National Repository of Grey Literature 21 records found  beginprevious12 - 21  jump to record: Search took 0.00 seconds. 
NMR Solution Structure of the Protein PsbQ from Photosystem II.
RATHNER, Petr
The PsbQ protein (16.5 kDa) is an extrinsic protein found in the thylakoid membrane of higher plants and green algae. As a member of the Psb protein family, it is situated in the oxygen evolving center and takes part in the water splitting reaction. The stable oxygen production in photosystem II depends on the cooperation of PsbQ with other photosynthetic proteins, mainly PsbP. In order to identify the possible interaction sites, the tertiary structure in solution has to be determined. Although the X-ray crystallographic structure of PsbQ was determined previously, the conformation of residues 14-33 (so-called "missing link") was still unknown at the onset of this work. The initial backbone assignment as well as a secondary structure estimation were achieved recently. In this thesis the resonance assignment was extended and 15N as well as 13C NOESY-HSQC spectra were recorded to obtain structural constraints. The solution structure was determined using the program CYANA. The results obtained show that, while the four helix bundle domain is nearly identical compared to the available X-Ray crystallographic structure significant deviations occur in the N-terminal region. In particular, the residues 37-41, where a short ?-strand had been proposed in the crystal structure, exhibit high ?-helical propensity.
Biosensors for Environmental Monitoring and Biomedical Applications
ŠTOFIK, Marcel
Study of biosensors has become an essential part of research in biotechnology. Biosensors as fast, portable, highly sensitive, and low-cost bioanalytical detection devices have been utilized in many fields of human activity. The first part of the presented work focuses on electrochemical biosensors for rapid environmental screening of herbicides as water pollutants. A sol-gel immobilization method for a photosystem II (PSII) complex is studied in order to enhance the sensitivity and the signal strength and stability of a PSII-based biosensor. Computer simulations of a PSII biosensor are employed with the aim to find out how the immobilization membrane properties influence the biosensor parameters. Newly developed immobilization by a thin-layer membrane based on the results of computer simulations and revised measurement protocols are presented. The second part of the work is devoted to synthesis and electrochemical detection of newly developed metal labels for electrochemical immunosensors. The synthesis of dendrimer-encapsulated silver nanoparticles and biorecognition properties of biotin-nanocomposite conjugates are discussed. For detection of synthesized labels, a microfluidic detector was manufactured and tested and different approaches to packing of a microfluidic chip employing polydimethylsiloxane (PDMS) were investigated. Newly designed microstructures for a microfluidic separator of magnetic beads (MBs) were studied by computer simulations. The separator was made and trapping of MBs for the further employment in MBs-based immunoassays are presented
Molecular characterisation of selective proteins from plant photosystem II
HELLER, Jiří
This qualification work is trying to shed a little bit more light on some proteins present in higher plants, which structure and function in photosynthetic reaction remain unclear. In particular it treats proteins of photosystem II, called PsbR, PsbW and PsbX that are responsible for photosynthetic reaction optimization. This thesis contains data about proteins acquisition and their sequences elucidation.
Membrane protein interactions studied on single molecular level by force spectroscopy, optical spectroscopy and methods of computational biochemistry
MATĚNOVÁ, Martina
I have set for a challenging study that combined experimental and theoretical approaches in an attempt to resolve a role of small aminoacids in intermolecular interactions. First, I have proposed a hypothesis that described the interaction among individual aminoacids forming D helices of D1 and D2 proteins based on molecular dynamic simulations of a simplified model representing the reaction centre of photosystem II. Stability of the putative interhelical hydrogen bond network connecting D1 and D2 proteins was investigated experimentally with dynamic force spectroscopy using atomic force microscope. The results of both methods are in a full agreement with each other and reveal the key role of D1-Gly208 aminoacid in stability and functionality of photosystem II by providing milieu for weak interactions among three contact points at the cross of D helices: D1-Gly208 (O) and D2-Cys211 (O?), D1-Ser209 (O?) and D2-Ile204 (O), D1-Ser212 (O?) and D2-Gly207 (O). Mutation of the D1-Gly208 led to the increase in probability of the binding among the aforementioned aminoacids, undesirably strengthening the overall interactions among the proteins compromising photosynthetic capacity (D1-Ser208) or disabling of autotrophic growth (D1-Val208).
Membrane protein interactions studied on single molecular level by force spectroscopy, optical spectroscopy and methods of computational biochemistry
MATĚNOVÁ, Martina
I have set for a challenging study that combined experimental and theoretical approaches in an attempt to resolve a role of small aminoacids in intermolecular interactions. First, I have proposed a hypothesis that described the interaction among individual aminoacids forming D helices of D1 and D2 proteins based on molecular dynamic simulations of a simplified model representing the reaction centre of photosystem II. Stability of the putative interhelical hydrogen bond network connecting D1 and D2 proteins was investigated experimentally with dynamic force spectroscopy using atomic force microscope. The results of both methods are in a full agreement with each other and reveal the key role of D1-Gly208 aminoacid in stability and functionality of photosystem II by providing milieu for weak interactions among three contact points at the cross of D helices: D1-Gly208 (O) and D2-Cys211 (O?), D1-Ser209 (O?) and D2-Ile204 (O), D1-Ser212 (O?) and D2-Gly207 (O). Mutation of the D1-Gly208 led to the increase in probability of the binding among the aforementioned aminoacids, undesirably strengthening the overall interactions among the proteins compromising photosynthetic capacity (D1-Ser208) or disabling of autotrophic growth (D1-Val208).
Structural analysis of extrinsic proteins from the oxygen-evolving complex of photosystem II from higher plants
KOHOUTOVÁ, Jaroslava
All life on earth depends mainly on the presence of oxygen. Largest producers of oxygen are green plants, cyanobacteria and algae. Oxygen is released from the oxygenevolving complex of photosystem II during photosynthesis and it is used in cellular respiration of all life complexes. The oxygen-evolving complex of photosystem II has the same function in each photosynthetic organism, but it has a different composition and organization of extrinsic proteins; only PsbO protein is ubiquitous in all known oxyphototrophs. Until now only low resolution electron microscopy structural models of plant PSII and crystal structures of cyanobacterial PSII are available. Higher plant extrinsic proteins (PsbP, PsbQ and PsbR) are structurally unrelated, non-homologues to the cyanobacterial extrinsic proteins (PsbO, PsbU and PsbV) and this is the reason why it is not possible to predict arrangement of these proteins on the lumenal site of higher plant PSII. Recently, models differ mainly in the structure of the oxygen-evolving complex, which could be resolved by determination of the exact binding sites for extrinsic proteins. An other question evolves: if the difference in the oxygen-evolving complex composition is the result of evolution or adaptation of photosynthetic organisms to their environment. Structural knowledge of extrinsic proteins that could help to resolve the location and subsequently the function of extrinsic proteins is still incomplete. From this case,structural analysis, interactions and probably arrangement of proteins PsbP and PsbQ was studied and is described in detail in this thesis.
Electron microscopic studies of photosynthetic membranes and their pigment-protein complexes
GARDIAN, Zdenko
The overall structure of photosynthetic pigment-protein complexes and thylakoid membranes of various photosynthetic organisms was studied using electron microscopy.
Preparation of recombinant PsbQ protein of photosystem II from spinach for studies on the interactions between oxygen-evolving complex proteins.
HELLER, Jiří
Proteins of the oxygen-evolving complex of photosystem II from spinach are studied to gain information about the interactions between the participating proteins and thus structural insight into its role in the mechanism underlying oxygenic photosyntesis in higher plants. The work describes in detail the recombinant expression and purification of PsbQ in Escherichia coli, and site-directed mutagenesis of the W71F and W71Y mutants as candidates for protein interactions studies.
Elektrochemický biosenzor na bázi PSII pro detekci fotosyntetických herbicidů
Frolík, Jan ; Nedoma, Roman ; Malý, J. ; Krejčí, J. ; Masojídek, Jiří
We have developed a prototype of the electrochemical biosensor based on immobilized Photosystem II useful for pre-screening of herbicide presence in soil. We present an up-to-date state of our biosensor set-up consisting of a microflow system vessel, a semiautomatic control unit specially designed for amperometric measurement of PS II activity, and optionally a portable computer
: Role podjednotky PsbI ve struktuře a funkci komplexu fotosystému II u sinice Synechocystis
Dobáková, Marika ; Komenda, Josef ; Tichý, Martin
PsbI belongs to a group of small transmembrane subunits of the Photosystem II complex (PSII). In the absence of PsbI the photochemical activity of the cyanobacterial PSII is significantly decreased and the complex is destabilized as reflected by accelerated turnover of the D1 protein

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