, Iglehart, J. Dirk, Marks, Jeff, Ballinger, Dennis G., Barrett, J. Carl, Skolnick, Mark H., and Kamb, Alexander

Published
1994

22. Rates of p16 (MTS-1) mutations in primary tumors with 9p loss

Author

Cairns, Paul, Mao, Li, Merlo, Adrian, Lee, Daniel J., Schwab, Donna, Eby, Yolanda, Tokino, Kaori, Van der Riet, Peter, Blaugrund, James E., Sidransky, David, Kamb, Alexander, Liu, Qingyun, Harshman, Keith, Tavtigian, Sean, Cordon-Cardo, Carlos, and Skolnick, Mark H.

Subjects
Research, Genetic aspects, Cancer genetics -- Genetic aspects -- Research, Tumor suppressor genes -- Research -- Genetic aspects, Cancer -- Genetic aspects
Abstract

A critical area of chromosomal loss at region 9p21-22 has been implicated in the genesis of different types of primary tumors. Initial observations defined deletions of this region in leukemia, [...]

Published
1994

23. NANS-mediated synthesis of sialic acid is required for brain and skeletal development

Author

van Karnebeek, Clara D M, Bonafé, Luisa, Wen, Xiao-Yan, Tarailo-Graovac, Maja, Balzano, Sara, Royer-Bertrand, Beryl, Ashikov, Angel, Garavelli, Livia, Mammi, Isabella, Turolla, Licia, Breen, Catherine, Donnai, Dian, Cormier, Valerie, Heron, Delphine, Nishimura, Gen, Uchikawa, Shinichi, Campos-Xavier, Belinda, Rossi, Antonio, Hennet, Thierry, Brand-Arzamendi, Koroboshka, Rozmus, Jacob, Harshman, Keith, Stevenson, Brian J, Girardi, Enrico, Superti-Furga, Giulio, Dewan, Tammie, Collingridge, Alissa, Halparin, Jessie, Ross, Colin J, Van Allen, Margot I, et al, University of Zurich, and van Karnebeek, Clara D M

Subjects
1311 Genetics, 570 Life sciences, biology, 610 Medicine & health, 10052 Institute of Physiology
Published
2016
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24. FAM111A Mutations Result in Hypoparathyroidism and Impaired Skeletal Development

Author

Unger, Sheila, Górna, Maria W., Le Béchec, Antony, Do Vale-Pereira, Sonia, Bedeschi, Maria Francesca, Geiberger, Stefan, Grigelioniene, Giedre, Horemuzova, Eva, Lalatta, Faustina, Lausch, Ekkehart, Magnani, Cinzia, Nampoothiri, Sheela, Nishimura, Gen, Petrella, Duccio, Rojas-Ringeling, Francisca, Utsunomiya, Akari, Zabel, Bernhard, Pradervand, Sylvain, Harshman, Keith, Campos-Xavier, Belinda, Bonafé, Luisa, Superti-Furga, Giulio, Stevenson, Brian, and Superti-Furga, Andrea

Published
2013
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25. Comparative genomic and phylogeographic analysis of Mycobacterium leprae.: Phylogeography of leprosy (titre du fichier auteur)

Author

Monot, Marc, Honoré, Nadine, Garnier, Thierry, Zidane, Nora, Sherafi, Diana, Paniz-Mondolfi, Alberto, Matsuoka, Masanori, Taylor, G Michael, Donoghue, Helen D, Bouwman, Abi, Mays, Simon, Watson, Claire, Lockwood, Diana, Khamesipour, Ali, Khamispour, Ali, Dowlati, Yahya, Jianping, Shen, Rea, Thomas H, Vera-Cabrera, Lucio, Stefani, Mariane M, Banu, Sayera, Macdonald, Murdo, Sapkota, Bishwa Raj, Spencer, John S, Thomas, Jérôme, Harshman, Keith, Singh, Pushpendra, Busso, Philippe, Gattiker, Alexandre, Rougemont, Jacques, Brennan, Patrick J, Cole, Stewart T, Instituto de Biomedicina, Instituto de biomedicina, Leprosy Research Centre [Japan], National Institute of Infectious Diseases [Tokyo], Centre for Infectious Diseases and International Health, UCL, Faculty of Life Sciences [Manchester], The University of Manchester [Manchester], Ancient Monuments Laboratory, English Heritage Centre for Archaeology, London School of Hygiene and Tropical Medicine (LSHTM), Center for Research and Training in Skin Diseases and Leprosy, Tehran University of Medical Sciences, National Center for Leprosy Control [China], Chinese Center for Disease Control and Prevention (China CDC), Department of Dermatology [Los Angeles, USA], Keck School of Medicine [Los Angeles], Servicio de Dermatología, Hospital Universitario José E. Gonzalez, Tropical Pathology and Public Health Institute [Brazil], Federal University of Goias, International Centre for Diarrhoeal Disease Research, Bangladesh (ICDDR,B), Leprosy Mission Nepal, Anandaban Hospital [Nepal], Department of Microbiology, Immunology and Pathology, Colorado State University [Fort Collins] (CSU), Center for Integrative Genomics - Institute of Bioinformatics, Génopode (CIG), University of Lausanne, Global Health Institute, Ecole Polytechnique Fédérale de Lausanne (EPFL), Bioinformatics and Biostatistics Core Facility [Lausanne], This work received the financial support of the Fondation Raoul Follereau, the Génopole programme, and the US National Institutes of Health, National Institute of Allergy and Infectious Diseases (grant RO1-AI47197-01A1 and contract NO1-AI25469)., Instituto de Biomedicina [Caracas], Universidad Central de Venezuela (UCV), University of Manchester [Manchester], University of Southern California (USC)-University of Southern California (USC), Swiss Institute of Bioinformatics [Lausanne] (SIB), Université de Lausanne (UNIL)-Université de Lausanne (UNIL), and Global Health Institute - Institut d'Infectiologie [Lausanne]

Subjects
MESH: Geography, Pseudogene, Biology, MESH: Genome, Bacterial, medicine.disease_cause, [SDV.BBM.BM] Life Sciences [q-bio]/Biochemistry, Molecular Biology/Molecular biology, Polymorphism, Single Nucleotide, Genome, Article, 03 medical and health sciences, Phylogenetics, Leprosy, Genetics, medicine, Humans, MESH: Phylogeny, Genotyping, Mycobacterium leprae, Phylogeny, 030304 developmental biology, Recombination, Genetic, Whole genome sequencing, Comparative genomics, Mycobacterium lepromatosis, 0303 health sciences, MESH: Humans, Geography, 030306 microbiology, MESH: Polymorphism, Single Nucleotide, [SDV.BBM.BM]Life Sciences [q-bio]/Biochemistry, Molecular Biology/Molecular biology, biology.organism_classification, MESH: Leprosy, 3. Good health, Genes, Bacterial, MESH: Recombination, Genetic, MESH: Mycobacterium leprae, MESH: Genes, Bacterial, Genome, Bacterial
Abstract

International audience; Reductive evolution and massive pseudogene formation have shaped the 3.31-Mb genome of Mycobacterium leprae, an unculturable obligate pathogen that causes leprosy in humans. The complete genome sequence of M. leprae strain Br4923 from Brazil was obtained by conventional methods (6x coverage), and Illumina resequencing technology was used to obtain the sequences of strains Thai53 (38x coverage) and NHDP63 (46x coverage) from Thailand and the United States, respectively. Whole-genome comparisons with the previously sequenced TN strain from India revealed that the four strains share 99.995% sequence identity and differ only in 215 polymorphic sites, mainly SNPs, and by 5 pseudogenes. Sixteen interrelated SNP subtypes were defined by genotyping both extant and extinct strains of M. leprae from around the world. The 16 SNP subtypes showed a strong geographical association that reflects the migration patterns of early humans and trade routes, with the Silk Road linking Europe to China having contributed to the spread of leprosy.

Published
2009
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26. The Genome of the Toluene-Degrading Pseudomonas veronii Strain 1YdBTEX2 and Its Differential Gene Expression in Contaminated Sand.

Author

Morales, Marian, Sentchilo, Vladimir, Bertelli, Claire, Komljenovic, Andrea, Kryuchkova-Mostacci, Nadezda, Bourdilloud, Audrey, Linke, Burkhard, Goesmann, Alexander, Harshman, Keith, Segers, Francisca, Delapierre, Fabien, Fiorucci, Damien, Seppey, Mathieu, Trofimenco, Evgeniya, Berra, Pauline, El Taher, Athimed, Loiseau, Chloé, Roggero, Dejan, Sulfiotti, Madeleine, and Etienne, Angela

Subjects
PSEUDOMONAS, GENE expression in bacteria, SOIL restoration, NUCLEOTIDE sequencing, CHEMOTAXIS, BACTERIA
Abstract

The natural restoration of soils polluted by aromatic hydrocarbons such as benzene, toluene, ethylbenzene and m- and p-xylene (BTEX) may be accelerated by inoculation of specific biodegraders (bioaugmentation). Bioaugmentation mainly involves introducing bacteria that deploy their metabolic properties and adaptation potential to survive and propagate in the contaminated environment by degrading the pollutant. In order to better understand the adaptive response of cells during a transition to contaminated material, we analyzed here the genome and short-term (1 h) changes in genome-wide gene expression of the BTEX-degrading bacterium Pseudomonas veronii 1YdBTEX2 in non-sterile soil and liquid medium, both in presence or absence of toluene. We obtained a gapless genome sequence of P. veronii 1YdBTEX2 covering three individual replicons with a total size of 8 Mb, two of which are largely unrelated to current known bacterial replicons. One-hour exposure to toluene, both in soil and liquid, triggered massive transcription (up to 208-fold induction) of multiple gene clusters, such as toluene degradation pathway(s), chemotaxis and toluene efflux pumps. This clearly underlines their key role in the adaptive response to toluene. In comparison to liquid medium, cells in soil drastically changed expression of genes involved in membrane functioning (e.g., lipid composition, lipid metabolism, cell fatty acid synthesis), osmotic stress response (e.g., polyamine or trehalose synthesis, uptake of potassium) and putrescine metabolism, highlighting the immediate response mechanisms of P. veronii 1YdBTEX2 for successful establishment in polluted soil. [ABSTRACT FROM AUTHOR]

Published
2016
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27. Comparative transcriptome profiling of the injured zebrafish and mouse hearts identifies miRNA-dependent repair pathways.

Author

Crippa, Stefania, Nemir, Mohamed, Ounzain, Samir, Ibberson, Mark, Berthonneche, Corinne, Sarre, Alexandre, Boisset, Gaëlle, Maison, Damien, Harshman, Keith, Xenarios, Ioannis, Diviani, Dario, Schorderet, Daniel, and Pedrazzini, Thierry

Subjects
HEART injuries, ZEBRA danio, MICRORNA, CARDIAC regeneration, CELL cycle
Abstract

Aims: The adult mammalian heart has poor regenerative capacity. In contrast, the zebrafish heart retains a robust capacity for regeneration into adulthood. These distinct responses are consequences of a differential utilization of evolutionaryconserved gene regulatory networks in the damaged heart. To systematically identify miRNA-dependent networks controlling cardiac repair following injury, we performed comparative gene and miRNA profiling of the cardiac transcriptome in adult mice and zebrafish. Methods and results: Using an integrated approach, we show that 45 miRNA-dependent networks, involved in critical biological pathways, are differentially modulated in the injured zebrafish vs. mouse hearts. We study, more particularly, the miR-26adependent response. Therefore, miR-26a is down-regulated in the fish heart after injury, whereas its expression remains constant in the mouse heart. Targets of miR-26a involve activators of the cell cycle and Ezh2, a component of the polycomb repressive complex 2 (PRC2). Importantly, PRC2 exerts repressive functions on negative regulators of the cell cycle. In cultured neonatal cardiomyocytes, inhibition of miR-26a stimulates, therefore, cardiomyocyte proliferation. Accordingly, miR-26a knockdown prolongs the proliferative window of cardiomyocytes in the post-natal mouse heart. Conclusions: This novel strategy identifies a series of miRNAs and associated pathways, in particular miR-26a, which represent attractive therapeutic targets for inducing repair in the injured heart. [ABSTRACT FROM AUTHOR]

Published
2016
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28. Sequencing and characterizing the genome of Estrella lausannensis as an undergraduate project: training students and biological insights.

Author

Bertelli, Claire, Aeby, Sèbastien, Chassot, Bèrènice, Clulow, James, Hilfiker, Olivier, Rappo, Samuel, Ritzmann, Sèbastien, Schumacher, Paolo, Terrettaz, Cèline, Benaglio, Paola, Falquet, Laurent, Farinelli, Laurent, Gharib, Walid H., Goesmann, Alexander, Harshman, Keith, Linke, Burkhard, Miyazaki, Ryo, Rivolta, Carlo, Robinson-Rechavi, Marc, and van der Meer, Jan Roelof

Subjects
NUCLEOTIDE sequencing, GENOMICS, LIFE sciences, INTEGRASES, TOXINS
Abstract

With the widespread availability of high-throughput sequencing technologies, sequencing projects have become pervasive in the molecular life sciences. The huge bulk of data generated daily must be analyzed further by biologists with skills in bioinformatics and by "embedded bioinformaticians, " i.e., bioinformaticians integrated in wet lab research groups. Thus, students interested in molecular life sciences must be trained in the main steps of genomics: sequencing, assembly, annotation and analysis. To reach that goal, a practical course has been set up for master students at the University of Lausanne: the "Sequence a genome" class. At the beginning of the academic year, a few bacterial species whose genome is unknown are provided to the students, who sequence and assemble the genome(s) and perform manual annotation. Here, we report the progress of the first class from September 2010 to June 2011 and the results obtained by seven master students who specifically assembled and annotated the genome of Estrella lausannensis, an obligate intracellular bacterium related to Chlamydia. The draft genome of Estrella is composed of 29 scaffolds encompassing 2,819,825 bp that encode for 2233 putative proteins. Estrella also possesses a 9136 bp plasmid that encodes for 14 genes, among which we found an integrase and a toxin/antitoxin module. Like all other members of the Chlamydiales order, Estrella possesses a highly conserved type III secretion system, considered as a key virulence factor. The annotation of the Estrella genome also allowed the characterization of the metabolic abilities of this strictly intracellular bacterium. Altogether, the students provided the scientific community with the Estrella genome sequence and a preliminary understanding of the biology of this recently-discovered bacterial genus, while learning to use cutting-edge technologies for sequencing and to perform bioinformatics analyses. [ABSTRACT FROM AUTHOR]

Published
2015
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29. Comparative genome analysis of P seudomonas knackmussii B13, the first bacterium known to degrade chloroaromatic compounds.

Author

Miyazaki, Ryo, Bertelli, Claire, Benaglio, Paola, Canton, Jonas, De Coi, Nicoló, Gharib, Walid H., Gjoksi, Bebeka, Goesmann, Alexander, Greub, Gilbert, Harshman, Keith, Linke, Burkhard, Mikulic, Josip, Mueller, Linda, Nicolas, Damien, Robinson ‐ Rechavi, Marc, Rivolta, Carlo, Roggo, Clémence, Roy, Shantanu, Sentchilo, Vladimir, and Siebenthal, Alexandra Von

Subjects
BACTERIAL genomes, AROMATIC compounds, PSEUDOMONAS, COMPARATIVE genomics, BACTERIAL metabolism, BIOREMEDIATION, NUCLEOTIDE sequence
Abstract

P seudomonas knackmussii B13 was the first strain to be isolated in 1974 that could degrade chlorinated aromatic hydrocarbons. This discovery was the prologue for subsequent characterization of numerous bacterial metabolic pathways, for genetic and biochemical studies, and which spurred ideas for pollutant bioremediation. In this study, we determined the complete genome sequence of B13 using next generation sequencing technologies and optical mapping. Genome annotation indicated that B13 has a variety of metabolic pathways for degrading monoaromatic hydrocarbons including chlorobenzoate, aminophenol, anthranilate and hydroxyquinol, but not polyaromatic compounds. Comparative genome analysis revealed that B13 is closest to P seudomonas denitrificans and P seudomonas aeruginosa. The B13 genome contains at least eight genomic islands [prophages and integrative conjugative elements ( ICEs)], which were absent in closely related pseudomonads. We confirm that two ICEs are identical copies of the 103 kb self-transmissible element ICE clc that carries the genes for chlorocatechol metabolism. Comparison of ICE clc showed that it is composed of a variable and a 'core' region, which is very conserved among proteobacterial genomes, suggesting a widely distributed family of so far uncharacterized ICE. Resequencing of two spontaneous B13 mutants revealed a number of single nucleotide substitutions, as well as excision of a large 220 kb region and a prophage that drastically change the host metabolic capacity and survivability. [ABSTRACT FROM AUTHOR]

Published
2015
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30. Genome-Wide RNA Polymerase II Profiles and RNA Accumulation Reveal Kinetics of Transcription and Associated Epigenetic Changes During Diurnal Cycles

Author

Le Martelot, Gwendal, Canella, Donatella, Symul, Laura, Migliavacca, Eugenia, Gilardi, Federica, Liechti, Robin, Martin, Olivier, Harshman, Keith, Delorenzi, Mauro, Desvergne, Béatrice, Herr, Winship, Deplancke, Bart, Schibler, Ueli, Rougemont, Jacques, Guex, Nicolas, Hernandez, Nouria, and Naef, Felix

Subjects
RNA polymerases, CIRCADIAN rhythms, CHROMATIN, GENE expression, LIVER, LABORATORY mice, GENETIC transcription
Abstract

Genome-wide rhythms in RNA polymerase II loading and dynamic chromatin remodeling underlie periodic gene expression during diurnal cycles in the mouse liver. [ABSTRACT FROM AUTHOR]

Published
2012
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31. Context-Dependent Dual Role of SKI8 Homologs in mRNA Synthesis and Turnover.

Author

Dorcey, Eavan, Rodriguez-Villalon, Antia, Salinas, Paula, Santuari, Luca, Pradervand, Sylvain, Harshman, Keith, and Hardtke, Christian S.

Subjects
EUKARYOTIC cells, ENZYMES, RNA polymerases, EXOSOMES, CYTOPLASM
Abstract

Eukaryotic mRNA transcription and turnover is controlled by an enzymatic machinery that includes RNA polymerase II and the 3' to 5' exosome. The activity of these protein complexes is modulated by additional factors, such as the nuclear RNA polymerase II-associated factor 1 (Paf1c) and the cytoplasmic Superkiller (SKI) complex, respectively. Their components are conserved across uni- as well as multi-cellular organisms, including yeast, Arabidopsis, and humans. Among them, SKI8 displays multiple facets on top of its cytoplasmic role in the SKI complex. For instance, nuclear yeast ScSKI8 has an additional function in meiotic recombination, whereas nuclear human hSKI8 (unlike ScSKI8) associates with Paf1c. The Arabidopsis SKI8 homolog VERNALIZATION INDEPENDENT 3 (VIP3) has been found in Paf1c as well; however, whether it also has a role in the SKI complex remains obscure so far. We found that transgenic VIP3-GFP, which complements a novel vip3 mutant allele, localizes to both nucleus and cytoplasm. Consistently, biochemical analyses suggest that VIP3-GFP associates with the SKI complex. A role of VIP3 in the turnover of nuclear encoded mRNAs is supported by random-primed RNA sequencing of wild-type and vip3 seedlings, which indicates mRNA stabilization in vip3. Another SKI subunit homolog mutant, ski2, displays a dwarf phenotype similar to vip3. However, unlike vip3, it displays neither early flowering nor flower development phenotypes, suggesting that the latter reflect VIP3's role in Paf1c. Surprisingly then, transgenic ScSKI8 rescued all aspects of the vip3 phenotype, suggesting that the dual role of SKI8 depends on species-specific cellular context. [ABSTRACT FROM AUTHOR]

Published
2012
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32. Exome sequencing identifies recurrent somatic MAP2K1 and MAP2K2 mutations in melanoma.

Author

Nikolaev, Sergey I, Rimoldi, Donata, Iseli, Christian, Valsesia, Armand, Robyr, Daniel, Gehrig, Corinne, Harshman, Keith, Guipponi, Michel, Bukach, Olesya, Zoete, Vincent, Michielin, Olivier, Muehlethaler, Katja, Speiser, Daniel, Beckmann, Jacques S, Xenarios, Ioannis, Halazonetis, Thanos D, Jongeneel, C Victor, Stevenson, Brian J, and Antonarakis, Stylianos E

Subjects
MELANOMA, ANTIBODY diversity, CELL lines, GERM cells, DNA repair, METASTASIS
Abstract

We performed exome sequencing to detect somatic mutations in protein-coding regions in seven melanoma cell lines and donor-matched germline cells. All melanoma samples had high numbers of somatic mutations, which showed the hallmark of UV-induced DNA repair. Such a hallmark was absent in tumor sample-specific mutations in two metastases derived from the same individual. Two melanomas with non-canonical BRAF mutations harbored gain-of-function MAP2K1 and MAP2K2 (MEK1 and MEK2, respectively) mutations, resulting in constitutive ERK phosphorylation and higher resistance to MEK inhibitors. Screening a larger cohort of individuals with melanoma revealed the presence of recurring somatic MAP2K1 and MAP2K2 mutations, which occurred at an overall frequency of 8%. Furthermore, missense and nonsense somatic mutations were frequently found in three candidate melanoma genes, FAT4, LRP1B and DSC1. [ABSTRACT FROM AUTHOR]

Published
2012
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37. Comparison of the positional cloning methods used to isolate the BRCA1 gene.

Author

Harshman, Keith, Bell, Russell, Rosenthal, Judith, Katcher, Harold, MlKl, Yoshio, Swenson, Jeff, Gholami, Zahra, Frye, Cheryl, Ding, Wei, Dayananth, Priya, Eddington, Ken, Norris, Franklin H., Bristow, Pamela K., Phelps, Robert, Haltier, Thomas, Stone, Steven, Shaffer, Daniel, Bayer, Steven, Hussey, Charles, and Tran, Thanh

Published
1995

39. Isolation and characterization of factors that interact with eukaryotic transcriptional enhancers

Author

Harshman, Keith D.

Subjects
Chemistry
Abstract

The regulatory region controlling the transcription of the SV40 early genes provides a useful system in which to study the mechanisms of eukaryotic gene expression. The enhancer element of this region is composed of sequence motifs that can function independently or in combination to potentiate transcription in a wide range of cellular contexts. This thesis describes the purification and characterization of two proteins that specifically bind separate motifs. An enhancer binding protein was identified in bovine thymus extracts and purified to homogeneity. This factor, designated EP2, was shown by chemical and enzymatic footprinting techniques to bind the core as well as two pseudo-core sequences. In a DNase I footprinting experiment, EP2 was unable to bind to a mutated core sequence that is incapable of activating transcription in vivo. EP-2 was shown to consist of a group of polypeptides, ranging in molecular weight from 34 kd to 43 kd, each of which has the ability to bind to the core and two pseudo-core sequences. It was shown that the sequence bound by the mammalian transcription factor AP-1-- the AP-1 recognition element (ARE)-- was capable of activating transcription in yeast. The ARE is very similar in sequence to the GCN4 recognition element (GCRE), yet the ARE was shown to activate transcription in a gcn4 yeast strain. A protein present in yeast extracts, designated yAP-l, was shown to bind to the ARE and was purified to near homogeneity based on this ability. yAP-1 and AP-1 display remarkably similar biochemical and DNA binding characteristics. It was shown in vitro that yAP-1 can discriminate between the ARE and the GCRE, while GCN4 exhibits approximately equal affinities for the two elements. The structural gene encoding yAP-1 was isolated and characterized. The DNA binding domain of the protein was localized to a sequence of 93 amino-acids in the amino-terminus. This sequence was shown to have significant homology with domains in cJUN and GCN4, which have been ascribed the ability to bind DNA. The YAP1 gene was shown to be non-essential by gene disruption. DNA-affinity blot experiments performed using extracts from YAP1 and yap1 strains suggest the existence of a family of yeast genes encoding proteins that recognize the ARE.

Published
1989
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44. Cortical-Bone Fragility--Insights from sFRP4 Deficiency in Pyle's Disease.

Author

Simsek Kiper, Pelin O., Hiroaki Saito, Gori, Francesca, Unger, Sheila, Hesse, Eric, Yamana, Kei, Kiviranta, Riku, Solban, Nicolas, Liu, Jeff, Brommage, Robert, Boduroglu, Koray, Bonafé, Luisa, Campos-Xavier, Belinda, Dikoglu, Esra, Eastell, Richard, Gossiel, Fatma, Harshman, Keith, Nishimura, Gen, Girisha, Katta M., and Stevenson, Brian J.

Subjects
*BONE physiology, *BONE remodeling, *ANIMALS, *BIOLOGICAL models, *BONE morphogenetic proteins, *BONES, *CELLULAR signal transduction, *GLYCOPROTEINS, *HOMEOSTASIS, *MICE, *GENETIC mutation, *PROTEINS, *RESEARCH funding, *BONE density, *MULTIPLE epiphyseal dysplasia, *SEQUENCE analysis
Abstract

Background: Cortical-bone fragility is a common feature in osteoporosis that is linked to nonvertebral fractures. Regulation of cortical-bone homeostasis has proved elusive. The study of genetic disorders of the skeleton can yield insights that fuel experimental therapeutic approaches to the treatment of rare disorders and common skeletal ailments.Methods: We evaluated four patients with Pyle's disease, a genetic disorder that is characterized by cortical-bone thinning, limb deformity, and fractures; two patients were examined by means of exome sequencing, and two were examined by means of Sanger sequencing. After a candidate gene was identified, we generated a knockout mouse model that manifested the phenotype and studied the mechanisms responsible for altered bone architecture.Results: In all affected patients, we found biallelic truncating mutations in SFRP4, the gene encoding secreted frizzled-related protein 4, a soluble Wnt inhibitor. Mice deficient in Sfrp4, like persons with Pyle's disease, have increased amounts of trabecular bone and unusually thin cortical bone, as a result of differential regulation of Wnt and bone morphogenetic protein (BMP) signaling in these two bone compartments. Treatment of Sfrp4-deficient mice with a soluble Bmp2 receptor (RAP-661) or with antibodies to sclerostin corrected the cortical-bone defect.Conclusions: Our study showed that Pyle's disease was caused by a deficiency of sFRP4, that cortical-bone and trabecular-bone homeostasis were governed by different mechanisms, and that sFRP4-mediated cross-regulation between Wnt and BMP signaling was critical for achieving proper cortical-bone thickness and stability. (Funded by the Swiss National Foundation and the National Institutes of Health.). [ABSTRACT FROM AUTHOR]

Published
2016
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45. Microarray Analysis Reveals Characteristic Changes of Host Cell Gene Expression in Response to Attenuated Modified Vaccinia Virus Ankara Infection of Human HeLa Cells.

Author

Guerra, Susana, López-Fernández, Luis A., Conde, Raquel, Pascual-Montano, Alberto, Harshman, Keith, and Esteban, Mariano

Subjects
*GENE expression, *VACCINIA, *HELA cells, *IMMUNE response, *GENES, *NATURAL immunity, *VIROLOGY
Abstract

The potential use of the modified vaccinia virus Ankara (MVA) strain as a live recombinant vector to deliver antigens and elicit protective immune responses against infectious diseases demands a comprehensive understanding of the effect of MVA infection on human host gene expression. We used microarrays containing more than 15,000 human cDNAs to identify gene expression changes in human HeLa cell cultures at 2, 6, and 16 h postinfection. Clustering of the 410 differentially regulated genes identified 11 discrete gene clusters with altered expression patterns after MVA infection. Clusters 1 and 2 (accounting for 16.59% [68 of 410] of the genes) contained 68 transcripts showing a robust induction pattern that was maintained during the course of infection. Changes in cellular gene transcription detected by microarrays after MVA infection were confirmed for selected genes by Northern blot analysis and by real-time reverse transcription-PCR. Upregulated transcripts in clusters 1 and 2 included 20 genes implicated in immune responses, including interleukin 1A (IL-1A), IL-6, IL-7, IL-8, and IL-15 genes. MVA infection also stimulated the expression of NF-κB and components of the NF-κB signal transduction pathway, including p50 and TRAF-interacting protein. A marked increase in the expression of histone family members was also induced during MVA infection. Expression of the Wiskott-Aldrich syndrome family members WAS, WASF1, and the small GTP-binding protein RAC-1, which are involved in actin cytoskeleton reorganization, was enhanced after MVA infection. This study demonstrates that MVA infection triggered the induction of groups of genes, some of which may be involved in host resistance and immune modulation during virus infection. [ABSTRACT FROM AUTHOR]

Published
2004
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46. Cellular Gene Expression Survey of Vaccinia Virus Infection of Human HeLa Cells.

Author

Guerra, Susana, López-Fernández, Luis A., Pascual-Montano, Alberto, Muñoz, Manuel, Harshman, Keith, and Esteban, Mariano

Subjects
*POXVIRUSES, *VACCINIA, *GENE expression
Abstract

Vaccinia virus (VV) is a cytocidal virus that causes major changes in host cell machinery shortly after infecting cells. To define the consequences of virus infection on host gene expression, we used microarrays of approximately 15,000 human cDNAs to examine expression levels of mRNAs isolated at 2, 6, and 16 h postinfection from cultures of infected HeLa cells. The majority of profiling changes during W infection corresponded to downregulation of genes at 16 h postinfection. Differentially expressed genes were clustered into seven groups to identify common regulatory pathways, with most of them (90%) belonging to clusters 6 and 7, which represent genes whose expression was repressed after infection. Cluster 1, however, contained 37 transcripts (2.81%) showing a robust pattern of induction that was maintained during the course of infection. Genes in cluster 1 included those for Wiskott-Aldrich syndrome protein (WASP) family member WASF1, thymosine, adenosine A2a receptor, glutamate decarboxylase 2, CD-80 antigen, KIAA0888 protein, selenophosphate synthetase, pericentrin, and attractin as well as several expressed sequence tags. We analyzed in more detail the fate of WASP protein in VV-infected cells, because a related family member, N-WASP, is involved in viral motility. WASP protein accumulated in the course of infection; its increase required viral DNA replication and de novo protein synthesis, and it localized in cytoplasmic structures distinct from uninfected cells. This study is the first quantitative analysis of host gene expression following W infection of cultured human cells, demonstrating global changes in the expression profile, and identifies upregulated genes with potential roles in the virus replication cycle. [ABSTRACT FROM AUTHOR]

Published
2003
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47. External Quality Assessment of SARS-CoV-2 Sequencing: an ESGMD-SSM Pilot Trial across 15 European Laboratories.

Author

Wegner F, Roloff T, Huber M, Cordey S, Ramette A, Gerth Y, Bertelli C, Stange M, Seth-Smith HMB, Mari A, Leuzinger K, Cerutti L, Harshman K, Xenarios I, Le Mercier P, Bittel P, Neuenschwander S, Opota O, Fuchs J, Panning M, Michel C, Hallin M, Demuyser T, De Mendonca R, Savelkoul P, Dingemans J, van der Veer B, Boers SA, Claas ECJ, Coolen JPM, Melchers WJG, Gunell M, Kallonen T, Vuorinen T, Hakanen AJ, Bernhoff E, Hetland MAK, Golan Berman H, Adar S, Moran-Gilad J, Wolf DG, Leib SL, Nolte O, Kaiser L, Schmutz S, Kufner V, Zaheri M, Trkola A, Aamot HV, Hirsch HH, Greub G, and Egli A

Subjects
Humans, Laboratories, Laboratories, Clinical, Pilot Projects, COVID-19, SARS-CoV-2
Abstract

This first pilot trial on external quality assessment (EQA) of severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) whole-genome sequencing, initiated by the European Society of Clinical Microbiology and Infectious Diseases (ESCMID) Study Group for Genomic and Molecular Diagnostics (ESGMD) and the Swiss Society for Microbiology (SSM), aims to build a framework between laboratories in order to improve pathogen surveillance sequencing. Ten samples with various viral loads were sent out to 15 clinical laboratories that had free choice of sequencing methods and bioinformatic analyses. The key aspects on which the individual centers were compared were the identification of (i) single nucleotide polymorphisms (SNPs) and indels, (ii) Pango lineages, and (iii) clusters between samples. The participating laboratories used a wide array of methods and analysis pipelines. Most were able to generate whole genomes for all samples. Genomes were sequenced to various depths (up to a 100-fold difference across centers). There was a very good consensus regarding the majority of reporting criteria, but there were a few discrepancies in lineage and cluster assignments. Additionally, there were inconsistencies in variant calling. The main reasons for discrepancies were missing data, bioinformatic choices, and interpretation of data. The pilot EQA was overall a success. It was able to show the high quality of participating laboratories and provide valuable feedback in cases where problems occurred, thereby improving the sequencing setup of laboratories. A larger follow-up EQA should, however, improve on defining the variables and format of the report. Additionally, contamination and/or minority variants should be a further aspect of assessment.

Published
2022
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48. Corrigendum: NANS-mediated synthesis of sialic acid is required for brain and skeletal development.

Author

van Karnebeek CDM, Bonafé L, Wen XY, Tarailo-Graovac M, Balzano S, Royer-Bertrand B, Ashikov A, Garavelli L, Mammi I, Turolla L, Breen C, Donnai D, Cormier V, Heron D, Nishimura G, Uchikawa S, Campos-Xavier B, Rossi A, Hennet T, Brand-Arzamendi K, Rozmus J, Harshman K, Stevenson BJ, Girardi E, Superti-Furga G, Dewan T, Collingridge A, Halparin J, Ross CJ, Van Allen MI, Rossi A, Engelke UF, Kluijtmans LAJ, van der Heeft E, Renkema H, de Brouwer A, Huijben K, Zijlstra F, Heisse T, Boltje T, Wasserman WW, Rivolta C, Unger S, Lefeber DJ, Wevers RA, and Superti-Furga A

Published
2017
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49. Identification and molecular characterisation of Lausanne Institutional Biobank participants with familial hypercholesterolaemia - a proof-of-concept study.

Author

Maurer F, Pradervand S, Guilleret I, Nanchen D, Maghraoui A, Chapatte L, Bojkowska K, Bhuiyan ZA, Jacquemont N, Harshman K, and Mooser V

Subjects
Adolescent, Adult, Biological Specimen Banks, Cholesterol blood, Cholesterol, LDL blood, Coronary Artery Disease epidemiology, Female, Humans, Hyperlipoproteinemia Type II blood, Male, Medical Records, Middle Aged, Mutation genetics, Polymerase Chain Reaction, Switzerland epidemiology, Young Adult, Apolipoproteins B genetics, Hyperlipoproteinemia Type II genetics, Proprotein Convertase 9 genetics, Receptors, LDL genetics
Abstract

Aims: We aimed to identify familial hypercholesterolaemia mutation carriers among participants to the Lausanne Institutional Biobank (BIL). Our experimental workflow was designed as a proof-of-concept demonstration of the resources and services provided by our integrated institutional clinical research support platform., Methods: Familial hypercholesterolaemia was used as a model of a relatively common yet often underdiagnosed and inadequately treated Mendelian disease. Clinical and laboratory information was extracted from electronic hospital records. Patients were selected using elevated plasma cholesterol levels (total cholesterol ≥7.5 mM or low-density lipoprotein cholesterol ≥5 mM), premature coronary artery disease status and age (18-60 yr) as main inclusion criteria. LDLR, APOB and PCSK9 were analysed by high-throughput DNA sequencing. The most relevant mutations were confirmed by Sanger sequencing., Results: Of 23 737 patients contacted by the BIL, 17 760 individuals consented to participate and 13 094 wished to be recontacted if there were findings requiring clinical action. Plasma cholesterol records were available for 5111 participants, of whom 94 were selected for genetic screening. Twenty-five of the tested patients presented with premature coronary artery disease while 69 had no such diagnosis. Seven heterozygous carriers of eight rare coding missense variants were identified. Three mutations were pathogenic (APOB p.R3527Q) or likely pathogenic (LDLR p.C27W, LDLR p.P526S) for hypercholesterolaemia, while the others were either benign or of unknown significance. One patient was a double heterozygote for variants APOB p.R3527Q and LDLR p.P526S., Conclusion: This work illustrates how clinical and translational research can benefit from a dedicated platform integrating both a hospital-based biobank and a data support team.

Published
2016
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50. NANS-mediated synthesis of sialic acid is required for brain and skeletal development.

Author

van Karnebeek CD, Bonafé L, Wen XY, Tarailo-Graovac M, Balzano S, Royer-Bertrand B, Ashikov A, Garavelli L, Mammi I, Turolla L, Breen C, Donnai D, Cormier-Daire V, Heron D, Nishimura G, Uchikawa S, Campos-Xavier B, Rossi A, Hennet T, Brand-Arzamendi K, Rozmus J, Harshman K, Stevenson BJ, Girardi E, Superti-Furga G, Dewan T, Collingridge A, Halparin J, Ross CJ, Van Allen MI, Rossi A, Engelke UF, Kluijtmans LA, van der Heeft E, Renkema H, de Brouwer A, Huijben K, Zijlstra F, Heise T, Boltje T, Wasserman WW, Rivolta C, Unger S, Lefeber DJ, Wevers RA, and Superti-Furga A

Subjects
Adult, Age of Onset, Animals, Bone Diseases, Developmental genetics, Bone Diseases, Developmental metabolism, Brain metabolism, Brain pathology, Child, Preschool, Developmental Disabilities genetics, Developmental Disabilities metabolism, Embryo, Nonmammalian metabolism, Embryo, Nonmammalian pathology, Female, Fibroblasts metabolism, Fibroblasts pathology, Humans, Infant, Infant, Newborn, Male, Metabolism, Inborn Errors genetics, Metabolism, Inborn Errors metabolism, Metabolism, Inborn Errors pathology, Zebrafish genetics, Zebrafish metabolism, Bone Diseases, Developmental pathology, Brain embryology, Developmental Disabilities pathology, Mutation genetics, Oxo-Acid-Lyases genetics, Sialic Acids metabolism, Zebrafish embryology
Abstract

We identified biallelic mutations in NANS, the gene encoding the synthase for N-acetylneuraminic acid (NeuNAc; sialic acid), in nine individuals with infantile-onset severe developmental delay and skeletal dysplasia. Patient body fluids showed an elevation in N-acetyl-D-mannosamine levels, and patient-derived fibroblasts had reduced NANS activity and were unable to incorporate sialic acid precursors into sialylated glycoproteins. Knockdown of nansa in zebrafish embryos resulted in abnormal skeletal development, and exogenously added sialic acid partially rescued the skeletal phenotype. Thus, NANS-mediated synthesis of sialic acid is required for early brain development and skeletal growth. Normal sialylation of plasma proteins was observed in spite of NANS deficiency. Exploration of endogenous synthesis, nutritional absorption, and rescue pathways for sialic acid in different tissues and developmental phases is warranted to design therapeutic strategies to counteract NANS deficiency and to shed light on sialic acid metabolism and its implications for human nutrition.

Published
2016
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