Advanced microscopy methods allow obtaining information on (dynamic) conformational changes in bi... more Advanced microscopy methods allow obtaining information on (dynamic) conformational changes in biomolecules via measuring a single molecular distance in the structure. It is, however, extremely challenging to capture the full depth of a three-dimensional biochemical state, binding-related structural changes or conformational cross-talk in multi-protein complexes using one-dimensional assays. In this paper we address this fundamental problem by extending the standard molecular ruler based on Förster resonance energy transfer (FRET) into a two-dimensional assay via its combination with protein-induced fluorescence enhancement (PIFE). We show that donor brightness (via PIFE) and energy transfer efficiency (via FRET) can simultaneously report on e.g., the conformational state of double stranded DNA (dsDNA) following its interaction with unlabelled proteins (BamHI, EcoRV, and T7 DNA polymerase gp5/trx). The PIFE-FRET assay uses established labelling protocols and single molecule fluorescence detection schemes (alternating-laser excitation, ALEX). Besides quantitative studies of PIFE and FRET ruler characteristics, we outline possible applications of ALEX-based PIFE-FRET for single-molecule studies with diffusing and immobilized molecules. Finally, we study transcription initiation and scrunching of E. coli RNA-polymerase with PIFE-FRET and provide direct evidence for the physical presence and vicinity of the polymerase that causes structural changes and scrunching of the transcriptional DNA bubble. Advanced microscopy methods have become powerful tools for structural studies of biomolecules. These methods can complement classical biochemical and biophysical techniques 1,2 , but most importantly emerged as key player in understanding structural dynamics 3,4. The underlying biophysical concept is straight forward: Construct a one-dimensional molecular ruler, in which the biochemical state of the system can be read out as a distance-related measure. Such a molecular ruler often uses a photophysical property such as fluorophore brightness or fluorescence lifetime to provide information on the structure of biomolecules in real time 5. A classic example for such a molecular ruler is Förster-type resonance energy transfer (FRET) 5 , which allows achieving structural information with a spatial resolution in the nanometre range and (sub)millisecond temporal resolution 6–10. However, other photophysical effects such as photo-induced electron transfer (PET) 11–14 or protein-induced fluorescence enhancement (PIFE) 15–32 can be used for similar purposes. Since the fluorescent signal can be read out with high time-resolution, even fast conformational changes 33–39 , as well as interactions between biomolecules, can be mapped in physiologically relevant environments in vitro 40,41 and in vivo 42,43 with a sensitivity allowing to address individual molecules. These molecular rulers suffer from limitations such as their restricted distance ranges and the need for labelling with fluorescent dyes. Most importantly, in the assessment of a three-dimensional (dynamic) structure, the largest limitation is embedded in the information accessible to these methods, which at best follow a single distance to capture a complex structural state.
Single-molecule, protein-induced fluorescence enhancement (PIFE) serves as a molecular ruler at m... more Single-molecule, protein-induced fluorescence enhancement (PIFE) serves as a molecular ruler at molecular distances inaccessible to other spectroscopic rulers such as Förster-type resonance energy transfer (FRET) or photoinduced electron transfer. In order to provide two simultaneous measurements of two distances on different molecular length scales for the analysis of macromolecular complexes, we and others recently combined measurements of PIFE and FRET (PIFE-FRET) on the single molecule level. PIFE relies on steric hindrance of the fluorophore Cy3, which is covalently attached to a biomolecule of interest, to rotate out of an excited-state trans isomer to the cis isomer through a 90° intermediate. In this work, we provide a theoretical framework that accounts for relevant photophysical and kinetic parameters of PIFE-FRET, show how this framework allows the extraction of the fold-decrease in isomerization mobility from experimental data, and show how these results provide information on changes in the accessible volume of Cy3. The utility of this model is then demonstrated for experimental results on PIFE-FRET measurement of different protein–DNA interactions. The proposed model and extracted parameters could serve as a benchmark to allow quantitative comparison of PIFE effects in different biological systems.
Advanced microscopy methods allow obtaining information on (dynamic) conformational changes in bi... more Advanced microscopy methods allow obtaining information on (dynamic) conformational changes in biomolecules via measuring a single molecular distance in the structure. It is, however, extremely challenging to capture the full depth of a three-dimensional biochemical state, binding-related structural changes or conformational cross-talk in multi-protein complexes using one-dimensional assays. In this paper we address this fundamental problem by extending the standard molecular ruler based on Förster resonance energy transfer (FRET) into a two-dimensional assay via its combination with protein-induced fluorescence enhancement (PIFE). We show that donor brightness (via PIFE) and energy transfer efficiency (via FRET) can simultaneously report on e.g., the conformational state of double stranded DNA (dsDNA) following its interaction with unlabelled proteins (BamHI, EcoRV, and T7 DNA polymerase gp5/trx). The PIFE-FRET assay uses established labelling protocols and single molecule fluorescence detection schemes (alternating-laser excitation, ALEX). Besides quantitative studies of PIFE and FRET ruler characteristics, we outline possible applications of ALEX-based PIFE-FRET for single-molecule studies with diffusing and immobilized molecules. Finally, we study transcription initiation and scrunching of E. coli RNA-polymerase with PIFE-FRET and provide direct evidence for the physical presence and vicinity of the polymerase that causes structural changes and scrunching of the transcriptional DNA bubble. Advanced microscopy methods have become powerful tools for structural studies of biomolecules. These methods can complement classical biochemical and biophysical techniques 1,2 , but most importantly emerged as key player in understanding structural dynamics 3,4. The underlying biophysical concept is straight forward: Construct a one-dimensional molecular ruler, in which the biochemical state of the system can be read out as a distance-related measure. Such a molecular ruler often uses a photophysical property such as fluorophore brightness or fluorescence lifetime to provide information on the structure of biomolecules in real time 5. A classic example for such a molecular ruler is Förster-type resonance energy transfer (FRET) 5 , which allows achieving structural information with a spatial resolution in the nanometre range and (sub)millisecond temporal resolution 6–10. However, other photophysical effects such as photo-induced electron transfer (PET) 11–14 or protein-induced fluorescence enhancement (PIFE) 15–32 can be used for similar purposes. Since the fluorescent signal can be read out with high time-resolution, even fast conformational changes 33–39 , as well as interactions between biomolecules, can be mapped in physiologically relevant environments in vitro 40,41 and in vivo 42,43 with a sensitivity allowing to address individual molecules. These molecular rulers suffer from limitations such as their restricted distance ranges and the need for labelling with fluorescent dyes. Most importantly, in the assessment of a three-dimensional (dynamic) structure, the largest limitation is embedded in the information accessible to these methods, which at best follow a single distance to capture a complex structural state.
Single-molecule, protein-induced fluorescence enhancement (PIFE) serves as a molecular ruler at m... more Single-molecule, protein-induced fluorescence enhancement (PIFE) serves as a molecular ruler at molecular distances inaccessible to other spectroscopic rulers such as Förster-type resonance energy transfer (FRET) or photoinduced electron transfer. In order to provide two simultaneous measurements of two distances on different molecular length scales for the analysis of macromolecular complexes, we and others recently combined measurements of PIFE and FRET (PIFE-FRET) on the single molecule level. PIFE relies on steric hindrance of the fluorophore Cy3, which is covalently attached to a biomolecule of interest, to rotate out of an excited-state trans isomer to the cis isomer through a 90° intermediate. In this work, we provide a theoretical framework that accounts for relevant photophysical and kinetic parameters of PIFE-FRET, show how this framework allows the extraction of the fold-decrease in isomerization mobility from experimental data, and show how these results provide information on changes in the accessible volume of Cy3. The utility of this model is then demonstrated for experimental results on PIFE-FRET measurement of different protein–DNA interactions. The proposed model and extracted parameters could serve as a benchmark to allow quantitative comparison of PIFE effects in different biological systems.
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Papers by Evelyn Plötz