Your search keyword '"Phil Holzmeister"' showing total 23 results

1. A Starting Point for Fluorescence-Based Single-Molecule Measurements in Biomolecular Research

Author

Alexander Gust, Adrian Zander, Andreas Gietl, Phil Holzmeister, Sarah Schulz, Birka Lalkens, Philip Tinnefeld, and Dina Grohmann

Subjects

single-molecule fluorescence spectroscopy, fluorescence resonance energy transfer, photophysics, photoprotection, fluorescent dye, dynamic heterogeneity, Organic chemistry, QD241-441

Abstract

Single-molecule fluorescence techniques are ideally suited to provide information about the structure-function-dynamics relationship of a biomolecule as static and dynamic heterogeneity can be easily detected. However, what type of single-molecule fluorescence technique is suited for which kind of biological question and what are the obstacles on the way to a successful single-molecule microscopy experiment? In this review, we provide practical insights into fluorescence-based single-molecule experiments aiming for scientists who wish to take their experiments to the single-molecule level. We especially focus on fluorescence resonance energy transfer (FRET) experiments as these are a widely employed tool for the investigation of biomolecular mechanisms. We will guide the reader through the most critical steps that determine the success and quality of diffusion-based confocal and immobilization-based total internal reflection fluorescence microscopy. We discuss the specific chemical and photophysical requirements that make fluorescent dyes suitable for single-molecule fluorescence experiments. Most importantly, we review recently emerged photoprotection systems as well as passivation and immobilization strategies that enable the observation of fluorescently labeled molecules under biocompatible conditions. Moreover, we discuss how the optical single-molecule toolkit has been extended in recent years to capture the physiological complexity of a cell making it even more relevant for biological research.

Published

2014

2. DNA Origami Seesaws as Comparative Binding Assay

Author

Stephanie S. Simmel, Phil Holzmeister, Hans C. Høiberg, Tim Liedl, Philip Tinnefeld, and Philipp C. Nickels

Subjects

0301 basic medicine, DNA, Single-Stranded, Nanotechnology, 010402 general chemistry, sensors, 01 natural sciences, Biochemistry, Binding, Competitive, 03 medical and health sciences, Nucleic acid thermodynamics, chemistry.chemical_compound, DNA structures, Microscopy, Electron, Transmission, DNA nanotechnology, DNA origami, A-DNA, DNA hybridisation, Molecular Biology, Chemistry, Ligand binding assay, Communication, Organic Chemistry, Force spectroscopy, Nucleic Acid Hybridization, self-assembly, DNA, Ligand (biochemistry), Communications, 0104 chemical sciences, Nanostructures, 030104 developmental biology, Biophysics, Molecular Medicine, Nucleic Acid Conformation

Abstract

The application of commonly used force spectroscopy in biological systems is often limited by the need for an invasive tether connecting the molecules of interest to a bead or cantilever tip. Here we present a DNA origami‐based prototype in a comparative binding assay. It has the advantage of in situ readout without any physical connection to the macroscopic world. The seesaw‐like structure has a lever that is able to move freely relative to its base. Binding partners on each side force the structure into discrete and distinguishable conformations. Model experiments with competing DNA hybridisation reactions yielded a drastic shift towards the conformation with the stronger binding interaction. With reference DNA duplexes of tuneable length on one side, this device can be used to measure ligand interactions in comparative assays.

Published

2016

3. Molecular force spectroscopy with a DNA origami–based nanoscopic force clamp

Author

Philip Tinnefeld, Bettina Wünsch, Philipp C. Nickels, Dina Grohmann, Phil Holzmeister, Wooli Bae, Tim Liedl, and Luisa M. Kneer

Subjects

0301 basic medicine, Magnetic tweezers, DNA, Single-Stranded, 02 engineering and technology, Bending, Article, 03 medical and health sciences, Fluorescence Resonance Energy Transfer, Holliday junction, Nanotechnology, A-DNA, Promoter Regions, Genetic, Nanoscopic scale, DNA, Cruciform, Multidisciplinary, Tension (physics), Chemistry, Force spectroscopy, TATA-Box Binding Protein, 021001 nanoscience & nanotechnology, Single Molecule Imaging, 030104 developmental biology, Förster resonance energy transfer, Gene Expression Regulation, Chemical physics, Biophysics, Stress, Mechanical, 0210 nano-technology, Protein Binding

Abstract

Forces in biological systems are typically investigated at the single-molecule level with atomic force microscopy or optical and magnetic tweezers, but these techniques suffer from limited data throughput and their requirement for a physical connection to the macroscopic world. We introduce a self-assembled nanoscopic force clamp built from DNA that operates autonomously and allows massive parallelization. Single-stranded DNA sections of an origami structure acted as entropic springs and exerted controlled tension in the low piconewton range on a molecular system, whose conformational transitions were monitored by single-molecule Förster resonance energy transfer. We used the conformer switching of a Holliday junction as a benchmark and studied the TATA-binding protein-induced bending of a DNA duplex under tension. The observed suppression of bending above 10 piconewtons provides further evidence of mechanosensitivity in gene regulation.

Published

2016

4. A Starting Point for Fluorescence-Based Single-Molecule Measurements in Biomolecular Research

Author

Birka Lalkens, Philip Tinnefeld, Phil Holzmeister, Dina Grohmann, Andreas Gietl, Sarah Schulz, Adrian Zander, and Alexander Gust

Subjects

fluorescence resonance energy transfer, Pharmaceutical Science, Nanotechnology, Review, Analytical Chemistry, lcsh:QD241-441, single-molecule fluorescence spectroscopy, lcsh:Organic chemistry, Drug Discovery, Microscopy, Molecule, Physical and Theoretical Chemistry, Fluorescent Dyes, photophysics, chemistry.chemical_classification, Total internal reflection fluorescence microscope, Research, Biomolecule, Organic Chemistry, Biocompatible material, Fluorescence, photoprotection, Spectrometry, Fluorescence, Förster resonance energy transfer, chemistry, Chemistry (miscellaneous), Molecular Medicine, fluorescent dye, dynamic heterogeneity

Abstract

Single-molecule fluorescence techniques are ideally suited to provide information about the structure-function-dynamics relationship of a biomolecule as static and dynamic heterogeneity can be easily detected. However, what type of single-molecule fluorescence technique is suited for which kind of biological question and what are the obstacles on the way to a successful single-molecule microscopy experiment? In this review, we provide practical insights into fluorescence-based single-molecule experiments aiming for scientists who wish to take their experiments to the single-molecule level. We especially focus on fluorescence resonance energy transfer (FRET) experiments as these are a widely employed tool for the investigation of biomolecular mechanisms. We will guide the reader through the most critical steps that determine the success and quality of diffusion-based confocal and immobilization-based total internal reflection fluorescence microscopy. We discuss the specific chemical and photophysical requirements that make fluorescent dyes suitable for single-molecule fluorescence experiments. Most importantly, we review recently emerged photoprotection systems as well as passivation and immobilization strategies that enable the observation of fluorescently labeled molecules under biocompatible conditions. Moreover, we discuss how the optical single-molecule toolkit has been extended in recent years to capture the physiological complexity of a cell making it even more relevant for biological research.

Published

2014

5. Zwillingsrekombination als Photostabilisierungsmechanismus für Fluoreszenzfarbstoffe

Author

Philip Tinnefeld, Phil Holzmeister, and Andreas Gietl

Subjects

General Medicine

Abstract

Entgegen der ublichen Annahme aufgrund von Photozerstorungswegen durch hoher angeregte Zustande zeigen wir, dass eine weitere Verbesserung der Photostabilitat mit diffusionsbasierten Photostabilisierungsstrategieren moglich ist. Einzelmolekul-Fluoreszenzspektroskopie offenbart, dass Thiolationen effektiv Triplett-Zustande durch photoinduzierten Elektronentransfer loschen. Dabei entsteht selten ein Radikalanion, sondern der Farbstoff kehrt durch einen nahezu instantan erfolgenden Elektronen-Rucktransfer (Zwillingsrekombination) effizient in den Grundzustand zuruck. Fur gewohnlich verwendete Reduktionmittel wie Ascorbinsaure oder Trolox wird hingegen keine Zwillingsrekombination beobachtet. Der Mechanismus vermeidet die Bildung von Radikalkationen und verbessert die Photostabilitat von Fluorophoren. Wir zeigen, dass eine Kombination aus β-Mercaptoethanol und klassischem reduzierenden und oxidierenden System fur einige Farbstoffe die besten Resultate liefert.

Published

2014

6. Geminate Recombination as a Photoprotection Mechanism for Fluorescent Dyes

Author

Phil Holzmeister, Philip Tinnefeld, and Andreas Gietl

Subjects

Photobleaching, Ultraviolet Rays, Chemistry, Ascorbic Acid, General Chemistry, Photochemistry, Ascorbic acid, Electron transport chain, Fluorescence, Catalysis, Photoinduced electron transfer, Fluorescence spectroscopy, Electron Transport, Electron transfer, Excited state, Sulfhydryl Compounds, Chromans, Oxidation-Reduction, Fluorescent Dyes, Mercaptoethanol

Abstract

Despite common presumption due to fast photodestruction pathways through higher excited states, we show that further improvement of photostability is still achievable with diffusion-limited photoprotection formulas. Single-molecule fluorescence spectroscopy reveals that thiolate ions effectively quench triplet states of dyes by photoinduced electron transfer. Interestingly, this reaction rarely yields a radical anion of the dye, but direct return to the ground state is promoted by an almost instantaneous back electron transfer (geminate recombination). This type of mechanism is not detected for commonly used reductants such as ascorbic acid and trolox. The mechanism avoids the formation of radical cations and improves the photostability of single fluorophores. We find that a combination of β-mercaptoethanol and classical reducing and oxidizing systems yields the best results for several dyes including Atto532 and Alexa568.

Published

2014

7. Choosing dyes for cw-STED nanoscopy using self-assembled nanorulers

Author

Birka Lalkens, Susanne Beater, Phil Holzmeister, Enrico Pibiri, and Philip Tinnefeld

Subjects

Materials science, Surface Properties, STED microscopy, General Physics and Astronomy, Nanotechnology, DNA, Microscopy, Atomic Force, Fluorescence, Self assembled, Nanostructures, Embedding Medium, Chemistry, Microscopy, Fluorescence, Microscopy, Fluorescence microscope, DNA origami, A-DNA, Physical and Theoretical Chemistry, Fluorescent Dyes

Abstract

DNA origami used as a platform to study the bleaching behavior of four commonly used fluorophores in cw-STED nanoscopy., Superresolution microscopy is currently revolutionizing optical imaging. A key factor for getting images of highest quality is – besides a well-performing imaging system – the labeling of the sample. We compared the fluorescent dyes Abberior Star 488, Alexa 488, Chromeo 488 and Oregon Green 488 for use in continuous wave (cw-)STED microscopy in aqueous buffer and in a durable polymer matrix. To optimize comparability, we designed DNA origami standards labeled with the fluorescent dyes including a bead-like DNA origami with dyes focused on one spot and a DNA origami with two marks at a designed distance of ∼100 nm. Our data show that all dyes are well suited for cw-STED microscopy but that the optimal dye depends on the embedding medium. The precise comparison enabled by DNA origami nanorulers indicates that these structures have matured from the proof-of-concept to easily applicable tools in fluorescence microscopy.

Published

2014

8. Breaking the concentration limit of optical single-molecule detection

Author

Guillermo P. Acuna, Phil Holzmeister, Philip Tinnefeld, and Dina Grohmann

Subjects

Diffraction, Detection limit, Materials science, business.industry, Sample (material), Design of experiments, Volume (computing), Equipment Design, General Chemistry, Microfluidic Analytical Techniques, Optics, Microscopy, Fluorescence, Models, Chemical, Limit of Detection, Range (statistics), Animals, Humans, Nanotechnology, Molecule, Computer Simulation, Limit (mathematics), Biological system, business, Fluorescent Dyes

Abstract

Over the last decade, single-molecule detection has been successfully utilized in the life sciences and materials science. Yet, single-molecule measurements only yield meaningful results when working in a suitable, narrow concentration range. On the one hand, diffraction limits the minimal size of the observation volume in optical single-molecule measurements and consequently a sample must be adequately diluted so that only one molecule resides within the observation volume. On the other hand, at ultra-low concentrations relevant for sensing, the detection volume has to be increased in order to detect molecules in a reasonable timespan. This in turn results in the loss of an optimal signal-to-noise ratio necessary for single-molecule detection. This review discusses the requirements for effective single-molecule fluorescence applications, reflects on the motivation for the extension of the dynamic concentration range of single-molecule measurements and reviews various approaches that have been introduced recently to solve these issues. For the high-concentration limit, we identify four promising strategies including molecular confinement, optical observation volume reduction, temporal separation of signals and well-conceived experimental designs that specifically circumvent the high concentration limit. The low concentration limit is addressed by increasing the measurement speed, parallelization, signal amplification and preconcentration. The further development of these ideas will expand our possibilities to interrogate research questions with the clarity and precision provided only by the single-molecule approach.

Published

2014

9. Single-molecule FRET supports the two-state model of Argonaute action

Author

Phil Holzmeister, Adrian Zander, Daniel Klose, Dina Grohmann, and Philip Tinnefeld

Subjects

Models, Molecular, Methanocaldococcus, Conformational change, Protein Conformation, chemistry.chemical_compound, Protein structure, Fluorescence Resonance Energy Transfer, A-DNA, Cloning, Molecular, Molecular Biology, Sequence Homology, Amino Acid, biology, DNA, Cell Biology, Single-molecule FRET, Argonaute, biology.organism_classification, Protein Structure, Tertiary, Förster resonance energy transfer, Biochemistry, chemistry, Argonaute Proteins, Biophysics, Protein Binding, Research Paper

Abstract

Argonaute can be found in all three domains of life and is the functional core of the eukaryotic RNA-silencing machinery. In order to shed light on the conformational changes that drive Argonaute action, we performed single-molecule FRET measurements employing a so far uncharacterized member of the Argonaute family, namely Argonaute from the archaeal organism Methanocaldococcus jannaschii (MjAgo). We show that MjAgo is a catalytically active Argonaute variant hydrolyzing exclusively DNA target strands out of a DNA/DNA hybrid. We studied the interplay between Argonaute and nucleic acids using fluorescent dyes covalently attached at different positions of the DNA guide as steric reporters. This allowed us to determine structurally confined parts of the protein scaffold and flexible regions of the DNA guide. Single-molecule FRET measurements demonstrate that the 3′end of the DNA guide is released from the PAZ domain upon target strand loading. This conformational change does not necessitate target strand cleavage but a fully complementary target strand. Thus, our data support the two state model for Argonaute action.

Published

2013

10. Counting Fluorescent Dye Molecules on DNA Origami by Means of Photon Statistics

Author

Jürgen J. Schmied, Kristin S. Grußmayer, Philip Tinnefeld, Anton Kurz, Phil Holzmeister, and Dirk-Peter Herten

Subjects

Microscope, Nanotechnology, 02 engineering and technology, law.invention, Biomaterials, 03 medical and health sciences, law, Microscopy, Fluorescence microscope, DNA origami, General Materials Science, Fluorescent Dyes, 030304 developmental biology, Photons, 0303 health sciences, Photon antibunching, Chemistry, STED microscopy, DNA, General Chemistry, 021001 nanoscience & nanotechnology, Fluorescence, Microscopy, Fluorescence, Temporal resolution, 0210 nano-technology, Biological system, Biotechnology

Abstract

Obtaining quantitative information about molecular assemblies with high spatial and temporal resolution is a challenging task in fluorescence microscopy. Single-molecule techniques build on the ability to count molecules one by one. Here, a method is presented that extends recent approaches to analyze the statistics of coincidently emitted photons to enable reliable counting of molecules in the range of 1-20. This method does not require photochemistry such as blinking or bleaching. DNA origami structures are labeled with up to 36 dye molecules as a new evaluation tool to characterize this counting by a photon statistics approach. Labeled DNA origami has a well-defined labeling stoichiometry and ensures equal brightness for all dyes incorporated. Bias and precision of the estimating algorithm are determined, along with the minimal acquisition time required for robust estimation. Complexes containing up to 18 molecules can be investigated non-invasively within 150 ms. The method might become a quantifying add-on for confocal microscopes and could be especially powerful in combination with STED/RESOLFT-type microscopy.

Published

2013

11. DNA Origami Force Balance

Author

Philipp C. Nickels, Dina Grohmann, Phil Holzmeister, Philipp Tinnefeld, Tim Liedl, and Bettina Wünsch

Subjects

Lever, business.product_category, Tension (physics), Chemistry, Force spectroscopy, Biophysics, Molecular physics, Folding (chemistry), Crystallography, Förster resonance energy transfer, Optical tweezers, Holliday junction, DNA origami, business

Abstract

Commonly used techniques to study conformational changes of interacting macromolecules such as atomic force microscopy and magnetic or optical tweezers today feature spatial resolutions of single nanometers and piconewton force sensitivity [1]. One of the limitations of these methods is the need to couple the molecules under investigation to a cantilever tip or micrometer-sized beads. By constructing molecular force spectroscopy tools with the help of DNA origami [2-4] we are trying to overcome this limitation. Our DNA origami-based force balance comprises a moveable lever on top of a base, which can exert defined forces in the regime between 1 pN and 10 pN between the lever and the base. The position of the lever can be detected with Transmission Electron Microscopy (TEM) and by Fluorescence Resonance Energy Transfer (FRET) in a dynamic fashion. Discrete and geometrically distinguishable conformations of our force balance can be observed when competing hybridizing DNA single-strands occupy their complementary counterparts on the structure on both sides of the lever. In model experiments where we tested different numbers of hybridizing strands on the two opposing ends of the lever, we observed surprisingly uniform populations of structures that were set in the “correct” conformation (∼ 90%).In a next step, we designed variants of the force balance with pre-stressed segments of DNA and investigated the dynamic switching of a Holliday junction under stress. In ongoing experiments we study the tension dependent bending behavior of DNA bending proteins.[1] C. Bustamante et al., Ten years of tension: single-molecule DNA mechanics, Nature (2003).[2] P. Rothemund, Folding DNA to create nanoscale shapes and patterns, Nature (2006).[3] H. Dietz et al., Folding DNA into twisted and curved nanoscale shapes, Nature (2009).[4] T. Liedl et al., Self-assembly of three-dimensional prestressed tensegrity structures from DNA, Nature Nanotechnology (2010).

Published

2016

12. Distance Dependence of Single-Fluorophore Quenching by Gold Nanoparticles Studied on DNA Origami

Author

Philip Tinnefeld, Ingo H. Stein, Guillermo P. Acuna, Tim Liedl, M. Bucher, Anton Kuzyk, Robert D. Schreiber, Friedrich C. Simmel, Fernando D. Stefani, Christian Steinhauer, Phil Holzmeister, and Alexander Moroz

Subjects

Optics and Photonics, Fluorescence-lifetime imaging microscopy, Fluorophore, Materials science, NANOPARTICLE, Metal Nanoparticles, General Physics and Astronomy, Nanoparticle, Nanotechnology, INGENIERÍAS Y TECNOLOGÍAS, 02 engineering and technology, 010402 general chemistry, 7. Clean energy, 01 natural sciences, DNA ORIGAMI, chemistry.chemical_compound, DNA nanotechnology, DNA origami, General Materials Science, Otras Nanotecnología, FLUORESCENCE, Fluorescent Dyes, Nanotecnología, Quenching (fluorescence), business.industry, General Engineering, DNA, 021001 nanoscience & nanotechnology, Single-molecule experiment, Fluorescence, 0104 chemical sciences, PLASMONICS, Spectrometry, Fluorescence, chemistry, Optoelectronics, Gold, 0210 nano-technology, business

Abstract

We study the distance-dependent quenching of fluorescence due to a metallic nanoparticle in proximity of a fluorophore. In our single-molecule measurements, we achieve excellent control over structure and stoichiometry by using self-assembled DNA structures (DNA origami) as a breadboard where both the fluorophore and the 10 nm metallic nanoparticle are positioned with nanometer precision. The single-molecule spectroscopy method employed here reports on the co-localization of particle and dye, while fluorescence lifetime imaging is used to directly obtain the correlation of intensity and fluorescence lifetime for varying particle to dye distances. Our data can be well explained by exact calculations that include dipole dipole orientation and distances. Fitting with a more practical model for nanosurface energy transfer yields 10.4 nm as the characteristic distance of 50% energy transfer. The use of DNA nanotechnology together with minimal sample usage by attaching the particles to the DNA origami directly on the microscope coverslip paves the way for more complex experiments exploiting dye nanoparticle interactions. Fil: Acuna, Guillermo P.. Technische Universität Braunschweig; Alemania Fil: Bucher, Martina. Ludwig Maximilians Universitat; Alemania Fil: Stein, Ingo H.. Ludwig Maximilians Universitat; Alemania Fil: Steinhauer, Christian. Ludwig Maximilians Universitat; Alemania Fil: Kuzyk, Anton. Technische Universitat Munchen; Alemania Fil: Holzmeister, Phil. Technische Universität Braunschweig; Alemania Fil: Schreiber, Robert. Ludwig Maximilians Universitat; Alemania Fil: Moroz, Alexander. Fil: Stefani, Fernando Daniel. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Ciudad Universitaria. Instituto de Física de Buenos Aires. Universidad de Buenos Aires. Facultad de Ciencias Exactas y Naturales. Instituto de Física de Buenos Aires; Argentina Fil: Liedl, Tim. Ludwig Maximilians Universitat; Alemania Fil: Simmel, Friedrich C.. Technische Universitat Munchen; Alemania Fil: Tinnefeld, Philip. Technische Universität Braunschweig; Alemania

Published

2012

13. Quantum yield and excitation rate of single molecules close to metallic nanostructures

Author

Enrico Pibiri, Phil Holzmeister, Philip Tinnefeld, Guillermo P. Acuna, Jürgen J. Schmied, and Tapasi Sen

Subjects

Multidisciplinary, Materials science, Quenching (fluorescence), Metallic nanostructures, General Physics and Astronomy, Quantum yield, Physics::Optics, General Chemistry, Bioinformatics, Fluorescence, General Biochemistry, Genetics and Molecular Biology, Article, Chemical physics, Radiative transfer, Molecule, Metal nanostructures, Excitation

Abstract

The interaction of dyes and metallic nanostructures strongly affects the fluorescence and can lead to significant fluorescence enhancement at plasmonic hot spots, but also to quenching. Here we present a method to distinguish the individual contributions to the changes of the excitation, radiative and non-radiative rate and use this information to determine the quantum yields for single molecules. The method is validated by precisely placing single fluorescent dyes with respect to gold nanoparticles as well as with respect to the excitation polarization using DNA origami nanostructures. Following validation, measurements in zeromode waveguides reveal that suppression of the radiative rate and enhancement of the non-radiative rate lead to a reduced quantum yield. Because the method exploits the intrinsic blinking of dyes, it can generally be applied to fluorescence measurements in arbitrary nanophotonic environments.

Published

2014

14. Single-molecule positioning in zeromode waveguides by DNA origami nanoadapters

Author

Enrico Pibiri, Birka Lalkens, Philip Tinnefeld, Phil Holzmeister, and Guillermo P. Acuna

Subjects

Nanostructure, Materials science, biology, Mechanical Engineering, Nanophotonics, Bioengineering, Nanotechnology, General Chemistry, DNA, Sequence Analysis, DNA, Condensed Matter Physics, Nanostructures, chemistry.chemical_compound, chemistry, biology.protein, DNA origami, Surface modification, Molecule, General Materials Science, Polymerase

Abstract

Nanotechnology is challenged by the need to connect top-down produced nanostructures with the bottom-up world of chemistry. A nanobiotechnological prime example is the positioning of single polymerase molecules in small holes in metal films, so-called zeromode waveguides (ZMWs), which is required for single-molecule real-time DNA sequencing. In this work, we present nanoadapters made of DNA (DNA origami) that match the size of the holes so that exactly one nanoadapter fits in each hole. By site-selective functionalization of the DNA origami nanoadapters, we placed single dye molecules in the ZMWs, thus optimizing the hole usage and improving the photophysical properties of dyes compared to stochastically immobilized molecules.

Published

2014

15. Controlled reduction of photobleaching in DNA origami gold nanoparticle hybrids

Author

Phil Holzmeister, Guillermo P. Acuna, Jesica Vanesa Pellegrotti, Fernando D. Stefani, Birka Lalkens, Andreas Gietl, Philip Tinnefeld, and Anastasiya Puchkova

Subjects

DNA SELF-ASSEMBLY, PHOTOBLEACHING, Ciencias Físicas, Metal Nanoparticles, Nanoparticle, Bioengineering, Nanotechnology, Biosensing Techniques, Photochemistry, purl.org/becyt/ford/1 [https], SINGLE MOLECULE, DNA origami, General Materials Science, Emission spectrum, Fluorescence loss in photobleaching, Óptica, Photons, Photobleaching, Chemistry, Mechanical Engineering, DNA, General Chemistry, purl.org/becyt/ford/1.3 [https], Condensed Matter Physics, Fluorescence, PLASMONICS, Colloidal gold, Gold, Biosensor, CIENCIAS NATURALES Y EXACTAS

Abstract

The amount of information obtainable from a fluorescence-based measurement is limited by photobleaching: Irreversible photochemical reactions either render the molecules nonfluorescent or shift their absorption and/or emission spectra outside the working range. Photobleaching is evidenced as a decrease of fluorescence intensity with time, or in the case of single molecule measurements, as an abrupt, single-step interruption of the fluorescence emission that determines the end of the experiment. Reducing photobleaching is central for improving fluorescence (functional) imaging, single molecule tracking, and fluorescence-based biosensors and assays. In this single molecule study, we use DNA self-assembly to produce hybrid nanostructures containing individual fluorophores and gold nanoparticles at a controlled separation distance of 8.5 nm. By changing the nanoparticles? size we are able to systematically increase the mean number of photons emitted by the fluorophores before photobleaching. Fil: Pellegrotti, Jesica Vanesa. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Parque Centenario. Centro de Investigaciones en Bionanociencias "Elizabeth Jares Erijman"; Argentina. Universidad de Buenos Aires. Facultad de Ciencias Exactas y Naturales. Departamento de Física; Argentina Fil: Acuña, Guillermo. Technische Universität Braunschweig. Institute for Physical and Theoretical Chemistry. NanoBioSciences Group; Alemania Fil: Puchkova, Anastasiya. Technische Universität Braunschweig. Institute for Physical and Theoretical Chemistry. NanoBioSciences Group; Alemania Fil: Holzmeister, Phil. Technische Universität Braunschweig. Institute for Physical and Theoretical Chemistry. NanoBioSciences Group; Alemania Fil: Gietl, Andreas. Technische Universität Braunschweig. Institute for Physical and Theoretical Chemistry. NanoBioSciences Group; Alemania Fil: Lalkens, Birka. Technische Universität Braunschweig. Institute for Physical and Theoretical Chemistry. NanoBioSciences Group; Alemania Fil: Stefani, Fernando Daniel. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Parque Centenario. Centro de Investigaciones en Bionanociencias "Elizabeth Jares Erijman"; Argentina. Universidad de Buenos Aires. Facultad de Ciencias Exactas y Naturales. Departamento de Física; Argentina Fil: Tinnefeld, Philip. Technische Universität Braunschweig. Institute for Physical and Theoretical Chemistry. NanoBioSciences Group; Alemania

Published

2014

16. ChemInform Abstract: Breaking the Concentration Limit of Optical Single-Molecule Detection

Author

Phil Holzmeister, Philip Tinnefeld, Dina Grohmann, and Guillermo P. Acuna

Subjects

Diffraction, Materials science, Cut off value, Design of experiments, Sample (material), Volume (computing), Range (statistics), Molecule, General Medicine, Limit (mathematics), Biological system

Abstract

Over the last decade, single-molecule detection has been successfully utilized in the life sciences and materials science. Yet, single-molecule measurements only yield meaningful results when working in a suitable, narrow concentration range. On the one hand, diffraction limits the minimal size of the observation volume in optical single-molecule measurements and consequently a sample must be adequately diluted so that only one molecule resides within the observation volume. On the other hand, at ultra-low concentrations relevant for sensing, the detection volume has to be increased in order to detect molecules in a reasonable timespan. This in turn results in the loss of an optimal signal-to-noise ratio necessary for single-molecule detection. This review discusses the requirements for effective single-molecule fluorescence applications, reflects on the motivation for the extension of the dynamic concentration range of single-molecule measurements and reviews various approaches that have been introduced recently to solve these issues. For the high-concentration limit, we identify four promising strategies including molecular confinement, optical observation volume reduction, temporal separation of signals and well-conceived experimental designs that specifically circumvent the high concentration limit. The low concentration limit is addressed by increasing the measurement speed, parallelization, signal amplification and preconcentration. The further development of these ideas will expand our possibilities to interrogate research questions with the clarity and precision provided only by the single-molecule approach.

Published

2014

17. Single-molecule photophysics of dark quenchers as non-fluorescent FRET acceptors

Author

Andreas Gietl, Bettina Wünsch, Phil Holzmeister, and Philip Tinnefeld

Subjects

Förster resonance energy transfer, Photoactivatable probes, Absorption spectroscopy, Chemistry, Excited state, Dark quencher, Molecule, Physical and Theoretical Chemistry, Chromophore, Photochemistry, Fluorescence

Abstract

Dark quencher chromophores are interesting alternatives to common single-molecule FRET acceptors. Due to their short excited state lifetime, they should be less prone to complex photophysics and bleaching. We find, however, that for common enzymatic oxygen scavenging systems and photoprotection strategies – the gold standard of single-molecule measurements – the quenchers BBQ650 and BHQ-2 induce frequent blinking of the donor molecule. They switch in a photoinduced process to what we identify as a radical anion state and back. We further make use of the broad absorption spectrum for selective bleaching of the quenchers in order to photoactivate the fluorescence of initially completely quenched dye molecules. This represents a general strategy to turn fluorescent dyes into photoactivatable probes.

Published

2013

18. DNA-Templated Nanoantennas for Single-Molecule Detection at Elevated Concentrations

Author

Friederike M. Möller, Philip Tinnefeld, Birka Lalkens, Phil Holzmeister, Guillermo P. Acuna, and Susanne Beater

Subjects

Materials science, Biomedical Engineering, Biotin, Metal Nanoparticles, Nanoparticle, Nanotechnology, 010402 general chemistry, 01 natural sciences, Biomaterials, Metal, 03 medical and health sciences, Image Processing, Computer-Assisted, DNA origami, Molecule, Particle Size, Plasmon, Fluorescent Dyes, 030304 developmental biology, 0303 health sciences, Microscopy, Confocal, business.industry, DNA, Models, Theoretical, Avidin, Single-molecule experiment, Fluorescence, Atomic and Molecular Physics, and Optics, 0104 chemical sciences, Electronic, Optical and Magnetic Materials, Spectrometry, Fluorescence, Microscopy, Fluorescence, Colloidal gold, visual_art, visual_art.visual_art_medium, Optoelectronics, Quantum efficiency, Nanometre, Gold, business, Luminescence, Dimerization

Abstract

The dynamic concentration range is one of the major limitations of single-molecule fluorescence techniques. Here, we show how bottom-up nano-antennas enhance the fluorescence intensity in a reduced hot-spot, ready for biological applications. We use self-assembled DNA origami structures as a breadboard where gold nanoparticle dimers are positioned with nanometer precision. A maximum of almost 100fold intensity enhancement is obtained using 100 nm gold nanoparticles within a gap of 23 nm between the particles. The results obtained are in good agreement with numerical simulations. Due to the intensity enhancement introduced by the nano-antenna, we are able to perform single molecule measurements at concentrations as high as 500 nM which represents an increment of 2 orders of magnitude compared to conventional measurements. The combination of metallic nanoparticles with DNA origami structures with docking points for biological assays paves the way for the development of bottom-up inexpensive enhancement chambers for single molecule measurements at high concentrations where processes like DNA sequencing occur.

Published

2013

19. Cover Picture: DNA Origami Seesaws as Comparative Binding Assay (ChemBioChem 12/2016)

Author

Stephanie S. Simmel, Tim Liedl, Hans C. Høiberg, Phil Holzmeister, Philipp C. Nickels, and Philip Tinnefeld

Subjects

Chemistry, Ligand binding assay, Organic Chemistry, Molecular Medicine, DNA origami, Cover (algebra), Nanotechnology, Computational biology, DNA hybridisation, Molecular Biology, Biochemistry

Published

2016

20. Fluorescence enhancement at docking sites of DNA-directed self-assembled nanoantennas

Author

Philip Tinnefeld, Susanne Beater, Friederike M. Möller, Phil Holzmeister, Birka Lalkens, and Guillermo P. Acuna

Subjects

Materials science, Metal Nanoparticles, Nanotechnology, 02 engineering and technology, 010402 general chemistry, 01 natural sciences, Fluorescence, chemistry.chemical_compound, Holliday junction, DNA origami, A-DNA, Particle Size, Plasmon, Fluorescent Dyes, DNA, Cruciform, Multidisciplinary, DNA, 021001 nanoscience & nanotechnology, Image Enhancement, 0104 chemical sciences, Spectrometry, Fluorescence, chemistry, Docking (molecular), Colloidal gold, Gold, 0210 nano-technology, Dimerization

Abstract

Building a Fluorescent Hotspot When two gold nanoparticles come close together, their overlapping plasmonic fields can create a region that acts as a nanoantenna that can enhance the fluorescent emission of a molecule. Acuna et al. (p. 506 ) used a surface-anchored DNA origami structure to assemble one or two gold nanoparticles next to a dye trapped within the structure. A > 100-fold enhancement in fluorescent emission was observed when the dye molecules were located in a 23-nm gap between two 100-nm gold nanoparticles.

Published

2012

21. Simple and aberration-free 4color-STED - multiplexing by transient binding

Author

Philip Tinnefeld, Phil Holzmeister, Susanne Beater, and Birka Lalkens

Subjects

Physics, Fluorophore, Microscope, Super-resolution microscopy, business.industry, STED microscopy, Atomic and Molecular Physics, and Optics, law.invention, chemistry.chemical_compound, Optics, Complementary sequences, chemistry, Confocal microscopy, law, Microscopy, Fluorescence microscope, business

Abstract

Most fluorescence microscopy experiments today require a multicolor-capable setup, e.g. to study the interaction between different proteins. Multicolor capabilities are also well desirable for superresolution images. However, especially for STED (Stimulated Emission Depletion) microscopy, which requires two laser lines for a single color, multicolor imaging is technically challenging. Here we present a straightforward, easy-to-implement method to extend a single-color fluorescence (STED) microscope to a multichannel microscope without the need of modifying the optical setup. Therefore, we use a labeling technique based on complementary DNA sequences: a single-stranded short DNA sequence is attached to each structure to be imaged, different colors for labeling different features are represented by different sequences. Within the imaging process, the corresponding complementary sequence labeled with an organic fluorophore is added and transiently binds to the corresponding structure. After imaging, the labeled sequence is washed away and replaced by a second fluorescently labeled DNA strand complementary to the sequence bound to another feature. This way, multiplexing is achieved using only one arbitrary fluorophore, therefore aberrations are avoided.

Published

2015

22. Fluorescence and super-resolution standards based on DNA origami

Author

Jürgen J. Schmied, Philip Tinnefeld, Andreas Gietl, Carsten Forthmann, Christian Steinhauer, Thorben Dammeyer, and Phil Holzmeister

Subjects

Materials science, Nanotechnology, DNA, Cell Biology, Biochemistry, Superresolution, Fluorescence, Förster resonance energy transfer, Microscopy, Fluorescence, Oligodeoxyribonucleotides, Calibration, Microscopy, Fluorescence Resonance Energy Transfer, Biophysics, DNA origami, Molecular Biology, Biotechnology

Published

2012

23. DNA origami as biocompatible surface to match single-molecule and ensemble experiments

Author

Philip Tinnefeld, Phil Holzmeister, Andreas Gietl, and Dina Grohmann

Subjects

chemistry.chemical_classification, DNA, Cruciform, Biomolecule, Nanotechnology, DNA, Biology, TATA-Box Binding Protein, Molecular biology, TATA Box, Molecular machine, Nanostructures, chemistry.chemical_compound, Förster resonance energy transfer, chemistry, DNA nanotechnology, Genetics, Holliday junction, Fluorescence Resonance Energy Transfer, DNA origami, Methods Online, Nucleic Acid Conformation, A-DNA

Abstract

Single-molecule experiments on immobilized molecules allow unique insights into the dynamics of molecular machines and enzymes as well as their interactions. The immobilization, however, can invoke perturbation to the activity of biomolecules causing incongruities between single molecule and ensemble measurements. Here we introduce the recently developed DNA origami as a platform to transfer ensemble assays to the immobilized single molecule level without changing the nano-environment of the biomolecules. The idea is a stepwise transfer of common functional assays first to the surface of a DNA origami, which can be checked at the ensemble level, and then to the microscope glass slide for single-molecule inquiry using the DNA origami as a transfer platform. We studied the structural flexibility of a DNA Holliday junction and the TATA-binding protein (TBP)-induced bending of DNA both on freely diffusing molecules and attached to the origami structure by fluorescence resonance energy transfer. This resulted in highly congruent data sets demonstrating that the DNA origami does not influence the functionality of the biomolecule. Single-molecule data collected from surface-immobilized biomolecule-loaded DNA origami are in very good agreement with data from solution measurements supporting the fact that the DNA origami can be used as biocompatible surface in many fluorescence-based measurements.

Published

2012