Time-resolved fluorescence of the two tryptophans in horse liver alcohol dehydrogenase

Jb, Ross; Schmidt, Carl J.; Brand, Ludwig

doi:10.1021/bi00518a021

Cited by 169 publications

(135 citation statements)

References 44 publications

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“…In our opinion, it seems unreasonable to interpret the two lifetime values obtained for HSOD using the two-exponential model with the presence of two molecular species, one of which accounts for about 10% of the total. At variance with other cases reported and with the classic example of horse liver alcohol dehydrogenase [13,14], the two tryptophauyl residues of HSOD are equivalent. In addition, it is very common to find single-tryptophan proteins with double-or triple-exponential decay [l].…”

Section: Resultscontrasting

confidence: 69%

A time-resolved fluorescence study of human copper-zinc superoxide dismutase

Rosato¹,

Mei²,

Gratton³

et al. 1990

Biophysical Chemistry

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Superoxide dismutase; Time-resolved fluorescence: Fluorescence lifetime distribution; (Human)The intrinsic fluorescence decay of human Cu,Zn superoxide dismutase was measured by frequency-domain techniques. The protein consists of two subunits, each containing one tryptophsn and no tyrosine residues. Using a synchrotron radiation source, which allows facile selection of the excitation wavelength, the dependence of the emission decay upon excitation was studied. No significant excitation wavelength effects were found The two vvptophans contained in the dimer, although fully equivalent and exposed to solvent, showed a fluorescence decay that cannot be described by a single lifetime. Either two lifetimes. or one Lorentzian-shaped continuous distribution of lifetimes, are needed to obtain a good fit. Under identical experimental conditions, control experiments showed that N-acetyltryptophanamide, an analogue of tryptophanyl residues in proteins, decays with a single lifetime. The hetero~eous decay of tryptophan fluoresce& in superoxide dismutase is interpreted as due to the,presence of static and/or dynamic conformers in the protein that deMy with different lifetimes. The two models of discrete lifetimes and continuous distribution of lifetimes are discussed with reference to measurements on holo-and ape-human superoxide dismutase.

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Section: Resultscontrasting

confidence: 69%

A time-resolved fluorescence study of human copper-zinc superoxide dismutase

Rosato¹,

Mei²,

Gratton³

et al. 1990

Biophysical Chemistry

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“…The fitting procedure was performed by an iterative non-linear least-squares method as described previously [15]. The simultaneous analysis of a series of fluorescence quenching data enabled the fluorescence emission spectrum to be resolved into components according to Eqn (5).…”

Section: Methodsmentioning

confidence: 99%

Fluorescence‐quenching‐resolved spectra of fluorophores in mixtures and micellar solutions

Wasylewski

Kaszycki

Guz

et al. 1988

European Journal of Biochemistry

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The application of a new fluorescence-quenching-resolved spectroscopic method [Wasylewski, Z., Koloczek, H. and Wahiowska, A. (1988) Eur. J . Biochem. 172, 719-7241 for resolving fluorescence emission spectra of a mixture of fluorophores into components is described. Contrary to fluorescence lifetime measurements, in this method the overlapping spectra can be decomposed even if the components have similar or the same fluorescence lifetimes, but differ in bimolecular-rate-quenching constants. Using this technique, we have resolved the emission spectra of a two-component mixture of fluorescein and riboflavin, which have very similar fluorescence lifetimes. To illustrate the utility of this approach in the study of fluorophores in compartmentalized biological systems such as lipid bilayers, we have also used the method to resolve the emission spectra of a two-component mixture of fluorophores commonly used in biological studies which undergo partition between water and a micellar phase.Fluorescence spectroscopy is frequently used as a quantitative method to analyze complex systems in the physical, chemical and biological sciences. The resolution of fluorescence emission heterogeneity, which can result both from ground-state heterogeneity and excited-state reactions [l], provides more detailed information about the mixture of fluorophore components or information about the environment of the fluorophore probes [l]. In order to resolve the fluorescence emission spectra of a heterogeneous system of a mixture of aromatic fluorophores or of two tryptophan residues in proteins, the time-domain [l -61 and phase-modulation techniques [7 -111 have been used. Both these approaches require the fluorescence lifetimes of the components investigated to be significantly different. To resolve the overlapping spectra one has to obtain a number of decay measurements at different emission wavelengths.Recently [12], we have developed a powerful new method which involves the determination of fluorescence-quenchingresolved spectra (FQRS). In this new procedure steady-state emission spectra are collected at several fluorescence quencher concentrations. Then the Stern-Volmer quenching analysis, performed by an iterative non-linear least-squares method at each particular wavelength, allows resolution of the emission spectra into components.In the FQRS method, the possibility of resolving the fluorescence emission spectra depends on differences in the dynamic Stern-Volmer quenching constants, K , of the components. Since the Stern-Volmer constant for an efficient quencher is proportional both to the fluorescence lifetime T~ and bimolecular rate quenching constant k,, a mixture of fluorophores differing in T~ and/or k, can be successfully resolved into components.We report here the first FQRS measurements for a twocomponent mixture of fluorophores of biological interest, which have similar fluorescence lifetimes, such as riboflavin and fluorescein. The FQRS method has also been used to resolve the heterogeneous fluorescence of probes (diph...

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“…Using single-photon counting techniques and the analysis of fluorescence decay curves as a function of emission wavelengths, Wahl et al [3, 41 first resolved complex fluorescence spectra of two-tryptophan-containing proteins such as Escherichia cofi lac repressor protein [3] and phosphoglycerate kinase [4]. Following a similar method, Ross et al [5] resolved the emission spectrum of alcohol liver dehydrogenase into two tryptophan residues. Using the phase-resolved fluorescence method, it has been shown recently that the spectrum of twotryptophan-containing metalloprotease from Staphylococcus aureus can be decomposed into two components, which have been attributed to each of the tryptophan residues [9].…”

mentioning

confidence: 99%

Fluorescence‐quenching‐resolved spectroscopy of proteins

Wasylewski

Kołoczek

Waśniowska

1988

European Journal of Biochemistry

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A new procedure is described for using fluorescence-quenching data of tryptophan residues in proteins to resolve their fluorescence emission spectra. In this concept the Stern-Volmer quenching plot is determined at each particular emission wavelength and itterative non-linear least-squares fitting procedure allowed to resolve the steady-state emission spectra into components. The resolved components, attributed to each of tryptophan residue, can be characterized by different accessibility to the quencher. The ability to resolve fluorescence emission spectra can be improved by using different kinds of efficient quenchers, which can selectively quench the emission of exposed or both exposed and buried fluorophores. The method was used to decompose emission fluorescence spectra in two-tryptophan-containing proteins; horse liver dehydrogenase, sperm whale apomyoglobin and metalloprotease from Staphylococcus aureus. The resolved spectra of alcohol dehydrogenase and metalloprotease are in excellent agreement with those previously obtained by single-photon counting or phase methods. The method presented here is technically simple and does not require expensive instrumentation.The intrinsic fluorescence of tryptophan residues in proteins has been widely used in the analysis the dynamics and conformational perturbation in these macromolecules. In native proteins these residues can occupy different locations where they can be influenced by the distinct environment, characterized by a particular set of physico-chemical conditions. In consequence the fluorescence contributions of particular tryptophan residues in multitryptophan-containing proteins can vary over a wide range [l]. Interpretation of the intrinsic fluorescence data of proteins often requires the resolution of the fluorescence properties. The resolution of fluorescence emission in proteins and its correlation with an individual tryptophan residue is still very difficult to achieve, since even single-tryptophan proteins can exhibit multiexponential decay kinetics [l].In principle, when dealing with a protein containing more than one tryptophan residue, steady-state fluorescence emission spectra can be resolved into components by the timedomain [2 -61 or frequence-domain method [7 -101. Using single-photon counting techniques and the analysis of fluorescence decay curves as a function of emission wavelengths, Wahl et al. [3, 41 first resolved complex fluorescence spectra of two-tryptophan-containing proteins such as Escherichia cofi lac repressor protein [3] and phosphoglycerate kinase [4]. Following a similar method, Ross et al. [5] resolved the emission spectrum of alcohol liver dehydrogenase into two tryptophan residues. Using the phase-resolved fluorescence method, it has been shown recently that the spectrum of twotryptophan-containing metalloprotease from Staphylococcus aureus can be decomposed into two components, which have been attributed to each of the tryptophan residues [9].Correspondence to Z. Wasylewski, Zaklad Biochemii, Instytut Biologii Molekula...

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Time-resolved fluorescence of the two tryptophans in horse liver alcohol dehydrogenase

Cited by 169 publications

References 44 publications

A time-resolved fluorescence study of human copper-zinc superoxide dismutase

A time-resolved fluorescence study of human copper-zinc superoxide dismutase

Fluorescence‐quenching‐resolved spectra of fluorophores in mixtures and micellar solutions

Fluorescence‐quenching‐resolved spectroscopy of proteins

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