UV/fluorescence detector

Coproporphyrinogen I was separated from other assay components by chromatography on a Partisil 5 column (4.6 mm x 250 mm) column. The mobile phase was composed of heptane-ethyl acetate-dichloromethane-methanol (60 25 14 1). Quantitation was by a UV fluorescence detector (excitation, 405 nm detection, 605 nm). At a flow rate of 1.1 mL/min, the... 

BAWS The bio-aerosol warning sensor (BAWS) is an ultraviolet (UV) fluorescence detector using laser illumination. BAWS units are planned to be integrated into the joint biological point detection system (JBPDS) as a trigger for the presence of a 1- to 10-micron-sized biological particle. 

UV Fluorescence Detector—A qualitative and quantitative detector capable of measuring Ugbt emitted from the fluorescence of sulfur dioxide by UV light. 

Note that in liquid phase chromatography there are no detectors that are both sensitive and universal, that is, which respond linearly to solute concentration regardless of its chemical nature. In fact, the refractometer detects all solutes but it is not very sensitive its response depends evidently on the difference in refractive indices between solvent and solute whereas absorption and UV fluorescence methods respond only to aromatics, an advantage in numerous applications. Unfortunately, their coefficient of response (in ultraviolet, absorptivity is the term used) is highly variable among individual components. 

Despite their importance, gas chromatography and liquid chromatography cannot be used to separate and analyze all types of samples. Gas chromatography, particularly when using capillary columns, provides for rapid separations with excellent resolution. Its application, however, is limited to volatile analytes or those analytes that can be made volatile by a suitable derivatization. Liquid chromatography can be used to separate a wider array of solutes however, the most commonly used detectors (UV, fluorescence, and electrochemical) do not respond as universally as the flame ionization detector commonly used in gas chromatography. 

In hplc, detection and quantitation have been limited by availabiHty of detectors. Using a uv detector set at 254 nm, the lower limit of detection is 3.5 X 10 g/mL for a compound such as phenanthrene. A fluorescence detector can increase the detectabiHty to 8 x 10 g/mL. The same order of detectabiHty can be achieved using amperometric, electron-capture, or photoioni2ation detectors. 

Colorless substances absorb at wavelengths shorter than those of the visible range (the UV range normally amenable to analysis X = 400...200 nm). Such compounds can be detected by the use of UV-sensitive detectors (photomultipliers. Sec. 2.2.3.1). Substances that absorb in the UV range and are stimulated to fluorescence or phosphorescence (luminescence) can be detected visually if they are irradiated with UV light. 

Reagents which form a derivative that strongly absorbs UV/visible radiation are called chromatags an example is the reagent ninhydrin, commonly used to obtain derivatives of amino acids which show absorption at about 570 nm. Derivatisation for fluorescence detectors is based on the reaction of non-fluorescent reagent molecules (fluorotags) with solutes to form fluorescent... 

The pressure sensitivity of a detector will be one of the factors that determines the long term noise and thus can be very important. It is usually measured as the change in detector output for unit change in sensor-cell pressure. Pressure sensitivity and flow sensitivity are to some extent interdependent, subject to the manner in which the detector functions. The UV detector, the fluorescence detector and the electrical... 

The popularity of the UV detector, the electrical conductivity detector and the fluorescence detector motivated Schmidt and Scott (5,6) to develop a trifunctional detector that detected solutes by all three methods simultaneously in a single low volume cell. 

Chromatograms demonstrating the simultaneous use of all three detector functions are shown in figure 22. It is seen that the anthracene is clearly picked out from the mixture of aromatics by the fluorescence detector and the chloride ion, not shown at all by the UV adsorption or fluorescence detectors, clearly shown by the electrical conductivity detector. 

The aromatic nucleus adsorbs in the UV and thus, the derivative can be detected by a UV detector. This is the most common type of chemical derivatization but the derivative may be chosen to be appropriate for different types of detector. For example, the solute can be reacted with a fluorescing reagent, producing a fluorescent derivative and thus be detectable by the fluorescence detector. Alternatively, a derivative can be made that is easily oxidized and, consequently, would be detectable by an electrochemical detector. 

The choice of detector is often crucial to the success of a particular HPLC method. A number are in routine use, including the UV, fluorescence, electrochemical, conductivity and refractive index detectors, and each has particular advantages and disadvantages, details of which can be found elsewhere [2-4],... 

Similarly to the methods used to characterize natural chlorophylls, RP-HPLC has been chosen by several authors to identify the individual components in Cn chlorophyllin preparations and in foods. The same ODS columns, mobile phase and ion pairing or ion suppressing techniques coupled to online photodiode UV-Vis and/or fluorescence detectors have been used. ° ... 

The detection of the migrating sample boundary in CE can be accomplished by UV, fluorescent, electrochemical, radiochemical, conductivity, and mass spectrometry (MS) means. The use of high-sensitivity detection systems is always a key issue in CE applications. The sensitivity of HPCE detectors may be at least 2 to 3 orders of magnitude better than that of HPLC detectors. Since the detection cell volume is very small, the concentration sensitivity... 

In order to achieve detection limits below the ng mL-1 range only amperometric, chemiluminescence, radiometric, or conventional fluorescence (CF) can be applied (Table 4.41). Fluorescence detectors are generally about 100 times more sensitive and more selective than UV detectors. The selectivity of fluorescence detection is due to the fact that only aromatic and conjugated molecules can be analysed, and by applying specific excitation and emission wavelengths the selectivity can even be increased. Pre- or postcolumn derivatisation in HPLC is a technique that is most commonly performed prior to UV absorption or fluorescence detection... 

Fluorescence is much more widely used for analysis than phosphorescence. Yet, the use of fluorescent detectors is limited to the restricted set of additives with fluorescent properties. Fluorescence detection is highly recommended for food analysis (e.g. vitamins), bioscience applications, and environmental analysis. As to poly-mer/additive analysis fluorescence and phosphorescence analysis of UV absorbers, optical brighteners, phenolic and aromatic amine antioxidants are most recurrent [25] with an extensive listing for 29 UVAs and AOs in an organic solvent medium at r.t. and 77 K by Kirkbright et al. [149]. 

High Performance Liquid Chromatographic (HPLC) Analysis. A Waters HPLC system (two Waters 501 pumps, automated gradient controller, 712 WISP, and 745 Data module) with a Shimadzu RF-535 fluorescence detector or a Waters 484 UV detector, and a 0.5 pm filter and a Rainin 30 x 4.6 mm Spheri-5 RP-18 guard column followed by a Waters 30 x 3.9 cm (10 pm particle size) p-Bondapak C18 column was used. The mobile phase consisted of a 45% aqueous solution (composed of 0.25% triethylamine, 0.9% phosphoric acid, and 0.01% sodium octyl sulfate) and 55% methanol for prazosin analysis or 40% aqueous solution and 60% methanol for naltrexone. The flow rate was 1.0 mL/min. Prazosin was measured by a fluorescence detector at 384 nm after excitation at 340 nm (8) and in vitro release samples of naltrexone were analyzed by UV detection at 254 nm. 

Fluorescence detectors can be made much more sensitive than uv absorbance detectors for favourable solutes (such as anthracene) the noise equivalent concentration can be as low as 10 12 g cm-3. Because both the excitation wavelength and the detected wavelength can be varied, the detector can be made highly selective, which can be very useful in trace analysis. The response of the detector is linear provided that no more than about 10% of the incident radiation is absorbed by the sample. This results in a linear range of 103-104. 

One type of ec detector (the coulometric detector) reacts all of the electroactive solute passing through it. This type has never become very popular (there is only one on the market at the moment). Another type (the amperometric detector) reacts a much smaller quantity of the solute, less than 1%. The currents observed with these detectors are very small (nanoamps), but such currents are not too difficult to measure and the detector has a high sensitivity, considerably higher than that of uv/visible absorbance detectors although not as good as fluorescence detectors. Noise equivalent concentrations of about 10, 0g cm-3 have been obtained in favourable cases. Another advantage of these detectors is that they can be made with a very small internal volume. 

The experiment is performed with a spectrofluorometer similar to the ones used for linear fluorescence and quantum yield measurements (Sect. 2.1). The excitation, instead of a regular lamp, is done using femtosecond pulses, and the detector (usually a photomultiplier tube or an avalanche photodiode) must either have a very low dark current (usually true for UV-VIS detectors but not for the NIR), or to be gated at the laser repetition rate. Figure 11 shows a simplified schematic for the 2PF technique. 

---