Your search keyword '"Meurer, Matthias"' showing total 50 results

1. Scalable RT‐LAMP‐based SARS‐CoV‐2 testing for infection surveillance with applications in pandemic preparedness

Author

Lou, Dan, Meurer, Matthias, Ovchinnikova, Svetlana, Burk, Robin, Denzler, Anna, Herbst, Konrad, Papaioannou, Ioannis A, Duan, Yuanqiang, Jacobs, Max L, Witte, Victoria, Ürge, Daniel, Kirrmaier, Daniel, Krogemann, Michelle, Gubicza, Krisztina, Boerner, Kathleen, Bundschuh, Christian, Weidner, Niklas M, Merle, Uta, Knorr, Britta, Welker, Andreas, Denkinger, Claudia M, Schnitzler, Paul, Kräusslich, Hans‐Georg, Dao Thi, Viet Loan, De Allegri, Manuela, Nguyen, Hoa Thi, Deckert, Andreas, Anders, Simon, and Knop, Michael

Published

2023

2. Timer-based proteomic profiling of the ubiquitin-proteasome system reveals a substrate receptor of the GID ubiquitin ligase

Author

Kong, Ka-Yiu Edwin, Fischer, Bernd, Meurer, Matthias, Kats, Ilia, Li, Zhaoyan, Rühle, Frank, Barry, Joseph D., Kirrmaier, Daniel, Chevyreva, Veronika, San Luis, Bryan-Joseph, Costanzo, Michael, Huber, Wolfgang, Andrews, Brenda J., Boone, Charles, Knop, Michael, and Khmelinskii, Anton

Published

2021

3. CRISPR/Cas12a-mediated labeling of MET receptor enables quantitative single-molecule imaging of endogenous protein organization and dynamics

Author

Baldering, Tim N., Karathanasis, Christos, Harwardt, Marie-Lena I.E., Freund, Petra, Meurer, Matthias, Rahm, Johanna V., Knop, Michael, Dietz, Marina S., and Heilemann, Mike

Published

2021

4. Correction: Comparison of Four Active SARS-CoV-2 Surveillance Strategies in Representative Population Sample Points: Two-Factor Factorial Randomized Controlled Trial

Author

Deckert, Andreas, primary, Anders, Simon, additional, Morales, Ivonne, additional, De Allegri, Manuela, additional, Nguyen, Hoa Thi, additional, Souares, Aurélia, additional, McMahon, Shannon, additional, Meurer, Matthias, additional, Burk, Robin, additional, Lou, Dan, additional, Brugnara, Lucia, additional, Sand, Matthias, additional, Koeppel, Lisa, additional, Maier-Hein, Lena, additional, Ross, Tobias, additional, Adler, Tim J, additional, Brenner, Stephan, additional, Dyer, Christopher, additional, Herbst, Konrad, additional, Ovchinnikova, Svetlana, additional, Marx, Michael, additional, Schnitzler, Paul, additional, Knop, Michael, additional, Bärnighausen, Till, additional, and Denkinger, Claudia M, additional

Published

2024

5. Correction: Comparison of Four Active SARS-CoV-2 Surveillance Strategies in Representative Population Sample Points: Two-Factor Factorial Randomized Controlled Trial (Preprint)

Author

Deckert, Andreas, primary, Anders, Simon, additional, Morales, Ivonne, additional, De Allegri, Manuela, additional, Nguyen, Hoa Thi, additional, Souares, Aurélia, additional, McMahon, Shannon, additional, Meurer, Matthias, additional, Burk, Robin, additional, Lou, Dan, additional, Brugnara, Lucia, additional, Sand, Matthias, additional, Koeppel, Lisa, additional, Maier-Hein, Lena, additional, Ross, Tobias, additional, Adler, Tim J, additional, Brenner, Stephan, additional, Dyer, Christopher, additional, Herbst, Konrad, additional, Ovchinnikova, Svetlana, additional, Marx, Michael, additional, Schnitzler, Paul, additional, Knop, Michael, additional, Bärnighausen, Till, additional, and Denkinger, Claudia M, additional

Published

2024

6. Effectiveness and cost-effectiveness of four different strategies for SARS-CoV-2 surveillance in the general population (CoV-Surv Study): a structured summary of a study protocol for a cluster-randomised, two-factorial controlled trial

Author

Deckert, Andreas, Anders, Simon, de Allegri, Manuela, Nguyen, Hoa Thi, Souares, Aurélia, McMahon, Shannon, Boerner, Kathleen, Meurer, Matthias, Herbst, Konrad, Sand, Matthias, Koeppel, Lisa, Siems, Tobias, Brugnara, Lucia, Brenner, Stephan, Burk, Robin, Lou, Dan, Kirrmaier, Daniel, Duan, Yuanqiang, Ovchinnikova, Svetlana, Marx, Michael, Kräusslich, Hans Georg, Knop, Michael, Bärnighausen, Till, and Denkinger, Claudia

Published

2021

7. Effectiveness and cost-effectiveness of four different strategies for SARS-CoV-2 surveillance in the general population (CoV-Surv Study): study protocol for a two-factorial randomized controlled multi-arm trial with cluster sampling

Author

Deckert, Andreas, Anders, Simon, De Allegri, Manuela, Nguyen, Hoa Thi, Souares, Aurélia, McMahon, Shannon, Meurer, Matthias, Burk, Robin, Sand, Matthias, Koeppel, Lisa, Hein, Lena Maier, Roß, Tobias, Adler, Tim, Siems, Tobias, Brugnara, Lucia, Brenner, Stephan, Herbst, Konrad, Kirrmaier, Daniel, Duan, Yuanqiang, Ovchinnikova, Svetlana, Boerner, Kathleen, Marx, Michael, Kräusslich, Hans-Georg, Knop, Michael, Bärnighausen, Till, and Denkinger, Claudia

Published

2021

8. Accurate and Sensitive Proteome-Scale Mapping of Protein Interactions Using a Quantitative Protein-Fragment Complementation Assay

Author

Lazarewicz, Natalia, primary, Le Dez, Gaëlle, additional, Cerjani, Romina, additional, Runeshaw, Lunelys, additional, Meurer, Matthias, additional, Knop, Michael, additional, Wysocki, Robert, additional, and Rabut, Gwenael, additional

Published

2024

9. Proteome-wide tagging with an H 2 O 2 biosensor reveals highly localized and dynamic redox microenvironments

Author

Kritsiligkou, Paraskevi, primary, Bosch, Katharina, additional, Shen, Tzu Keng, additional, Meurer, Matthias, additional, Knop, Michael, additional, and Dick, Tobias P., additional

Published

2023

10. Alterations in cellular metabolism triggered by URA7 or GLN3 inactivation cause imbalanced dNTP pools and increased mutagenesis

Author

Schmidt, Tobias T., Reyes, Gloria, Gries, Kerstin, Ceylan, Cemile Ümran, Sharma, Sushma, Meurer, Matthias, Knop, Michael, Chabes, Andrei, and Hombauer, Hans

Published

2017

11. Protein Abundance Control by Non-coding Antisense Transcription

Author

Huber, Florian, Bunina, Daria, Gupta, Ishaan, Khmelinskii, Anton, Meurer, Matthias, Theer, Patrick, Steinmetz, Lars M., and Knop, Michael

Published

2016

12. Pooled clone collections by multiplexed CRISPR-Cas12a-assisted gene tagging in yeast

Author

Buchmuller, Benjamin C., Herbst, Konrad, Meurer, Matthias, Kirrmaier, Daniel, Sass, Ehud, Levy, Emmanuel D., and Knop, Michael

Published

2019

13. Proteome-wide tagging with an H2O2 biosensor reveals highly localized and dynamic redox microenvironments.

Author

Kritsiligkou, Paraskevi, Bosch, Katharina, Tzu Keng Shen, Meurer, Matthias, Knop, Michael, and Dick, Tobias P.

Subjects

BIOSENSORS, OXIDATION-reduction reaction, HYDROGEN peroxide

Abstract

Hydrogen peroxide (H2O2) sensing and signaling involves the reversible oxidation of particular thiols on particular proteins to modulate protein function in a dynamic manner. H2O2 can be generated from various intracellular sources, but their identities and relative contributions are often unknown. To identify endogenous "hotspots" of H2O2 generation on the scale of individual proteins and protein complexes, we generated a yeast library in which the H2O2 sensor HyPer7 was fused to the C-terminus of all protein-coding open reading frames (ORFs). We also generated a control library in which a redox-insensitive mutant of HyPer7 (SypHer7) was fused to all ORFs. Both libraries were screened side-by-side to identify proteins located within H2O2-generating environments. Screening under a variety of different metabolic conditions revealed dynamic changes in H2O2 availability highly specific to individual proteins and protein complexes. These findings suggest that intracellular H2O2 generation is much more localized and functionally differentiated than previously recognized. [ABSTRACT FROM AUTHOR]

Published

2023

14. Genome-wide C-SWAT library for high-throughput yeast genome tagging

Author

Meurer, Matthias, Duan, Yuanqiang, Sass, Ehud, Kats, Ilia, Herbst, Konrad, Buchmuller, Benjamin C., Dederer, Verena, Huber, Florian, Kirrmaier, Daniel, Štefl, Martin, Van Laer, Koen, Dick, Tobias P., Lemberg, Marius K., Khmelinskii, Anton, Levy, Emmanuel D., and Knop, Michael

Published

2018

15. Comparison of Four Active SARS-CoV-2 Surveillance Strategies in Representative Population Sample Points: Two-Factor Factorial Randomized Controlled Trial (Preprint)

Author

Deckert, Andreas, primary, Anders, Simon, additional, Morales, Ivonne, additional, De Allegri, Manuela, additional, Nguyen, Hoa Thi, additional, Souares, Aurélia, additional, McMahon, Shannon, additional, Meurer, Matthias, additional, Burk, Robin, additional, Lou, Dan, additional, Brugnara, Lucia, additional, Sand, Matthias, additional, Koeppel, Lisa, additional, Maier-Hein, Lena, additional, Ross, Tobias, additional, Adler, Tim J, additional, Brenner, Stephan, additional, Dyer, Christopher, additional, Herbst, Konrad, additional, Ovchinnikova, Svetlana, additional, Marx, Michael, additional, Schnitzler, Paul, additional, Knop, Michael, additional, Bärnighausen, Till, additional, and Denkinger, Claudia M, additional

Published

2022

16. Two-factor factorial randomized multi-arm parallel controlled trial of four SARS-CoV-2 surveillance strategies in representative population sample points (Preprint)

Author

Deckert, Andreas, primary, Anders, Simon, additional, Morales, Ivonne, additional, De Allegrie, Manuela, additional, Nguyen, Hoa Thi, additional, Souares, Aurélia, additional, McMahon, Shannon, additional, Meurer, Matthias, additional, Burk, Robin, additional, Lou, Dan, additional, Brugnara, Lucia, additional, Sand, Matthias, additional, Koeppel, Lisa, additional, Maier-Hein, Lena, additional, Roß, Tobias, additional, Adler, Tim, additional, Brenner, Stephan, additional, Dyer, Christopher, additional, Herbst, Konrad, additional, Ovchinnikova, Svetlana, additional, Marx, Michael, additional, Schnitzler, Paul, additional, Knop, Michael, additional, Bärnighausen, Till, additional, and Denkinger, Claudia M., additional

Published

2022

17. Scalable RT-LAMP-based SARS-CoV-2 testing for infection surveillance with applications in pandemic control

Author

Lou, Dan, primary, Meurer, Matthias, additional, Ovchinnikova, Svetlana, additional, Burk, Robin, additional, Denzler, Anna, additional, Herbst, Konrad, additional, Papaioannou, Ioannis A., additional, Duan, Yuanqiang, additional, Jacobs, Max L., additional, Witte, Victoria, additional, Uerge, Daniel, additional, Kirrmaier, Daniel, additional, Krogemann, Michelle, additional, Gubicza, Krisztina, additional, Boerner, Kathleen, additional, Bundschuh, Christian, additional, Weidner, Niklas M., additional, Merle, Uta, additional, Knorr, Britta, additional, Welker, Andreas, additional, Denkinger, Claudia M., additional, Schnitzler, Paul, additional, Kraeusslich, Hans-Georg, additional, Thi, Viet Loan Dao, additional, Deckert, Andreas, additional, Anders, Simon, additional, and Knop, Michael, additional

Published

2022

18. Protein quality control at the inner nuclear membrane

Author

Khmelinskii, Anton, Blaszczak, Ewa, Pantazopoulou, Marina, Fischer, Bernd, Omnus, Deike J., Le Dez, Gaelle, Brossard, Audrey, Gunnarsson, Alexander, Barry, Joseph D., Meurer, Matthias, Kirrmaier, Daniel, Boone, Charles, Huber, Wolfgang, Rabut, Gwenael, Ljungdahl, Per O., and Knop, Michael

Subjects

Protein research, Membrane proteins -- Research, Nuclear membranes -- Physiological aspects, Environmental issues, Science and technology, Zoology and wildlife conservation

Abstract

Author(s): Anton Khmelinskii [1]; Ewa Blaszczak [2, 3]; Marina Pantazopoulou [4]; Bernd Fischer [5, 6]; Deike J. Omnus [4]; Gaelle Le Dez [2, 3]; Audrey Brossard [2, 3]; Alexander Gunnarsson [...]

Published

2014

19. Quantification of cytosolic interactions identifies Ede1 oligomers as key organizers of endocytosis

Author

Boeke, Dominik, Trautmann, Susanne, Meurer, Matthias, Wachsmuth, Malte, Godlee, Camilla, Knop, Michael, and Kaksonen, Marko

Published

2014

20. Colorimetric RT-LAMP and LAMP-sequencing for Detecting SARS-CoV-2 RNA in Clinical Samples

Author

Herbst, Konrad, primary, Meurer, Matthias, additional, Kirrmaier, Daniel, additional, Anders, Simon, additional, Knop, Michael, additional, and Dao Thi, Loan, additional

Published

2021

21. A colorimetric RT-LAMP assay and LAMP-sequencing for detecting SARS-CoV-2 RNA in clinical samples

Author

Dao Thi, Viet Loan, primary, Herbst, Konrad, additional, Boerner, Kathleen, additional, Meurer, Matthias, additional, Kremer, Lukas PM, additional, Kirrmaier, Daniel, additional, Freistaedter, Andrew, additional, Papagiannidis, Dimitrios, additional, Galmozzi, Carla, additional, Stanifer, Megan L., additional, Boulant, Steeve, additional, Klein, Steffen, additional, Chlanda, Petr, additional, Khalid, Dina, additional, Barreto Miranda, Isabel, additional, Schnitzler, Paul, additional, Kräusslich, Hans-Georg, additional, Knop, Michael, additional, and Anders, Simon, additional

Published

2020

22. SARS-CoV-2 RNA Extraction Using Magnetic Beads for Rapid Large-Scale Testing by RT-qPCR and RT-LAMP

Author

Klein, Steffen, primary, Müller, Thorsten G., additional, Khalid, Dina, additional, Sonntag-Buck, Vera, additional, Heuser, Anke-Mareil, additional, Glass, Bärbel, additional, Meurer, Matthias, additional, Morales, Ivonne, additional, Schillak, Angelika, additional, Freistaedter, Andrew, additional, Ambiel, Ina, additional, Winter, Sophie L., additional, Zimmermann, Liv, additional, Naumoska, Tamara, additional, Bubeck, Felix, additional, Kirrmaier, Daniel, additional, Ullrich, Stephanie, additional, Barreto Miranda, Isabel, additional, Anders, Simon, additional, Grimm, Dirk, additional, Schnitzler, Paul, additional, Knop, Michael, additional, Kräusslich, Hans-Georg, additional, Dao Thi, Viet Loan, additional, Börner, Kathleen, additional, and Chlanda, Petr, additional

Published

2020

23. CRISPR-Cas12a–assisted PCR tagging of mammalian genes

Author

Fueller, Julia, primary, Herbst, Konrad, additional, Meurer, Matthias, additional, Gubicza, Krisztina, additional, Kurtulmus, Bahtiyar, additional, Knopf, Julia D., additional, Kirrmaier, Daniel, additional, Buchmuller, Benjamin C., additional, Pereira, Gislene, additional, Lemberg, Marius K., additional, and Knop, Michael, additional

Published

2020

24. Screening for SARS-CoV-2 infections with colorimetric RT-LAMP and LAMP sequencing

Author

Thi, Viet Loan Dao, primary, Herbst, Konrad, additional, Boerner, Kathleen, additional, Meurer, Matthias, additional, Kremer, Lukas PM, additional, Kirrmaier, Daniel, additional, Freistaedter, Andrew, additional, Papagiannidis, Dimitrios, additional, Galmozzi, Carla, additional, Klein, Steffen, additional, Chlanda, Petr, additional, Khalid, Dina, additional, Miranda, Isabel Barreto, additional, Schnitzler, Paul, additional, Kräusslich, Hans-Georg, additional, Knop, Michael, additional, and Anders, Simon, additional

Published

2020

25. CRISPR/Cas12a-mediated labeling of MET receptor enables quantitative single-molecule imaging of endogenous protein organization and dynamics

Author

Baldering, Tim N., Karathanasis, Christos, Harwardt, Marie-Lena, Freund, Petra, Meurer, Matthias, Rahm, Johanna V., Knop, Michael, Dietz, Marina, Heilemann, Mike, Baldering, Tim N., Karathanasis, Christos, Harwardt, Marie-Lena, Freund, Petra, Meurer, Matthias, Rahm, Johanna V., Knop, Michael, Dietz, Marina, and Heilemann, Mike

Abstract

Single-molecule localization microscopy (SMLM) reports on protein organization in cells with near-molecular resolution and in combination with stoichiometric labeling enables protein counting. Fluorescent proteins allow stoichiometric labeling of cellular proteins; however, most methods either lead to overexpression or are complex and time demanding. We introduce CRISPR/Cas12a for simple and efficient tagging of endogenous proteins with a photoactivatable protein for quantitative SMLM and single-particle tracking. We constructed a HEK293T cell line with the receptor tyrosine kinase MET tagged with mEos4b and demonstrate full functionality. We determine the oligomeric state of MET with quantitative SMLM and find a reorganization from monomeric to dimeric MET upon ligand stimulation. In addition, we measured the mobility of single MET receptors in vivo in resting and ligand-treated cells. The combination of CRISPR/Cas12a-assisted endogenous protein labeling and super-resolution microscopy represents a powerful tool for cell biological research with molecular resolution.

Published

2020

26. Accurate and sensitive interactome profiling using a quantitative protein-fragment complementation assay

Author

Lazarewicz, Natalia, Le Dez, Gaëlle, Cerjani, Romina, Runeshaw, Lunelys, Meurer, Matthias, Knop, Michael, Wysocki, Robert, and Rabut, Gwenaël

Abstract

An accurate description of protein-protein interaction (PPI) networks is key to understanding the molecular mechanisms underlying cellular systems. Here, we constructed genome-wide libraries of yeast strains to systematically probe protein-protein interactions using NanoLuc Binary Technology (NanoBiT), a quantitative protein-fragment complementation assay (PCA) based on the NanoLuc luciferase. By investigating an array of well-documented PPIs as well as the interactome of four proteins with varying levels of characterization—including the well-studied nonsense-mediated mRNA decay (NMD) regulator Upf1 and the SCF complex subunits Cdc53 and Met30—we demonstrate that ratiometric NanoBiT measurements enable highly precise and sensitive mapping of PPIs. This work provides a foundation for employing NanoBiT in the assembly of more comprehensive and accurate protein interaction maps as well as in their functional investigation.

Published

2024

27. Pooled clone collections by multiplexed CRISPR-Cas12a-assisted gene tagging in yeast

Author

Buchmuller, Benjamin C., primary, Herbst, Konrad, additional, Meurer, Matthias, additional, Kirrmaier, Daniel, additional, Sass, Ehud, additional, Levy, Emmanuel D., additional, and Knop, Michael, additional

Published

2018

28. CRISPR-Cas12a-assisted PCR tagging of mammalian genes

Author

Fueller, Julia, primary, Herbst, Konrad, additional, Meurer, Matthias, additional, Gubicza, Krisztina, additional, Kurtulmus, Bahtiyar, additional, Knopf, Julia D., additional, Kirrmaier, Daniel, additional, Buchmuller, Benjamin C., additional, Pereira, Gislene, additional, Lemberg, Marius K., additional, and Knop, Michael, additional

Published

2018

29. YeastRGB: comparing the abundance and localization of yeast proteins across cells and libraries

Author

Dubreuil, Benjamin, primary, Sass, Ehud, additional, Nadav, Yotam, additional, Heidenreich, Meta, additional, Georgeson, Joseph M, additional, Weill, Uri, additional, Duan, Yuanqiang, additional, Meurer, Matthias, additional, Schuldiner, Maya, additional, Knop, Michael, additional, and Levy, Emmanuel D, additional

Published

2018

30. Monitoring Protein Dynamics in Protein O-Mannosyltransferase Mutants In Vivo by Tandem Fluorescent Protein Timers

Author

Castells-Ballester, Joan, primary, Zatorska, Ewa, additional, Meurer, Matthias, additional, Neubert, Patrick, additional, Metschies, Anke, additional, Knop, Michael, additional, and Strahl, Sabine, additional

Published

2018

31. A genome-wide resource for high-throughput genomic tagging of yeast ORFs

Author

Meurer, Matthias, primary, Duan, Yuanqiang, additional, Sass, Ehud, additional, Kats, Ilia, additional, Herbst, Konrad, additional, Buchmuller, Benjamin C, additional, Dederer, Verena, additional, Huber, Florian, additional, Kirrmaier, Daniel, additional, Štefl, Martin, additional, Van Laer, Koen, additional, Dick, Tobias P, additional, Lemberg, Marius K, additional, Khmelinskii, Anton, additional, Levy, Emmanuel D, additional, and Knop, Michael, additional

Published

2017

32. Upregulation of SPS100 gene expression by an antisense RNA via a switch of mRNA isoforms with different stabilities

Author

Bunina, Daria, primary, Štefl, Martin, additional, Huber, Florian, additional, Khmelinskii, Anton, additional, Meurer, Matthias, additional, Barry, Joseph D., additional, Kats, Ilia, additional, Kirrmaier, Daniel, additional, Huber, Wolfgang, additional, and Knop, Michael, additional

Published

2017

33. Alterations in cellular metabolism triggered by URA7 or GLN3 inactivation cause imbalanced dNTP pools and increased mutagenesis

Author

Schmidt, Tobias T, Reyes, Gloria, Gries, Kerstin, Ceylan, Cemile Ümran, Sharma, Sushma, Meurer, Matthias, Knop, Michael, Chabes, Andrei, Hombauer, Hans, Schmidt, Tobias T, Reyes, Gloria, Gries, Kerstin, Ceylan, Cemile Ümran, Sharma, Sushma, Meurer, Matthias, Knop, Michael, Chabes, Andrei, and Hombauer, Hans

Abstract

Eukaryotic DNA replication fidelity relies on the concerted action of DNA polymerase nucleotide selectivity, proofreading activity, and DNA mismatch repair (MMR). Nucleotide selectivity and proofreading are affected by the balance and concentration of deoxyribonucleotide (dNTP) pools, which are strictly regulated by ribonucleotide reductase (RNR). Mutations preventing DNA polymerase proofreading activity or MMR function cause mutator phenotypes and consequently increased cancer susceptibility. To identify genes not previously linked to high-fidelity DNA replication, we conducted a genome-wide screen in Saccharomyces cerevisiae using DNA polymerase active-site mutants as a "sensitized mutator background." Among the genes identified in our screen, three metabolism-related genes (GLN3, URA7, and SHM2) have not been previously associated to the suppression of mutations. Loss of either the transcription factor Gln3 or inactivation of the CTP synthetase Ura7 both resulted in the activation of the DNA damage response and imbalanced dNTP pools. Importantly, these dNTP imbalances are strongly mutagenic in genetic backgrounds where DNA polymerase function or MMR activity is partially compromised. Previous reports have shown that dNTP pool imbalances can be caused by mutations altering the allosteric regulation of enzymes involved in dNTP biosynthesis (e.g., RNR or dCMP deaminase). Here, we provide evidence that mutations affecting genes involved in RNR substrate production can cause dNTP imbalances, which cannot be compensated by RNR or other enzymatic activities. Moreover, Gln3 inactivation links nutrient deprivation to increased mutagenesis. Our results suggest that similar genetic interactions could drive mutator phenotypes in cancer cells.

Published

2017

34. The regulatableMAL32promoter inSaccharomyces cerevisiae: characteristics and tools to facilitate its use

Author

Meurer, Matthias, primary, Chevyreva, Veronika, additional, Cerulus, Bram, additional, and Knop, Michael, additional

Published

2016

35. A genome wide screen to identify genes that prevent the accumulation of mutations

Author

Hombauer, Hans Wolfgang, primary, Schmidt, Tobias, additional, Cava, Gloria Ximena Reyes, additional, Ceylan, Umran, additional, Gries, Kerstin, additional, Meurer, Matthias, additional, and Knop, Michael, additional

Published

2016

36. One library to make them all: streamlining the creation of yeast libraries via a SWAp-Tag strategy

Author

Yofe, Ido, primary, Weill, Uri, additional, Meurer, Matthias, additional, Chuartzman, Silvia, additional, Zalckvar, Einat, additional, Goldman, Omer, additional, Ben-Dor, Shifra, additional, Schütze, Conny, additional, Wiedemann, Nils, additional, Knop, Michael, additional, Khmelinskii, Anton, additional, and Schuldiner, Maya, additional

Published

2016

37. YeastRGB: comparing the abundance and localization of yeast proteins across cells and libraries.

Author

Dubreuil, Benjamin, Sass, Ehud, Nadav, Yotam, Heidenreich, Meta, Georgeson, Joseph M, Weill, Uri, Duan, Yuanqiang, Meurer, Matthias, Schuldiner, Maya, Knop, Michael, and Levy, Emmanuel D

Published

2019

38. Incomplete proteasomal degradation of green fluorescent proteins in the context of tandem fluorescent protein timers

Author

Khmelinskii, Anton, primary, Meurer, Matthias, additional, Ho, Chi-Ting, additional, Besenbeck, Birgit, additional, Füller, Julia, additional, Lemberg, Marius K., additional, Bukau, Bernd, additional, Mogk, Axel, additional, and Knop, Michael, additional

Published

2016

39. Incomplete proteasomal degradation of green fluorescent proteins in the context of tandem fluorescent protein timers

Author

Khmelinskii, Anton, primary, Meurer, Matthias, additional, Ho, Chi-Ting, additional, Besenbeck, Birgit, additional, Fueller, Julia, additional, Lemberg, Marius K, additional, Bukau, Bernd, additional, Mogk, Axel, additional, and Knop, Michael, additional

Published

2015

40. Live-cell multiphoton fluorescence correlation spectroscopy with an improved large Stokes shift fluorescent protein

Author

Guan, Yinghua, primary, Meurer, Matthias, additional, Raghavan, Sarada, additional, Rebane, Aleksander, additional, Lindquist, Jake R., additional, Santos, Sofia, additional, Kats, Ilia, additional, Davidson, Michael W., additional, Mazitschek, Ralph, additional, Hughes, Thomas E., additional, Drobizhev, Mikhail, additional, Knop, Michael, additional, and Shah, Jagesh V., additional

Published

2015

41. PCR Duplication: A One-Step Cloning-Free Method to Generate Duplicated Chromosomal Loci and Interference-Free Expression Reporters in Yeast

Author

Huber, Florian, primary, Meurer, Matthias, additional, Bunina, Daria, additional, Kats, Ilia, additional, Maeder, Céline I., additional, Štefl, Martin, additional, Mongis, Cyril, additional, and Knop, Michael, additional

Published

2014

42. Quantification of cytosolic interactions identifiesEde1 oligomers as key organizers of endocytosis

Author

Boeke, Dominik, primary, Trautmann, Susanne, additional, Meurer, Matthias, additional, Wachsmuth, Malte, additional, Godlee, Camilla, additional, Knop, Michael, additional, and Kaksonen, Marko, additional

Published

2014

43. Seamless gene tagging by endonuclease-driven homologous recombination.

Author

Khmelinskii, Anton, Meurer, Matthias, Duishoev, Nurlanbek, Delhomme, Nicolas, Knop, Michael, Khmelinskii, Anton, Meurer, Matthias, Duishoev, Nurlanbek, Delhomme, Nicolas, and Knop, Michael

Abstract

Gene tagging facilitates systematic genomic and proteomic analyses but chromosomal tagging typically disrupts gene regulatory sequences. Here we describe a seamless gene tagging approach that preserves endogenous gene regulation and is potentially applicable in any species with efficient DNA double-strand break repair by homologous recombination. We implement seamless tagging in Saccharomyces cerevisiae and demonstrate its application for protein tagging while preserving simultaneously upstream and downstream gene regulatory elements. Seamless tagging is compatible with high-throughput strain construction using synthetic genetic arrays (SGA), enables functional analysis of transcription antisense to open reading frames and should facilitate systematic and minimally-invasive analysis of gene functions.

Published

2011

44. The regulatable MAL32 promoter in Saccharomyces cerevisiae: characteristics and tools to facilitate its use.

Author

Meurer, Matthias, Chevyreva, Veronika, Cerulus, Bram, and Knop, Michael

Abstract

Here we describe a set of tools to facilitate the use of maltose and the MAL32 promoter for regulated gene expression in yeast, alone or in combination with the GAL1 promoter. Using fluorescent protein reporters we find that under non-inducing conditions the MAL32 promoter exhibits a low basal level of expression, similar to the GAL1 promoter, and that both promoters can be induced independently of each other using the respective sugars, maltose and galactose. While their repression upon glucose addition is immediate and complete, we found that the MAL32 and GAL1 promoters each exhibit distinct induction kinetics. A set of plasmids is available to facilitate the application of the MAL32 promoter for chromosomal modifications using PCR targetting and for plasmid based gene expression. Copyright © 2016 John Wiley & Sons, Ltd. [ABSTRACT FROM AUTHOR]

Published

2017

45. Tandem fluorescent protein timers for in vivo analysis of protein dynamics

Author

Khmelinskii, Anton, primary, Keller, Philipp J, additional, Bartosik, Anna, additional, Meurer, Matthias, additional, Barry, Joseph D, additional, Mardin, Balca R, additional, Kaufmann, Andreas, additional, Trautmann, Susanne, additional, Wachsmuth, Malte, additional, Pereira, Gislene, additional, Huber, Wolfgang, additional, Schiebel, Elmar, additional, and Knop, Michael, additional

Published

2012

46. Seamless Gene Tagging by Endonuclease-Driven Homologous Recombination

Author

Khmelinskii, Anton, primary, Meurer, Matthias, additional, Duishoev, Nurlanbek, additional, Delhomme, Nicolas, additional, and Knop, Michael, additional

Published

2011

47. Artificial tethering to nuclear pores promotes partitioning of extrachromosomal DNA during yeast asymmetric cell division

Author

Khmelinskii, Anton, primary, Meurer, Matthias, additional, Knop, Michael, additional, and Schiebel, Elmar, additional

Published

2011

48. Comparison of Four Active SARS-CoV-2 Surveillance Strategies in Representative Population Sample Points: Two-Factor Factorial Randomized Controlled Trial.

Author

Deckert A, Anders S, Morales I, De Allegri M, Nguyen HT, Souares A, McMahon S, Meurer M, Burk R, Lou D, Brugnara L, Sand M, Koeppel L, Maier-Hein L, Ross T, Adler TJ, Brenner S, Dyer C, Herbst K, Ovchinnikova S, Marx M, Schnitzler P, Knop M, Bärnighausen T, and Denkinger CM

Subjects

Humans, Pandemics prevention & control, Specimen Handling, Laboratories, SARS-CoV-2, COVID-19 epidemiology

Abstract

Background: The COVID-19 pandemic is characterized by rapid increases in infection burden owing to the emergence of new variants with higher transmissibility and immune escape. To date, monitoring the COVID-19 pandemic has mainly relied on passive surveillance, yielding biased epidemiological measures owing to the disproportionate number of undetected asymptomatic cases. Active surveillance could provide accurate estimates of the true prevalence to forecast the evolution of the pandemic, enabling evidence-based decision-making., Objective: This study compared 4 different approaches of active SARS-CoV-2 surveillance focusing on feasibility and epidemiological outcomes., Methods: A 2-factor factorial randomized controlled trial was conducted in 2020 in a German district with 700,000 inhabitants. The epidemiological outcome comprised SARS-CoV-2 prevalence and its precision. The 4 study arms combined 2 factors: individuals versus households and direct testing versus testing conditioned on symptom prescreening. Individuals aged ≥7 years were eligible. Altogether, 27,908 addresses from 51 municipalities were randomly allocated to the arms and 15 consecutive recruitment weekdays. Data collection and logistics were highly digitized, and a website in 5 languages enabled low-barrier registration and tracking of results. Gargle sample collection kits were sent by post. Participants collected a gargle sample at home and mailed it to the laboratory. Samples were analyzed with reverse transcription loop-mediated isothermal amplification (RT-LAMP); positive and weak results were confirmed with real-time reverse transcription-polymerase chain reaction (RT-PCR)., Results: Recruitment was conducted between November 18 and December 11, 2020. The response rates in the 4 arms varied between 34.31% (2340/6821) and 41.17% (2043/4962). The prescreening classified 16.61% (1207/7266) of the patients as COVID-19 symptomatic. Altogether, 4232 persons without prescreening and 7623 participating in the prescreening provided 5351 gargle samples, of which 5319 (99.4%) could be analyzed. This yielded 17 confirmed SARS-CoV-2 infections and a combined prevalence of 0.36% (95% CI 0.14%-0.59%) in the arms without prescreening and 0.05% (95% CI 0.00%-0.108%) in the arms with prescreening (initial contacts only). Specifically, we found a prevalence of 0.31% (95% CI 0.06%-0.58%) for individuals and 0.35% (95% CI 0.09%-0.61%) for households, and lower estimates with prescreening (0.07%, 95% CI 0.0%-0.15% for individuals and 0.02%, 95% CI 0.0%-0.06% for households). Asymptomatic infections occurred in 27% (3/11) of the positive cases with symptom data. The 2 arms without prescreening performed the best regarding effectiveness and accuracy., Conclusions: This study showed that postal mailing of gargle sample kits and returning home-based self-collected liquid gargle samples followed by high-sensitivity RT-LAMP analysis is a feasible way to conduct active SARS-CoV-2 population surveillance without burdening routine diagnostic testing. Efforts to improve participation rates and integration into the public health system may increase the potential to monitor the course of the pandemic., Trial Registration: Deutsches Register Klinischer Studien (DRKS) DRKS00023271; https://tinyurl.com/3xenz68a., International Registered Report Identifier (irrid): RR2-10.1186/s13063-021-05619-5., (©Andreas Deckert, Simon Anders, Ivonne Morales, Manuela De Allegri, Hoa Thi Nguyen, Aurélia Souares, Shannon McMahon, Matthias Meurer, Robin Burk, Dan Lou, Lucia Brugnara, Matthias Sand, Lisa Koeppel, Lena Maier-Hein, Tobias Ross, Tim J Adler, Stephan Brenner, Christopher Dyer, Konrad Herbst, Svetlana Ovchinnikova, Michael Marx, Paul Schnitzler, Michael Knop, Till Bärnighausen, Claudia M Denkinger. Originally published in JMIR Public Health and Surveillance (https://publichealth.jmir.org), 17.08.2023.)

Published

2023

49. Colorimetric RT-LAMP and LAMP-sequencing forDetecting SARS-CoV-2 RNA in Clinical Samples.

Author

Herbst K, Meurer M, Kirrmaier D, Anders S, Knop M, and Thi VLD

Abstract

During pandemics, such as the one caused by SARS-CoV-2 coronavirus, simple methods to rapidly test large numbers of people are needed. As a faster and less resource-demanding alternative to detect viral RNA by conventional qPCR, we used reverse transcription loop-mediated isothermal amplification (RT-LAMP). We previously established colorimetric RT-LAMP assays on both purified and unpurified SARS-CoV-2 clinical specimens and further developed a multiplexed sequencing protocol (LAMP-sequencing) to analyze the outcome of many RT-LAMP reactions at the same time (Dao Thi et al. , 2020). Extending on this work, we hereby provide step-by-step protocols for both RT-LAMP assays and read-outs., Competing Interests: Competing interestsThe authors declare no competing interests., (Copyright © 2021 The Authors; exclusive licensee Bio-protocol LLC.)

Published

2021

50. CRISPR/Cas12a-mediated labeling of MET receptor enables quantitative single-molecule imaging of endogenous protein organization and dynamics.

Author

Baldering TN, Karathanasis C, Harwardt MIE, Freund P, Meurer M, Rahm JV, Knop M, Dietz MS, and Heilemann M

Abstract

Single-molecule localization microscopy (SMLM) reports on protein organization in cells with near-molecular resolution and in combination with stoichiometric labeling enables protein counting. Fluorescent proteins allow stoichiometric labeling of cellular proteins; however, most methods either lead to overexpression or are complex and time demanding. We introduce CRISPR/Cas12a for simple and efficient tagging of endogenous proteins with a photoactivatable protein for quantitative SMLM and single-particle tracking. We constructed a HEK293T cell line with the receptor tyrosine kinase MET tagged with mEos4b and demonstrate full functionality. We determine the oligomeric state of MET with quantitative SMLM and find a reorganization from monomeric to dimeric MET upon ligand stimulation. In addition, we measured the mobility of single MET receptors in vivo in resting and ligand-treated cells. The combination of CRISPR/Cas12a-assisted endogenous protein labeling and super-resolution microscopy represents a powerful tool for cell biological research with molecular resolution., Competing Interests: The authors declare no competing interests., (© 2020 The Author(s).)

Published

2020