Prosthetic groups structure

Tyr 143, 36 293 Tyr 254, 36 291-293 NMR spectroscopy, 36 271-272 pH dependence, 36 274-275 primary stmcture, 36 261-263 prosthetic groups structure, 36 258 quaternary structure, 36 261-262 reduction potentials, 36 268-269 short electron transport chain, 36 258-259 site-directed mutagenesis, 36 289-290 substrate specificity, 36 272-274 Flavocytochrome C552 electrochemistry, 36 365-367, 369... 

Structure of the MoFe Protein. Extensive spectroscopic studies of the MoEe proteia, the appHcation of cluster extmsion techniques (84,151), x-ray anomalous scattering, and x-ray diffraction (10,135—137,152) have shown that the MoEe proteia contains two types of prosthetic groups, ie, protein-bound metal clusters, each of which contains about 50% of the Ee and content. Sixteen of the 30 Ee atoms and 14—16 of the 32—34... 

Oxidation of P-nicotinamide adenine dinucleotide (NADH) to NAD+ has attracted much interest from the viewpoint of its role in biosensors reactions. It has been reported that several quinone derivatives and polymerized redox dyes, such as phenoxazine and phenothiazine derivatives, possess catalytic activities for the oxidation of NADH and have been used for dehydrogenase biosensors development [1, 2]. Flavins (contain in chemical structure isoalloxazine ring) are the prosthetic groups responsible for NAD+/NADH conversion in the active sites of some dehydrogenase enzymes. Upon the electropolymerization of flavin derivatives, the effective catalysts of NAD+/NADH regeneration, which mimic the NADH-dehydrogenase activity, would be synthesized [3]. 

Koda, P., and Lee, J. (1979). Separation and structure of the prosthetic group of the blue fluorescence protein from the bioluminescent bacterium Photobacterium phosphoreum. Proc. Natl. Acad. Sci. USA 76 3068-3072. 

Prosthetic Groups Are Tightly Integrated Into an Enzyme s Structure... 

HRP is a hemoprotein containing photohemin IX as its prosthetic group. The presence of the heme structure gives the enzyme its characteristic color and maximal absorptivity at 403 nm.The ratio of its absorbance in solution at 403 nm to its absorbance at 275 nm, called the RZ or Reinheitzahl ratio, can be used to approximate the purity of the enzyme. However, at least seven isoenzymes exist for HRP (Shannon et al., 1966 Kay et al., 1967 Strickland et al., 1968), and their RZ values vary from 2.50 to 4.19. Thus, unless the RZ ratio is precisely known or determined for the particular isoenzyme of HRP utilized in the preparation of an antibody-enzyme conjugate, subsequent measurement after crosslinking would yield questionable results in the determination of the amount of HRP present in the conjugate. 

Glucose oxidase (GOD) is a typical flavin enzyme with flavin adenine dinucleotide (FAD) as redox prosthetic group. Its biological function is to catalyze glucose to form gluconolaction, while the enzyme itself is turned from GOD(FAD) to GOD(FADH2). GOD was used to prepare biosensors in extensive fields. Many materials that can be used to immobilize other proteins can be suitable for GOD. GOD adsorbed on CdS nanoparticles maintained its bioactivity and structure, and could electrocatalyze... 

It is quite evident that the ferrous complexes of porphyrins, both natural and synthetic, have extremely high affinities towards NO. A series of iron (II) porphyrin nitrosyls have been synthesized and their structural data [11, 27] revealed non-axial symmetry and the bent form of the Fe-N=0 moiety [112-116]. It has been found that the structure of the Fe-N-O unit in model porphyrin complexes is different from those observed in heme proteins [117]. The heme prosthetic group is chemically very similar, hence the conformational diversity was thought to arise from the steric and electronic interaction of NO with the protein residue. In order to resolve this issue femtosecond infrared polarization spectroscopy was used [118]. The results also provided evidence for the first time that a significant fraction (35%) of NO recombines with the heme-Fe(II) within the first 5 ps after the photolysis, making myoglobin an efficient N O scavenger. 

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