Refractive index detector. HPLC

Model RR/066 351 and 352 pumps models 750/16 variable-wavelength UV monitor detector 750/11 variable filter UV detector, MPD 880S multiwave plasma detector, 750/14 mass detector 750/350/06 electrochemical detector refractive index detector HPLC columns column heaters, autosamplers, pre-columns derivatization systems, solvent degassers, preparative HPLC systems... 

A comparative study of the analysis of aliphatic amines by GC-FID, GC-TSD and HPLC with refractive index detector (RID), using isopropylamine as internal standard, gave good results in all cases. Determination of trimethylamine oxide by HPLC with a pulsed amperometric detector was problematic136. 

Classical LC detectors (refractive index, fixed wavelength UV absorbance at 254 or 280 nm) have lacked the sensitivity to allow direct analysis of cannabi-noids in biological fluids. However, recent development of variable wavelength absorbance detectors extending into the 195-220nm UV region and of fluorescence detectors for HPLC led the authors to initiate... 

Figure 2. Typical response peaks for HPLC separation of saturates and aromatics. Column, 1-ft /i-PorasU soU vent, n-heptane (1 mL/min) sample, 10 fiL of vacuum gas oil in n-heptane detectors, refractive index, and Pye Unicam moving wire.

The first is a UV-vis-absorption or absorbance spectrophotometric (the phenomenon responsible for the signal is absorption, however, what is actually measured is absorbance, UV) detector. The second is a molecular fluorescence luminescence spectrophotometric (commonly called fluorescence, FL) detector. Other non-mass-spectrometric detectors designed for HPLC include refractive index (RI), electrochemical (EC), and of a more recent vintage, the light-scattering evaporative detector (LSED). RI and LSED HPLC detectors are not sensitive enough to meet the needs of TEQA. Electrochemical HPLC detectors have the required sensitivity, but due to frequent fowling of electrode surfaces they have not really found a place in TEQA. This author knows of no EPA methods as yet that incorporate EC HPLC detectors. For this reason, EC HPLC detectors will be not considered. 

Additional detectors available for HPLC analysis include fluorescence detectors, high-sensitivity diode-array detectors, refractive index detectors, and electrochemical detectors. 

Other widely used detectors for HPLC include refractive index (RI), fluorescence and evaporative light-scattering (ELS). The use of Rl and ELS detectors for pantothenic acid analysis in multivitamin dietary supplements has not been reported. The main reason is that the two detectors are not selective and thus cannot resolve pantothenic acid from other components existing in a multivitamin dietary supplement. Although fluorescence detection can be highly selective depending on the application, pantothenic acid does not have fluorescence excitation and emission and so fluorescence detection cannot be used for pantothenic acid analysis unless derivatization methods are applied (Pakin et al. 2004 Takahashi et al. 2009). Derivatization adds more complexity to analytical method and should not be used unless neeessary. For deteetion and quantitation of pantothenic add in multivitamin dietary supplements with HPLC/UHPLC, a highly selective detector such as MS should be the instrument of choice. 

Using these nanomaterials, an interesting example in the field, is the coupling of copper nanowires (CuNWs) to ME. Indeed, CuNWs exhibit electrocatalysis toward carbohydrates becoming a selective detector with the expected enhanced sensitivity. This coupling has been explored for the fast and reliable analysis of monosaccharides in honey samples [56]. To this end, a representative group of nine honey samples were analyzed and the results were compared with those obtained by HPLC-RI (refractive index). ME-CuNWs approach... 

Hplc techniques are used to routinely separate and quantify less volatile compounds. The hplc columns used to affect this separation are selected based on the constituents of interest. They are typically reverse phase or anion exchange in nature. The constituents routinely assayed in this type of analysis are those high in molecular weight or low in volatility. Specific compounds of interest include wood sugars, vanillin, and tannin complexes. The most common types of hplc detectors employed in the analysis of distilled spirits are the refractive index detector and the ultraviolet detector. Additionally, the recent introduction of the photodiode array detector is making a significant impact in the analysis of distilled spirits. 

For acrylate polymers with higher levels of carboxylic acids, THF can be modified by the addition of acids such as acetic, phosphoric, or trifluoroacetic. Levels as high as 10% acetic acid are considered acceptable by most manufacturers for their styrene/DVB columns. If such a modified mobile phase is used, it may need to be premixed rather than generated using a dynamic mixing HPLC pump because on-line mixing often leads to much noisier baselines, particularly when using a refractive index detector. 

Thin-layer chromatography (TLC) is used both for characterization of alcohol sulfates and alcohol ether sulfates and for their analysis in mixtures. This technique, combined with the use of scanning densitometers, is a quantitative analytical method. TLC is preferred to HPLC in this case as anionic surfactants do not contain strong chromophores and the refractive index detector is of low sensitivity and not suitable for gradient elution. A recent development in HPLC detector technology, the evaporative light-scattering detector, will probably overcome these sensitivity problems. 

Sodium dodecyl sulfate present in hydrophilic ointments has been determined by TLC on silica gel with flame ionization detection, which was considered better than the colorimetric method. TLC is preferred to HPLC in this case due to the low sensitivity of the refractive index detector that makes difficult the analysis of small amounts of sodium dodecyl sulfate [284]. 

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],... 

Solvent — The transition energy responsible for the main absorption band is dependent on the refractive index of the solvent, the transition energy being lower as the refractive index of the solvent increases. In other words, the values are similar in petroleum ether, hexane, and diethyl ether and much higher in benzene, toluene, and chlorinated solvents. Therefore, for comparison of the UV-Vis spectrum features, the same solvent should be used to obtain all carotenoid data. In addition, because of this solvent effect, special care should be taken when information about a chromophore is taken from a UV-Vis spectrum measured online by a PDA detector during HPLC analysis. 

Another variation of the preceding method is to apply HPLC to fractionate the cleaned-up aliphatic-aromatic fraction from flash colurim separation of soluble organic matter as it is performed in the Chevron laboratory, for example, as described in Reference 2. A Waters HPLC system equipped with a preparative Whatman Partisil 10 silica column (9.4 X 500 mm), a HPLC pump, and two detectors for separation monitoring (a UV and refractive index detector) are used, giving three fractions of aliphatic hydrocarbons, mono-, di-, and triaromatics and polar compounds. The hrst two fractions are eluted with hexane, whereas polar compounds are eluted with... 

Sample preparation, injection, calibration, and data collection, must be automated for process analysis. Methods used for flow injection analysis (FLA) are also useful for reliable sampling for process LC systems.1 Dynamic dilution is a technique that is used extensively in FIA.13 In this technique, sample from a loop or slot of a valve is diluted as it is transferred to a HPLC injection valve for analysis. As the diluted sample plug passes through the HPLC valve it is switched and the sample is injected onto the HPLC column for separation. The sample transfer time typically is determined with a refractive index detector and valve switching, which can be controlled by an integrator or computer. The transfer time is very reproducible. Calibration is typically done by external standardization using normalization by response factor. Internal standardization has also been used. To detect upsets or for process optimization, absolute numbers are not always needed. An alternative to... 

Specifications for modem detectors in HPLC are given by Hanai [538] and comprise spectroscopic detectors (UV, F, FUR, Raman, RID, ICP, AAS, AES), electrochemical detectors (polarography, coulometry, (pulsed) amperometry, conductivity), mass spectromet-ric and other devices (FID, ECD, ELSD, ESR, NMR). None of these detectors meets all the requirement criteria of Table 4.40. The four most commonly used HPLC detectors are UV (80%), electrochemical, fluorescence and refractive index detectors. As these detectors are several orders of magnitude less sensitive than their GC counterparts, sensor contamination is not so severe, and... 

Advances in size-exclusion chromatography, coupled with refractive index, absorption, viscosity, and lightscattering detectors, and MALDI-ToFMS, have made it possible to accurately determine molecular weight distribution (oligomer profiling), even at the relatively low values of polymeric additives (up to about 5000 Da). Advances in column design, e.g. high-resolution PS/DVB columns (> 105 plates m-1) mean that SEC can provide a valuable alternative to conventional HPLC techniques for the separation of small molecules. 

HPLC analysis for succinic acid, succinamic acid, succinamide, succinimide, N-methylsuccinimide, butyric acid, and propionic acid was performed with a Waters Model 515 HPLC pump equipped with a Waters Model 2410 Refractive Index Detector. Separations were performed with an Aminex HPX-87H 300mm column (Bio-Rad Laboratories, Hercules, CA) operated at 35°C, and using 0.005 M H2S04 elluent. 

Products were analyzed via Waters Model 515 HPLC Pump fitted with a Waters model 2410 refractive index detector. Separations was performed via an Aminex HP-87H 300mm column at 65°C using 0.005M H2SO4 as the mobile phase. Compounds calibrated for this work included xylitol, arabitol, erythritol, threitol, PG, EG, glycerol, lactate, 1-propanol, 2-propanol, ethanol, methanol, and the butanetriol isomers. Any compounds not visible by RID were not quantified in this work. 

The function of the detector in hplc is to monitor the mobile phase emerging from the column. The output of the detector is an electrical signal that is proportional to some property of the mobile phase and/or the solutes. Refractive index, for example, is a property of both the solutes and the mobile phase. A detector that measures such a property is called a bulk property detector. Alternatively, if the property is possessed essentially by the solute, such as absorption of uv/visible radiation or electrochemical activity, the detector is called a solute property detector. Quite a large number of devices, some of them rather complicated and tempremental, have been used as hplc detectors, but only a few have become generally useful, and we will examine five such types. Before doing this, it is helpful to have an idea of the sort of characteristics that are required of a detector. 

These detectors sense the difference in refractive index between the column eluent and a reference stream of pure mobile phase. They are the closest thing in hplc to a universal detector, as any solute can be detected as long as there is a difference in ri between the solute and the mobile phase. 

Detection in 2DLC is the same as encountered in one-dimensional HPLC. A variety of detectors are presented in Table 5.2. The choice of detector is dependent on the molecule being detected, the problem being solved, and the separation mode used for the second dimension. If MS detection is utilized, then volatile buffers are typically used in the second-dimension separation. Ultraviolet detection is used for peptides, proteins, and any molecules that contain an appropriate chromophore. Evaporative light scattering detection has become popular for the analysis of polymers and surfactants that do not contain UV chromophores. Refractive index (RI) detection is generally used with size exclusion chromatography for the analysis of polymers. 

The ideal HPLC detector should have the same characteristics as those required for GC detectors, i.e. rapid and reproducible response to solutes, a wide range of linear response, high sensitivity and stability of operation. No truly universal HPLC detector has yet been developed but the two most widely applicable types are those based on the absorption of UV or visible radiation by the solute species and those which monitor refractive index differences between solutes dissolved in the mobile phase and the pure mobile phase. Other detectors which are more selective in their response rely on such solute properties as fluorescence, electrical conductivity, diffusion currents (amperometric) and radioactivity. The characteristics of the various types of detector are summarized in Table 4.14. 

There are many HPLC detectors that can turn the presence of your compound into an electrical signal to be written on a chart recorder. Time was the refractive index detector was common. Clean eluent, used as a reference, went through one side of the detector, and the eluent with the samples went through the other side. A difference in the refractive index between the sample and reference caused an electrical signal to be generated and sent to a chart recorder. If you ve read the section on gas chromatography and looked ahead at infrared, you shouldn t be surprised to find both a sample and a reference. I did tell you the reference/sample pair is common in instrumentation. 

Five different detectors are common in HPLC (1) UV, (2) refractive index (RI), (3) conductivity, (4) inductively coupled plasma atomic emission, and (5) mass spectrometry. A UV detector passes a specific wavelength of UV light... 

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