Two‐Color Two‐Photon Excitation of Intrinsic Protein Fluorescence: Label‐Free Observation of Proteolytic Digestion of Bovine Serum Albumin

Quentmeier, Stefan; Quentmeier, Claudia C.; Walla, Peter Jomo; Gericke, Karl‐Heinz

doi:10.1002/cphc.200800586

Cited by 8 publications

(11 citation statements)

References 43 publications

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“…As measuring parameters, intensity and fluorescence decay time have been previously used. 5,6 The measurement of the emission maximum and its shift with proteolysis presented here is new. The measurement of fluorescence intensity is considered less appropriate because it is influenced by many different factors, while both the decay time and the shift of the maximum appear to be more specific.…”

Section: Resultsmentioning

confidence: 98%

“…4 Fluorescence spectroscopy was also used for the monitoring of proteolysis processes by the measurements of the changes in intrinsic tryptophan fluorescence. 5,6 These studies engaged different spectroscopic methods, including simple measurements at one wavelength of the changes in static fluorescence intensity of Trp residues 5 , or much more complicate technique based on the determination of the apparent life time changes with two-color two-photon laser equipment. 6 In many cases, extrinsic fluorophores with emission in the visible range of the spectrum are used which can be easily measured.…”

Section: Introductionmentioning

confidence: 99%

“…5,6 These studies engaged different spectroscopic methods, including simple measurements at one wavelength of the changes in static fluorescence intensity of Trp residues 5 , or much more complicate technique based on the determination of the apparent life time changes with two-color two-photon laser equipment. 6 In many cases, extrinsic fluorophores with emission in the visible range of the spectrum are used which can be easily measured. Measurements of the fluorescence of extrinsic fluorophores attached to the protein substrate was also used for monitoring of proteolysis.…”

Section: Introductionmentioning

confidence: 99%

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Monitoring of Demasking of Peptide Bonds During Proteolysis by Analysis of the Apparent Spectral Shift of Intrinsic Protein Fluorescence

et al. 2011

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Demasking of peptide bonds during proteolysis of β-casein and β-lactoglobulin by trypsin was monitored by the measurement of the overall spectral shift of intrinsic protein fluorescence. A clear shift of the apparent emission maxima from approximately 340-345 nm to 355-360 nm during proteolysis was observed, with a time course, which follows protein degradation and structural opening. In contrast to procedures using extrinsic fluorescence labels, this label-free procedure does not bear the risk of structural alterations. It is easy to perform, fast, and has a relatively high accuracy of determination. Proteolysis was modelled as simple two-step process with consecutive demasking and hydrolysis stages. It was shown that the fluorescence shift can be attributed to the demasking stage. Formally, kinetics of the peptide bond demasking obeys a first-order kinetic law. Both the theoretical simulations and experiment are in accordance giving the similar dependences of the hydrolysis degree on the degree of peptide bond demasking.

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Section: Resultsmentioning

confidence: 98%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Monitoring of Demasking of Peptide Bonds During Proteolysis by Analysis of the Apparent Spectral Shift of Intrinsic Protein Fluorescence

et al. 2011

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“…As mentioned above, one of the first applications of 2C2P fluorescence was the label-free monitoring of a proteolytic digestion of the protein BSA by subtilisin [15]. BSA contains five tryptophans, which act as a natural built-in probe for their surroundings.…”

Section: Experimental Setup and Resultsmentioning

confidence: 99%

“…In addition to the above-mentioned proteolytic cleavage of BSA by subtilisin, a similar reaction between BSA and elastase is monitored. The experimental setup is shown in figure 1 and was described in detail previously [15]. The reaction is performed at concentrations of 0.1 mM BSA and 0.01 mM elastase.…”

Section: Experimental Setup and Resultsmentioning

confidence: 99%

Applications of the time-resolved two-colour two-photon excitation of UV fluorophores using femtosecond laser pulses

et al. 2009

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A short overview of the principles and applications of the two-colour two-photon (2C2P) excitation of fluorescence by using femtosecond pulses is given. Fluorescence is generated by the simultaneous absorption of an 800 nm photon and a 400 nm photon of overlapping laser beams of a titanium:sapphire laser. Two examples of its application are presented: firstly, it is used to monitor the enzymatic cleavage of bovine serum albumin (BSA) by elastase. The fluorescent amino acid tryptophan present in BSA is excited corresponding to an effective one-photon wavelength of 266 nm. Secondly, it is shown how one can utilize the different polarizations of the excited beams for determining the symmetry of the excited states of molecules, exemplarily shown for p-terphenyl in cyclohexane. Further applications and experiments for 2C2P are suggested for using it in UV-fluorescence microscopy and for determining the properties of the electronic states of biomolecules by using differently polarized photons.

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Label-Free Spatial Analysis of Free and Enzyme-Bound NAD(P)H in the Presence of High Concentrations of Melanin

et al. 2011

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The analysis of autofluorescence, often regarded as undesired noise during the imaging of biological samples, allows label free, unbiased detection of NAD(P)H and melanin in native samples. Because both the emission and absorption spectra of these fluorophores overlap and they can hence not be differentiated using emission filters or with different excitation wavelengths, fluorescence lifetime imaging microscopy (FLIM) is used to differentiate between them. In the present paper the application of two-photon excitation microscopy is presented to investigate the autofluorescence of fungal spores. The model organism which was examined is Aspergillus ochraceus. Furthermore a strategy is developed which allows to quantitatively analyze the fluorescence lifetimes of melanin, free NAD(P)H and protein-bound NAD(P)H using forward convolution of a multiexponential decay function with the instrument response function (IRF) and subsequent fitting to the experimental fluorescence data. As a consequence proteins, which are able to bind NAD(P)H, are located with sub-cellular resolution. Furthermore a spatial differentiation of the fluorophores NAD(P)H and melanin inside the spores, is revealed.

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Two‐Color Two‐Photon Excitation of Intrinsic Protein Fluorescence: Label‐Free Observation of Proteolytic Digestion of Bovine Serum Albumin

Cited by 8 publications

References 43 publications

Monitoring of Demasking of Peptide Bonds During Proteolysis by Analysis of the Apparent Spectral Shift of Intrinsic Protein Fluorescence

Monitoring of Demasking of Peptide Bonds During Proteolysis by Analysis of the Apparent Spectral Shift of Intrinsic Protein Fluorescence

Applications of the time-resolved two-colour two-photon excitation of UV fluorophores using femtosecond laser pulses

Label-Free Spatial Analysis of Free and Enzyme-Bound NAD(P)H in the Presence of High Concentrations of Melanin

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