Fluorescence and concentration

Relatively recently, AIS Sommer GmbH of Germany delivered a laser-induced fluorescence (LIP) analyzer for quality control in minerals and mineral processing (Broicher 2000). The LIP analyzer includes two light detector systems with three photomultipliers each, which evaluate three spectral bands in two time windows each. It was done in the Kiruna phosphorous iron ore mine, Sweden. The limitation of LIP analysis is that its accuracy depends on the complexity of the composition of the ore and the concentration and fluorescence properties of the critical minerals in relation to all the other minerals present. The phosphorous iron ore in Kiruna is ideal for LIP analyzes, because its iron minerals are practically non-luminescent, while magmatic apatite is strongly fluorescent with intensive emissions of Ce and Eu ". ... 

Diamond KR, Farrell TJ, Patterson MS. Measurement of fluorophore concentrations and fluorescence quantum yield in tissue-simulating phantoms using three diffusion models of steady-state spatially resolved fluorescence. Physics in Medicine and Biology 2003,48, 4135 1149. 

Since the pioneering work by Cotton et al. on heme proteins (Cotton et al., 1980), surface enhanced resonance Raman spectroscopy (SERRS), Sec. 6.1, has been used to study a large variety of biomolecules, such as retinal proteins (Nabiev et al., 1985), flavoproteins (Coperland et al., 1984 Holt and Cotton, 1987), chlorophylls (Cotton and Van Duyne, 1982 Hildebrandt and Spiro, 1988), and oxyhemoglobins (de Groot and Hesters, 1987). The advantages of this technique include low sample concentration and fluorescence quenching. The main question is whether or not the native structure and function of the molecule is preserved on the metal surface. 

The mechanism of fluorescein staining of ocular epithelia has been subject to some conjecture. In earlier work it was suggested that staining occurred due to accumulation in intraepithelial spaces rather than direct staining of the cells. However, it has become clear that fluorescein can directly stain diseased human corneal cells and rabbit epithelial cells. Moreover, the hyperfluorescence that probably represents micropunctate clinical staining is likely due to optimum dye concentration and fluorescence within the cell rather than simple pooling. Cellular hyperfluorescence occurred from both mechanical abrasion and chemically induced toxicity, conditions that presumably promote an intracellular concentration that allows definitive clinical visualization. An issue that has received some attention is whether repeated... 

A single environmental variable, such as pH, may affect both concentration and fluorescence quantum yield. If so, then the product of concentration and quantum yield becomes a single term in the multilinear model. 

Direct quantitation of receptor concentrations and dmg—receptor interactions is possible by a variety of techniques, including fluorescence, nmr, and radioligand binding. The last is particularly versatile and has been appHed both to sophisticated receptor quantitation and to dmg screening and discovery protocols (50,51). The use of high specific activity, frequendy pH]- or p lj-labeled, dmgs bound to cmde or purified cellular materials, to whole cells, or to tissue shces, permits the determination not only of dmg—receptor saturation curves, but also of the receptor number, dmg affinity, and association and dissociation kinetics either direcdy or by competition. Complete theoretical and experimental details are available (50,51). 

Fluorescence. The fluorescence detection technique is often used in clinical chemistry analyzers for analyte concentrations that are too low for the simpler absorbance method to be appHed. Fluorescence measurements can be categorized into steady-state and dynamic techniques. Included in the former are the conventional simultaneous excitation-emission method and fluorescence polarization. 

The use of agarose as an electrophoretic method is widespread (32—35). An example of its use is in the evaluation and typing of DNA both in forensics (see Forensic chemistry) and to study heritable diseases (36). Agarose electrophoresis is combined with other analytical tools such as Southern blotting, polymerase chain reaction, and fluorescence. The advantages of agarose electrophoresis are that it requires no additives or cross-linkers for polymerization, it is not hazardous, low concentration gels are relatively sturdy, it is inexpensive, and it can be combined with many other analytical methods. 

Fast concentration and sample injection are considered with the use of a theory of vibrational relaxation. A possibility to reduce a detection limit for trinitrotoluene to 10 g/cnf in less than 1 min is shown. Such a detection limit can by obtained using selective ionization combined with ion drift spectrometry. The time of detection in this case is 1- 3 s. A detection technique based on fluorescent reinforcing polymers, when the target molecules strongly quench fluorescence, holds much promise for developing fast detectors. 

The aim of this work was to study the influence of a second ligand, the concentration and nature of surfactants on flumequine-sensitized fluorescence of lanthanides and the usage of such a mixed-ligand complex for fluorimetric determination of flumequine in hen meat tissues. 

For an electron-transparent specimen the absorption and fluorescence correction parts can often be neglected, this is the so-called thin-film criterion introduced by Cliff and Lorimer [4.118]. Thus, for a thin specimen containing two elements A and B yielding the net X-ray intensities I a and 1b, the concentration ratio reduces to ... 

It is often experimentally convenient to use an analytical method that provides an instrumental signal that is proportional to concentration, rather than providing an absolute concentration, and such methods readily yield the ratio clc°. Solution absorbance, fluorescence intensity, and conductance are examples of this type of instrument response. The requirements are that the reactants and products both give a signal that is directly proportional to their concentrations and that there be an experimentally usable change in the observed property as the reactants are transformed into the products. We take absorption spectroscopy as an example, so that Beer s law is the functional relationship between absorbance and concentration. Let A be the reactant and Z the product. We then require that Ea ez, where e signifies a molar absorptivity. As initial conditions (t = 0) we set Ca = ca and cz = 0. The mass balance relationship Eq. (2-47) relates Ca and cz, where c is the product concentration at infinity time, that is, when the reaction is essentially complete. 

It is instructive to compare the sensitivity which may be achieved by absorption and fluorescence methods. The overall precision with which absorbance can be measured is certainly not better than 0.001 units using a 1 cm cell. Since for most molecules the value of emax is rarely greater than 105, then on the basis of the Beer-Lambert Law the minimum detectable concentration is given by cmin> 10 3/105= 10 8M. 

After the laser flash, one then monitors the progress of events by some rapidly responding method. Conductivity, absorption spectroscopy, and fluorescence spectroscopy are the methods most commonly used. If a reaction product has a characteristic absorption band of sufficient intensity, one can monitor its buildup with time. This might be a UV, visible, or IR band. The need for a band with a high molar absorptivity arises because the reactive transient is usually present at a relatively low concentration, KT6-lCr5 M being typical. If the species of interest is phosphorescent, then the timed decay of its phosphorescence intensity can be recorded. 

Fig. 2. Concentration changes of MB under UV-A (left) and fluorescent light (right) by untreated and H2+Ar plasma treated Xi02 films (blank refers to the reference line for the calibration of concentration changes due to the evaporation of water by lights during the measurements)...

The absorption and fluorescence spectra of a neat film made of RdB-den-drimer are shown in Fig. 2. The absorption spectrum in visible-wavelength region was similar to that obtained from a solution of RdB with a concentration less than 0.1 mmol/1. Interpretation of the fluorescence in terms of the Frank-Condon mechanism indicated that the core RdB chromophore behaved with a site-isolation effect and had little interaction with the neighboring chro-... 

Figure 4.4 Release of amino acids from cortical slices exposed to 50 mM K+. Measurements by HPEC and fluorescence detection after reaction of amino acids with o-phthalaldehyde 1, aspartate 2, glutamate 3, asparagine 4, serine 5, glutamine 6, histidine 7, homoserine (internal standard) 8, glycine 9, threonine 10, arginine 11, taurine 12, alanine 13, GABA 14, tyrosine. Glutamate concentration is almost 1 pmol/gl which represents a release rate of 30 pmol/min/mg tissue...

To quantify the concentration of a colorant, one must consider that linearity between the colorant concentration and the fluorescence emission intensity exists only at very low concentrations. The reason for deviation from linearity may be reabsorption of the emission light by other fluorophores or formation of dimers. If no extraction and controlled dilution of the fluorescent colorant are performed, the colorant quantification will be only qualitative. 

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