Turnover number molecular

The turnover number of an enzyme, is a measure of its maximal catalytic activity, is defined as the number of substrate molecules converted into product per enzyme molecule per unit time when the enzyme is saturated with substrate. The turnover number is also referred to as the molecular activity of the enzyme. For the simple Michaelis-Menten reaction (14.9) under conditions of initial velocity measurements, Provided the concentration of... 

Quantum yield and luciferase activity The quantum yield of coelenterazine in the luminescence reaction catalyzed by Oplophorus luciferase was 0.34 when measured in 15 mM Tris-HCl buffer, pH 8.3, containing 0.05 M NaCl at 22°C (Shimomura et al., 1978). The specific activity of pure luciferase in the presence of a large excess of coelenterazine (0.9pg/ml) in the same buffer at 23°C was 1.75 x 1015 photons s 1 mg-1 (Shimomura et al., 1978). Based on these data and the molecular weight of luciferase (106,000), the turnover number of luciferase is calculated at 55/min. 

Renilla luciferase. The luciferase of Renilla reniformis has been purified and characterized by Karkhanis and Cormier (1971) and Matthews et al. (1977a). The purified luciferase has a molecular weight of 35,000, and catalyzes the luminescence reaction of coelenterazine. The luciferase-catalyzed luminescence is optimum at pH 7.4, at a temperature of 32°C, and in the presence of 0.5 M salt (such as NaCl or KC1). The luciferase has a specific activity of 1.8 x 1015 photons s"1mg"1, and a turnover number of 111/min. The luminescence spectrum shows a maximum at 480 nm. The absorbance A28O of a 0.1% luciferase solution is 2.1. The luciferase has a tendency to self-aggregate, forming higher molecular weight species of lower luminescence activities. 

Theories neglect that catalysts usually have limited turnover numbers due to destructive side reactions. This may not be so obvious in analytical experiments but it has severe consequences for large scale applications. A simple calculation can illustrate this problem if a redox polymer with a monomer molecular weight of 400 Da and a density of 1 g cm " is considered with all redox centers addressable from the electrode and accessible to the substrate with a turnover number of 1000, then, to react 1 nunol of substrate at a 1 cm electrode surface, at least 5 pmol of active catalyst centers corresponding to 2 mg of polymer, or a dry film thickness of 20 pm are required. This is 20 times more than the calculated optimum film thickness for rather favorable conditions... 

The oxidation of phenol, ortho/meta cresols and tyrosine with Oj over copper acetate-based catalysts at 298 K is shown in Table 3 [7]. In all the cases, the main product was the ortho hydroxylated diphenol product (and the corresponding orthoquinones). Again, the catalytic efficiency (turnover numbers) of the copper atoms are higher in the encapsulated state compared to that in the "neat" copper acetate. From a linear correlation observed [7] between the concentration of the copper acetate dimers in the molecular sieves (from ESR spectroscopic data) and the conversion of various phenols (Fig. 5), we had postulated [8] that dimeric copper atoms are the active sites in the activation of dioxygen in zeolite catalysts containing encapsulated copper acetate complexes. The high substratespecificity (for mono-... 

Table 1. Some molybdenum-containing enzymes. For some of the enzymes the numerical data are rather approximate only. Turnover numbers refer to temperatures between 23 and 30°. Since some of the molecular weights are particularly uncertain, contents of flavin etc. are expressed per molybdenum atom rather than per mole of protein. Most of the enzymes have a much wider range of substrate specificities than has been indicated...

The turnover number of an enzyme is defined as the maximum number of moles of substrate reacted per mole of enzyme (or molecules per molecule) per minute under optimum conditions (i.e., saturating substrate concentration, optimum pH, etc). If 2 mg/cm3 of a pure enzyme (50,000 molecular weight, Michaelis constant Km = 0.03 mole/m3) catalyzes a reaction at a rate of 2.5 jumoles/nUksec when the substrate concentration is 5 x 10 3 moles/m3, determine the turnover number corresponding to this definition and the actual number of moles of substrate reacting per minute per mole of enzyme. 

What is really happening [23, 24] in the glucose —> mannitol cascade [19] can be seen from the quite complicated kinetic and molecular picture shown in Fig. 13.9, including three different types of kinetics (expressed in turnover numbers in Table 13.1) ... 

The "catalyst" may be added to the reactants in a different form, the catalyst precursor, which has to be brought into an active form ("activated"). During the catalytic cycle the catalyst may be present in several intermediate forms when we look more closely at the molecular level. An active catalyst will pass a number of times through this cycle of states in this sense the catalyst remains unaltered. The number of times that a catalyst goes through this cycle is the turnover number. The turnover number (TON) is the total number of substrate... 

The most fundamental unit for reporting enzyme activity is its turnover number, the number of substrate molecules converted to product by one molecule of the enzyme in one minute. Its calculation, however, requires pure protein and knowledge of the enzyme s molecular mass. 

This transformation has been applied to several chiral production processes, the first being the synthesis of a pheromone (Disparlure) intermediate (S) albeit with low turnover numbers and only 91 % ee. Another industrial product is the epoxide of allyl alcohol as developed by PPG-Sipsy, to give a process where catalyst loading was decreased by molecular sieve addition and the safety factors involving peroxide contamination were overcome. These examples are shown in Figure 1.46. 

The kcat is given in the unit min" . The commentary lists the names of the substrates, sometimes with information on the reaction conditions or the type of reaction if the enzyme is capable of catalyzing different reactions with a single substrate. For cases where it is impossible to give the turnover number in the defined unit (e.g., substrates without a defined molecular weight, or an undefined amount of protein) this is summarized in Additional Information. 

Here Et is the total enzyme, namely, the free enzyme E plus enzyme-substrate complex ES. The equation holds only at substrate saturation, that is, when the substrate concentration is high enough that essentially all of the enzyme has been converted into the intermediate ES. The process is first order in enzyme but is zero order in substrate. The rate constant k is a measure of the speed at which the enzyme operates. When the concentration [E]t is given in moles per liter of active sites (actual molar concentration multiplied by the number of active sites per mole) the constant k is known as the turnover number, the molecular activity, or kcat. The symbol fccat is also used in place of k in Eq. 9-6 for complex rate expressions in which fccat cannot represent a single rate constant but is an algebraic expression that contains a number of different constants. 

Of the two homogeneous preparations of a nonspecific adenosine aminohydrolase from Aspergillus oryzae (Takadiastase) (92,179), that described by Wolfenden et al. (92) appears to be more facile and concise. Both procedures yield enzyme with turnover numbers near 105 moles adenosine deaminated per minute and molecular weights near 215,000. The mo-... 

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