Desolvate

The direct ligand-protein interactions and the net solvation-desolvation term together should give an energy contribution that strongly favors formation of the complex (large and negative), since the other two components favor its dissociation. 

Rognan published the scoring function FRESNO (fast free energy scoring function), which considers a hydrogen-bond term, a lipophilic terra, a repulsive term for the buried polar surface, a rotational term, and a desolvation terra [82]. 

Constanciel R and R Contreras 1984. Self-Consistent Field Theory of Solvent Effects Representation by Continuum Models - Introduction of Desolvation Contribution. Theoretica Chimica Acta 65 1-11. 

Jones G, P Willett and R C Glen 1995b. Molecular Recognition of Receptor Sites Using a Geneti Algorithm with a Description of Desolvation. Journal of Molecular Biology 245 43-53. 

Interactions between nonpolar compounds are generally stronger in water than in organic solvents. At concentrations where no aggregation or phase separation takes place, pairwise hydrophobic interactions can occur. Under these conditions, the lowest energy state for a solute molecule is the one in which it is completely surrounded by water molecules. However, occasionally, it will also meet other solute molecules, and form short-lived encounter complexes. In water, the lifetime of these complexes exceeds that in organic solvents, since the partial desolvation that accompanies the formation of these complexes is less unfavourable in water than in organic solvents. 

For the chromatographic column, flow of solution from the narrow inlet tube into the ionization/desolvation region is measured in terms of only a few microliters per minute. Under these circumstances, spraying becomes very easy by application of a high electrical potential of about 3-4 kV to the end of the nanotube. Similarly, spraying from any narrow capillary is also possible. The ions formed as part of the spraying process follow Z-shaped trajectories, as discussed below. 

A typical arrangement for producing a particle beam from a stream of liquid, showing (1) the nebulizer, (2) the desolvation chamber, (3) the wall heater, (4) the exit nozzle, (5, 6) skimmers 1, 2, (7) the end of the ion source, (8) the ion source, and (9) the mass analyzer. An optional GC inlet into the ion source is shown. 

Suitable inlets commonly used for liquids or solutions can be separated into three major classes, two of which are discussed in Parts A and C (Chapters 15 and 17). The most common method of introducing the solutions uses the nebulizer/desolvation inlet discussed here. For greater detail on types and operation of nebulizers, refer to Chapter 19. Note that, for all samples that have been previously dissolved in a liquid (dissolution of sample in acid, alkali, or solvent), it is important that high-purity liquids be used if cross-contamination of sample is to be avoided. Once the liquid has been vaporized prior to introduction of residual sample into the plasma flame, any nonvolatile impurities in the liquid will have been mixed with the sample itself, and these impurities will appear in the results of analysis. The problem can be partially circumvented by use of blanks, viz., the separate examination of levels of residues left by solvents in the absence of any sample. 

The nebulization concept has been known for many years and is commonly used in hair and paint spays and similar devices. Greater control is needed to introduce a sample to an ICP instrument. For example, if the highest sensitivities of detection are to be maintained, most of the sample solution should enter the flame and not be lost beforehand. The range of droplet sizes should be as small as possible, preferably on the order of a few micrometers in diameter. Large droplets contain a lot of solvent that, if evaporated inside the plasma itself, leads to instability in the flame, with concomitant variations in instrument sensitivity. Sometimes the flame can even be snuffed out by the amount of solvent present because of interference with the basic mechanism of flame propagation. For these reasons, nebulizers for use in ICP mass spectrometry usually combine a means of desolvating the initial spray of droplets so that they shrink to a smaller, more uniform size or sometimes even into small particles of solid matter (particulates). 

These factors make it necessary to reduce the amount of solvent vapor entering the flame to as low a level as possible and to make any droplets or particulates entering the flame as small and of as uniform a droplet size as possible. Desolvation chambers are designed to optimize these factors so as to maintain a near-constant efficiency of ionization and to flatten out fluctuations in droplet size from the nebulizer. Droplets of less than 10 pm in diameter are preferred. For flow rates of less than about 10 pl/min issuing from micro- or nanobore liquid chromatography columns, a desolvation chamber is unlikely to be needed. 

The simplest desolvation chambers consist simply of a tube heated to about 150°C through which the spray of droplets passes. During passage through this heated region, solvent evaporates rapidly from the droplets and forms vapor. The mixed vapor and residual small droplets or particulates of sample matter are swept by argon through a second cooled tube, which allows vapor to... 

A second form of desolvation chamber relies on diffusion of small vapor molecules through pores in a Teflon membrane in preference to the much larger droplets (molecular agglomerations), which are held back. These devices have proved popular with thermospray and ultrasonic nebulizers, both of which produce large quantities of solvent and droplets in a short space of time. Bundles of heated hollow polyimide or Naflon fibers have been introduced as short, high-surface-area membranes for efficient desolvation. 

Solutions can be examined by ICP/MS by (a) removing the solvent (direct and electrothermal methods) and then vaporizing residual sample solute or (b) nebulizing the sample solution into a spray of droplets that is swept into the plasma flame after passing through a desolvation chamber, where excess solvent is removed. The direct and electrothermal methods are not as convenient as the nebulization inlets for multiple samples, but the former are generally much more efficient in transferring samples into the flame for analysis. 

An aerosol produced instrumentally has similar properties, except that the aerosol is usually produced from solutions and not from pure liquids. For solutions of analytes, the droplets consist of solute and solvent, from which the latter can evaporate to give smaller droplets of increasingly concentrated solution (Figure 19.1). If the solvent evaporates entirely from a droplet, the desolvated dry solute appears as small solid particles, often simply called particulate matter. 

The calculation shows how rapidly a droplet changes in diameter with time as it flows toward the plasma flame. At 40°C, a droplet loses 90% of its size within alxtut 1.5 sec, in which time the sweep gas has flowed only about 8 cm along the tube leading to the plasma flame. Typical desolvation chambers operate at 150°C and, at these temperatures, similar changes in diameter will be complete within a few milliseconds. The droplets of sample solution lose almost all of their solvent (dry out) to give only residual sample (solute) particulate matter before reaching the plasma flame. 

Many designs of nebulizer are commonly used in ICP/MS, but their construction and mode of operation can be collated into a small number of groups pneumatic, ultrasonic, thermospray, APCI, and electrospray. These different types are discussed in the following sections, which are followed by further sections on spray and desolvation chambers. 

In a concentric-tube nebulizer, the sample solution is drawn through the inner capillary by the vacuum created when the argon gas stream flows over the end (nozzle) at high linear velocity. As the solution is drawn out, the edges of the liquid forming a film over the end of the inner capillary are blown away as a spray of droplets and solvent vapor. This aerosol may pass through spray and desolvation chambers before reaching the plasma flame. 

The thermospray device produces a wide dispersion of droplet sizes and transfers much of sample solution in unit time to the plasma flame. Therefore, it is essential to remove as great a proportion of the bigger droplets and solvent as possible to avoid compromising the flame performance. Consequently, the thermospray device usually requires both spray and desolvation chambers, especially for analyte solutions in organic solvents. 

Thermospray nebulizers are somewhat expensive but can be used on-line to a liquid chromatographic column. About 10% of sample solution is transferred to the plasma flame. The overall performance of the thermospray device compares well with pneumatic and ultrasonic sprays. When used with microbore liquid chromatographic columns, which produce only about 100 pl/min of eluant, the need for spray and desolvation chambers is reduced, and detection sensitivities similar to those of the ultrasonic devices can be attained both are some 20 times better than the sensitivities routinely found in pneumatic nebulizers. 

Having removed the larger droplets, it may remain only to encourage natural evaporation of solvent from the remaining small droplets by use of a desolvation chamber. In this chamber, the droplets are heated to temperatures up to about 150 C, often through use of infrared heaters. The extra heat causes rapid desolvation of the droplets, which frequently dry out completely to leave the analyte as small particles that are swept by the argon flow into the flame. 

Having assisted desolvation in this way, the carrier gas then carries solvent vapor produced in the initial nebulization with more produced in the desolvation chamber. The relatively large amounts of solvent may be too much for the plasma flame, causing instability in its performance and, sometimes, putting out the flame completely. Therefore, the desolvation chamber usually contains a second section placed after the heating section. In this second part of the desolvation chamber, the carrier gas and entrained vapor are strongly cooled to temperatures of about 0 to -10 C. Much of the vapor condenses out onto the walls of the cooled section and is allowed to drain away. Since this drainage consists only of solvent and not analyte solution, it is normally directed to waste. 

Introduction of sample solution via a nebulizer may need both spray and a desolvation chamber, but a well-designed, efficient nebulizer needs neither. 

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