Mass quantitation

Mass spectrometry Separation based on mass- Quantitative analysis [228, 229]... 

Determination of the CO2 content in Au/Zr02 andAu/Ti02 catalysts The quantitative interpretation of the TG curve is even more uncertain when the temperature ranges of the various decomposition stages overlap so that the specific stages of the decomposition are not discernible. Also, when the total mass change is below 1-2 mass%, quantitative interpretation is difficult due to the buoyancy effect. 

Mass spectrometry allows analysis by hydrocarbon family for a variety of petroleum cuts as deep as vacuum distillates since we have seen that the molecules must be vaporized. The study of vacuum residues can be conducted by a method of direct introduction which we will address only briefly because the quantitative aspects are ek r metiy difficult to master. Table 3.6 gives some examples the matrices used differ according to the distillation cut and the chemical content such as the presence or absence of olefins or sulfur. 

Transfer 30 g. of the hydrochloride to a 500 ml. separatory funnel, add 100 ml. of water and shake until a thin paste of uniform consistency is obtained add 10 per cent, aqueous sodium hydroxide solution in the cold with shaking until the whole mass has become bright green (the colour of the free base) and the mixture has an alkaUne reaction. Extract the free base by shaking with two 60 ml. portions of benzene (1). Dry the combined benzene extracts with a Uttle anhydrous potassium carbonate, and filter into a distiUing flask fitted with a water condenser. Distil off about half of the benzene, and pour the residual hot benzene solution into a beaker. Upon cooUng, the p-nitrosodimethylaniUne erystallises in deep green leaflets. Filter these off and dry them in the air. The yield of p-nitrosodimethylaniUne, m.p. 85°, from the hydrochloride is almost quantitative. 

Place a mixture of 30 g. of 3 5-dinitrobenzoic acid (Section IV,168 and 33 g. of phosphorus pentachloride in a Claisen flask fit a reflux condenser into the short neck and cork the other neck and side arm (compare Fig. Ill, 31, 1). Heat the mixture in an oil bath at 120-130° for 75 minutes. Allow to cool. Remove the phosphorus oxychloride by distillation under reduced pressure (25°/20 mm.) raise the temperature of the bath to 110°. The residual 3 5-dinitrobenzoyl chloride solidifies on cooling to a brown mass the yield is quantitative. Recrystallise from carbon tetrachloride the yield is 25 g., m.p. 67-68° and this is satisfactory for most purposes. Further recrystallisation from a large volume of light petroleum b.p. 40-60°, gives a perfectly pure product, m.p. 69 -6°. 

The amino add analysis of all peptide chains on the resins indicated a ratio of Pro Val 6.6 6.0 (calcd. 6 6). The peptides were then cleaved from the resin with 30% HBr in acetic acid and chromatogra phed on sephadex LH-20 in 0.001 M HCl. 335 mg dodecapeptide was isolated. Hydrolysis followed by quantitative amino acid analysis gave a ratio of Pro Val - 6.0 5.6 (calcd. 6 6). Cycll2ation in DMF with Woodward s reagent K (see scheme below) yielded after purification 138 mg of needles of the desired cyc-lododecapeptide with one equiv of acetic add. The compound yielded a yellow adduct with potassium picrate, and here an analytically more acceptable ratio Pro Val of 1.03 1.00 (calcd. 1 1) was found. The mass spectrum contained a molecular ion peak. No other spectral measurements (lack of ORD, NMR) have been reported. For a thirty-six step synthesis in which each step may cause side-reaaions the characterization of the final product should, of course, be more elaborate. 

You should be able to describe a system at equilibrium both qualitatively and quantitatively. Rigorous solutions to equilibrium problems can be developed by combining equilibrium constant expressions with appropriate mass balance and charge balance equations. Using this systematic approach, you can solve some quite complicated equilibrium problems. When a less rigorous an-... 

Caffeine is extracted from beverages by a solid-phase microextraction using an uncoated fused silica fiber. The fiber is suspended in the sample for 5 min and the sample stirred to assist the mass transfer of analyte to the fiber. Immediately after removing the fiber from the sample it is transferred to the gas chromatograph s injection port where the analyte is thermally desorbed. Quantitation is accomplished by using a C3 caffeine solution as an internal standard. 

Quantitative Calculations In precipitation gravimetry the relationship between the analyte and the precipitate is determined by the stoichiometry of the relevant reactions. As discussed in Section 2C, gravimetric calculations can be simplified by applying the principle of conservation of mass. The following example demonstrates the application of this approach to the direct analysis of a single analyte. 

A second approach to gravimetry is to thermally or chemically decompose a solid sample. The volatile products of the decomposition reaction may be trapped and weighed to provide quantitative information. Alternatively, the residue remaining when decomposition is complete may be weighed. In thermogravimetry, which is one form of volatilization gravimetry, the sample s mass is continuously monitored while the applied temperature is slowly increased. 

Several standard methods for the quantitative analysis of food samples are based on measuring the sample s mass following a selective solvent extraction. For example, the crude fat content in chocolate can be determined by extracting with ether for 16 h in a Soxhlet extractor. After the extraction is complete, the ether is allowed to evaporate, and the residue is weighed after drying at 100 °C. This analysis has also been accomplished indirectly by weighing a sample before and after extracting with supercritical GO2. 

In a gravimetric analysis a measurement of mass or change in mass provides quantitative information about the amount of analyte in a sample. The most common form of gravimetry uses a precipitation reaction to generate a product whose mass is proportional to the analyte. In many cases the precipitate includes the analyte however, an indirect analysis in which the analyte causes the precipitation of another compound also is possible. Precipitation gravimetric procedures must be carefully controlled to produce precipitates that are easily filterable, free from impurities, and of known stoichiometry. 

Isotope Dilution Another important quantitative radiochemical method is isotope dilution. In this method of analysis a sample of analyte, called a tracer, is prepared in a radioactive form with a known activity. Ax, for its radioactive decay. A measured mass of the tracer, Wf, is added to a sample containing an unknown mass, w, of a nonradioactive analyte, and the material is homogenized. The sample is then processed to isolate wa grams of purified analyte, containing both radioactive and nonradioactive materials. The activity of the isolated sample, A, is measured. If all the analyte, both radioactive and nonradioactive, is recovered, then A and Ax will be equal. Normally, some of the analyte is lost during isolation and purification. In this case A is less than Ax, and... 

Mixtures passed through special columns (chromatography) in the gas phase (GC) or liquid phase (LC) can be separated into their individual components and analyzed qualitatively and/or quantitatively. Both GC and LC analyzers can be directly coupled to mass spectrometers, a powerful combination that can simultaneously separate and identify components of mixtures. 

Mass analysis. A process by which a mixture of ionic (or neutral) species is separated according to the mass-to-charge (m/z) ratios (for ions) or their aggregate atomic masses (for neutrals). The analysis can be qualitative or quantitative. 

Millard, B.J., Quantitative Mass Spectrometry, Heyden, London, 1978. 

The elasticity of a fiber describes its abiUty to return to original dimensions upon release of a deforming stress, and is quantitatively described by the stress or tenacity at the yield point. The final fiber quaUty factor is its toughness, which describes its abiUty to absorb work. Toughness may be quantitatively designated by the work required to mpture the fiber, which may be evaluated from the area under the total stress-strain curve. The usual textile unit for this property is mass pet unit linear density. The toughness index, defined as one-half the product of the stress and strain at break also in units of mass pet unit linear density, is frequentiy used as an approximation of the work required to mpture a fiber. The stress-strain curves of some typical textile fibers ate shown in Figure 5. 

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