LEE- Moleküler Biyoloji-Genetik ve Biyoteknoloji-Yüksek Lisans
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ÖgeThe synthesis, SLIC based labeling, and characterization of microbial rhodopsins by using custom build spectroscopic methods(Graduate School, 2023-01-26) Çavdar, Cansu ; Bayraktar, Halil ; 521191105 ; Molecular Biology-Genetics and BiotechnologyType I opsins (also known as microbial opsins) are seven transmembrane-domain proteins with retinal chromophore absorbing incoming light. Most of them are ion channels or pumps although they do not directly bind to G protein complexes. They are found in all three domains of life. Numerous homologous forms of rhodopsins have been identified in the microorganisms, including light sensors (sensory rhodopsins), transmembrane chloride pumps (halorhodopsins), and energy saving transmembrane proton pumps (bacteriorhodopsin or proteorhodopsin). Rhodopsin proteins are widely used in the field of biotechnology. For example, it is used to determine the membrane voltage level in neurons. The use of rhodopsins as tools to control membrane potential with light is another technique for transformative optogenetics technology. Membrane voltage is present in all cells, and it creates an electric signal to carry the signal across the cell membrane and provides cell-cell communication. Since the absorption methods are not sufficient to measure voltage signal due to low signal to noise ratio in cells, more sensitive fluorescent methods based on rhodopsin are strongly preferred for a wide spectrum of applications. An understanding of the dynamics of the microbial rhodopsin proteins is essential to tune the photophysical properties of rhodopsins. It is also necessary to label them with fluorescent proteins and characterize their localization in detail. For the fluorescent signal to vary with the amount of light absorption in the membrane protein, the linker peptide between the proteins has to be optimized for various applications. For electrochromic fluorescent energy transfer, it is necessary to select the appropriate fluorescent protein. The emission signal of the fluorescent protein must overlap with the absorption signal of the membrane protein. After the most suitable fluorescent proteins are selected by calculating the amount of overlap, the structure of the peptide that binds the membrane and the fluorescent protein should be determined. Since both the length and the bending ratio of the selected peptide are important, it is necessary to optimize by testing different constructs. Here we have synthesized, purified, and studied the rhodopsin by using molecular biology and various spectroscopy methods. After the synthesis of rhodospins in BL21 cells, it was purified with his-tag affinity column chromatography and reconstituted with a detergent solution. The color tuning of rhodopsin as a function of pH was investigated by using absorption spectroscopy. We found that BPR undergoes a large red shift under acidic conditions. A pH value was increased the color turned from orange to red at the basic solution. We concluded that the deprotonation of the retinal at the rhodopsin center results in a significant change in the color of BPR. We have also measured the transient absorption changes of BPR by using a custom home built spectrometer that was equipped with two laser lines and an op amp light detector. The data acquisition and the control of lasers were performed an by arduino and field programmable gate array device programmed with arduino and labview respectively. Our results indicate that BPR underwent an absorption change after stimulated with a 532 nm diode laser. Finally, the fluorescent proteins were also cloned into the SRII gene by using SLIC cloning method and expressed in BL21 cells to determine the changes in fluorescent emission. Sensory rhodopsin was similarly characterized by using absorption spectroscopy. As conclusion, BPR undergoes a large spectral shift due to deprotonation upon decreasing pH and alters the color of the protein. SLIC method provides a cost-efficient method to prepare fluorescently labeled rhodopsin proteins. Contrary to the standard cloning techniques used in molecular biology, the SLIC method, which is convenient in terms of time and cost, has been studied and the method has been optimized. The optimized SLIC method can be used as an alternative to other molecular cloning techniques. The custom build pump-probe system can also be used for the characterization of fluorescently labeled other rhodopsin proteins in future studies.