Origin of fluorescence and voltage sensitivity in microbial rhodopsin-based voltage sensors

QuasArs, eine neue Klasse von fluoreszierenden Membranspannungssensoren basierend auf Archaerhodopsin-3, wurde von Hochbaum et al. im Jahr 2014 beschrieben. Die neuen Konstrukte zeigen eine für mikrobielle Rhodopsine außergewöhnlich hohe Fluoreszenzquantenausbeute. Außerdem ist die Fluoreszenz spannungsabhängig, was für Membranspannungssensoren eine wünschenswerte Eigenschaft ist. Diese Sensoren bieten ein hohes räumliches und zeitliches Auflösungsvermögen, wodurch neuronale Aktivität verfolgt werden könnte. Obwohl mehrere Varianten vorgeschlagen wurden ist ihre Fluoreszenzquantenausbeute immer noch zu gering (<1%) für Anwendungen in lebenden Nagetieren und erfordert weitere Verbesserungen für bildgebende Anwendungen. Das rationale Design der Rhodopsin-basierten Fluoreszenzsensoren der nächsten Generation ist jedoch nur eingeschränkt möglich, da die derzeit verwendeten QuasArs mittels zufälliger Mutagenese gefunden wurden. Um verbesserte Konstrukte zu entwickeln, ist es wichtig die Funktionalität der spannungssensitiven Fluoreszenz und die Rolle der eingeführten Mutationen zu verstehen. In dieser Arbeit wurden die mikrobiellen Rhodopsin-basierten Spannungssensoren und der Ursprung ihrer spannungsmodulierten Fluoreszenz untersucht. Die Photodynamik dieser Spannungssensoren wurde mit UV/Vis-Steady-State und -transienter Spektroskopie untersucht. Die Archaerhodopsin-3 Varianten durchlaufen einen ungewöhnlichen Photozyklus mit verlängerter Lebensdauer des angeregten Zustands und ineffizienter Photoisomerisierung. Präresonanz-Raman-Spektroskopie und Hochdruckflüssigkeitschromatographie ermöglichten die direkte Untersuchung des Chromophors in diesen besonderen Rhodopsinen. Molekulardynamiksimulationen, unterstützt durch spektroskopische Studien, liefern ein Modell der Proteindynamik unter Einfluss der Membranspannung. Protein-Engineering ermöglichte die Identifizierung der Aminosäuren, die für die Erhöhung der Fluoreszenzquantenausbeute benötigt werden, und der Schlüsselreste, die an der Spannungsmessung beteiligt sind. Aussichtsreiche Konstrukte mit verbesserten Eigenschaften wurden vorgeschlagen und getestet.Novel class of fluorescent membrane voltage sensors QuasArs, based on Archaerhodopsin-3, have been reported by Hochbaum et al. in 2014. The new constructs show unusually high fluorescence quantum yield for microbial rhodopsins. Furthermore the fluorescence is voltage-dependent, which is a desirable property for membrane voltage sensors. These tools would offer high spatiotemporal resolution allowing to track neuronal spiking. Although multiple constructs have been proposed, their fluorescence quantum yield is still too low (<1%) for applications in living rodents and requires further improvement for imaging applications. However, rational design of the next generation rhodopsin-based fluorescent sensors is restrained since the current constructs were found using random mutagenesis. To develop improved constructs it is essential to understand the functionality of the voltage-sensitive fluorescence and the role of the introduced mutations. In this thesis, the microbial rhodopsin based voltage sensors and the origin of their voltage-modulated fluorescence were studied. The photodynamics of microbial rhodopsin-based voltage sensors were studied with UV/Vis steady state and transient spectroscopy. The archaerhodopsin-3 variants undergo an unusual photocycle with extended excited state lifetime and inefficient photoisomerization. Pre-resonance Raman spectroscopy and high-pressure liquid chromatography allowed to directly study the chromophore composition in these peculiar rhodopsins. Molecular dynamics simulations, supported by spectroscopic studies, provide a model of protein dynamics taking place under different membrane voltage conditions. Protein engineering allowed to identify the residues needed for the increase of the fluorescence quantum yield and key residues involved in the voltage sensing. Promising constructs, with improved properties, were proposed and tested

Photocycle Dynamics of the Archaerhodopsin 3 Based Fluorescent Voltage Sensor QuasAr1

The retinal photocycle dynamics of the fluorescent voltage sensor QuasAr1 (Archaerhodopsin 3 P60S-T80S-D95H-D106H-F161V mutant from Halorubrum sodomense) in pH 8 Tris buffer was studied. The samples were photoexcited to the first absorption band of the protonated retinal Schiff base (PRSB) Ret_580 (absorption maximum at lambda(max) approximate to 580 nm), and the retinal Schiff base photoisomerization and protonation state changes were followed by absorption spectra recordings during light exposure and after light exposure. Ret_580 turned out to be composed of two protonated retinal Schiff base isomers, namely Ret_580(I) and Ret_580(II). Photoexcitation of Ret_580(I) resulted in barrier-involved isomerization to Ret_540 (quantum yield approximate to 0.056) and subsequent retinal proton release leading to Ret_410 deprotonated retinal Schiff base (RSB). In the dark, Ret_410 partially recovered to Ret_580(I) and partially stabilized to irreversible Ret_400 due to apoprotein restructuring (Ret_410 lifetime approximate to 2 h). Photoexcitation of Ret_580(II) resulted in barrier-involved isomerization to Ret_640 (quantum yield approximate to 0.00135) and subsequent deprotonation to Ret_370 (RSB). In the dark, Ret_370 partially recovered to Ret_580(II) and partially stabilized to irreversible Ret_350 due to apoprotein restructuring (Ret_370 lifetime approximate to 10 h). Photocycle schemes and reaction coordinate diagrams for Ret_580(I) and Ret_580(II) were developed and photocyle parameters were determined

Absorption and Emission Spectroscopic Investigation of the Thermal Dynamics of the Archaerhodopsin 3 Based Fluorescent Voltage Sensor Archon2

Archon2 is a fluorescent voltage sensor derived from Archaerhodopsin 3 (Arch) of Halorubrum sodomense using robotic multidimensional directed evolution approach. Here we report absorption and emission spectroscopic studies of Archon2 in Tris buffer at pH 8. Absorption cross-section spectra, fluorescence quantum distributions, fluorescence quantum yields, and fluorescence excitation spectra were determined. The thermal stability of Archon2 was studied by long-time attenuation coefficient measurements at room temperature (21 +/- 1 degrees C) and at refrigerator temperature (3 +/- 1 degrees C). The apparent melting temperature was determined by stepwise sample heating up and cooling down (obtained apparent melting temperature: 63 +/- 3 degrees C). In the protein melting process protonated retinal Schiff base (PRSB) with absorption maximum at 586 nm converted to de-protonated retinal Schiff base (RSB) with absorption maximum at 380 nm. Storage of Archon2 at room temperature and refrigerator temperature caused absorption coefficient decrease because of partial protein clustering to aggregates at condensation nuclei and sedimentation. At room temperature an onset of light scattering was observed after two days because of the beginning of protein unfolding. During the period of observation (18 days at 21 degrees C, 22 days at 3 degrees C) no change of retinal isomer composition was observed indicating a high potential energy barrier of S-0 ground-state isomerization

QuasAr Odyssey: the origin of fluorescence and its voltage sensitivity in microbial rhodopsins

Rhodopsins had long been considered non-fluorescent until a peculiar voltage-sensitive fluorescence was reported for archaerhodopsin-3 (Arch3) derivatives. These proteins named QuasArs have been used for imaging membrane voltage changes in cell cultures and small animals. However due to the low fluorescence intensity, these constructs require use of much higher light intensity than other optogenetic tools. To develop the next generation of sensors, it is indispensable to first understand the molecular basis of the fluorescence and its modulation by the membrane voltage. Based on spectroscopic studies of fluorescent Arch3 derivatives, we propose a unique photo-reaction scheme with extended excited-state lifetimes and inefficient photoisomerization. Molecular dynamics simulations of Arch3, of the Arch3 fluorescent derivative Archon1, and of several its mutants have revealed different voltage-dependent changes of the hydrogen-bonding networks including the protonated retinal Schiff-base and adjacent residues. Experimental observations suggest that under negative voltage, these changes modulate retinal Schiff base deprotonation and promote a decrease in the populations of fluorescent species. Finally, we identified molecular constraints that further improve fluorescence quantum yield and voltage sensitivity

The femtosecond-to-second photochemistry of red-shifted fast-closing anion channelrhodopsin PsACR1

Anion channelrhodopsins (ACRs) are of great interest due to their ability to inhibit electrical signaling in optogenetic experiments. The photochemistry of ACRs is currently poorly understood and an improved understanding would be beneficial for rational design of ACRs with modified properties. Activation/deactivation of ACRs involves a series of photoreactions ranging from femtoseconds to seconds, thus real-time observation is essential to comprehend the full complexity of the photochemical processes. Here we investigate the photocycle of an ACR from Proteomonas sulcata (PsACR1), which is valuable for optogenetic applications due to the red-shifted absorption and action spectra compared to the prototype ACRs from Guillardia theta: GtACR1 and GtACR2, and the fast channel closing properties. From femto-to-submillisecond transient absorption spectroscopy, flash photolysis, and point mutations of acidic residues near the retinal Schiff base (RSB), E64, and D230, we found that the photoisomerization occurs in similar to 500 fs independent of the protonation state of E64. Notably, E64 is involved in the rearrangement of the hydrogen-bond network near the RSB after photoisomerization. Furthermore, we suggest that E64 works as a primary proton acceptor during deprotonation of the RSB as has been proposed for GtACR1. Our findings allow for a deeper understanding of the photochemistry on the activation/deactivation of ACRs

QuasAr Odyssey: the origin of fluorescence and its voltage sensitivity in microbial rhodopsins

Rhodopsins had long been considered non-fluorescent until a peculiar voltage-sensitive fluorescence was reported for archaerhodopsin-3 (Arch3) derivatives. These proteins named QuasArs have been used for imaging membrane voltage changes in cell cultures and small animals, but they could not be applied in living rodents. To develop the next generation of sensors, it is indispensable to first understand the molecular basis of the fluorescence and its modulation by the membrane voltage. Based on spectroscopic studies of fluorescent Arch3 derivatives, we propose a unique photo-reaction scheme with extended excited-state lifetimes and inefficient photoisomerization. Molecular dynamics simulations of Arch3, of the Arch3 fluorescent derivative Archon1, and of several its mutants have revealed different voltage-dependent changes of the hydrogen-bonding networks including the protonated retinal Schiff-base and adjacent residues. Experimental observations suggest that under negative voltage, these changes modulate retinal Schiff base deprotonation and promote a decrease in the populations of fluorescent species. Finally, we identified molecular constraints that further improve fluorescence quantum yield and voltage sensitivity