Thin Layer Chromatography

differently between two phases, a mobile phase and a stationary phase. You have already had some

experience with gas chromatography where the mobile phase is an inert gas, usually helium, and the

stationary phase is a high boiling liquid coating absorbed on the surface of a granular solid in a column. In

thin layer chromatography, or TLC, the mobile phase is a liquid and the stationary phase is a solid

absorbent.

Theory of Thin Layer Chromatography

In thin layer chromatography, a solid phase, the adsorbent, is coated onto a solid support as a thin

layer (about 0.25 mm thick). In many cases, a small amount of a binder such as plaster of Paris is mixed

with the absorbent to facilitate the coating. Many different solid supports are employed, including thin

sheets of glass, plastic, and aluminum. The mixture (A plus B) to be separated is dissolved in a solvent and

the resulting solution is spotted onto the thin layer plate near the bottom. A solvent, or mixture of solvents,

called the eluant, is allowed to flow up the plate by capillary action. At all times, the solid will adsorb a

certain fraction of each component of the mixture and the remainder will be in solution. Any one molecule

will spend part of the time sitting still on the adsorbent with the remainder moving up the plate with the

solvent. A substance that is strongly adsorbed (say, A) will have a greater fraction of its molecules

adsorbed at any one time, and thus any one molecule of A will spend more time sitting still and less time

moving. In contrast, a weakly adsorbed substance (B) will have a smaller fraction of its molecules

adsorbed at any one time, and hence any one molecule of B will spend less time sitting and more time

moving. Thus, the more weakly a substance is adsorbed, the farther up the plate it will move. The more

strongly a substance is adsorbed, the closer it will stays near the origin.

Several factors determine the efficiency of a chromatographic separation. The adsorbent should show

a maximum of selectivity toward the substances being separated so that the differences in rate of elution

will be large. For the separation of any given mixture, some adsorbents may be too strongly adsorbing or

too weakly adsorbing. Table 1 lists a number of adsorbents in order of adsorptive power.

Table 1. Chromatographic adsorbents. The order in the table is approximate, since it depends upon the

substance being adsorbed, and the solvent used for elution.

Most Strongly Adsorbent Alumina Al2O3

Charcoal C

Florisil MgO/SiO2 (anhydrous)

Least Strongly Adsorbent Silica gel SiO2

The eluting solvent should also show a maximum of selectivity in its ability to dissolve or desorb the

substances being separated. The fact that one substance is relatively soluble in a solvent can result in its

being eluted faster than another substance. However, a more important property of the solvent is its ability

to be itself adsorbed on the adsorbent. If the solvent is more strongly adsorbed than the substances being

separated, it can take their place on the adsorbent and all the substances will flow together. If the solvent is

less strongly adsorbed than any of the components of the mixture, its contribution to different rates of

elution will be only through its difference in solvent power toward them. If, however, it is more, strongly

adsorbed than some components of the mixture and less strongly than others, it will greatly speed the

elution of those substances that it can replace on the absorbent, without speeding the elution of the others.

Table 2 lists a number of common solvents in approximate order of increasing adsorbability, and hence

in order of increasing eluting power. The order is only approximate since it depends upon the nature of the

adsorbent. Mixtures of solvents can be used, and, since increasing eluting power results mostly from

preferential adsorbtion of the solvent, addition of only a little (0.5-2%, by volume) of a more strongly

adsorbed solvent will result in a large increase in the eluting power. Because water is among the most

strongly adsorbed solvents, the presence of a little water in a solvent can greatly increase its eluting power.

For this reason, solvents to be used in chromatography should be quite dry. The particular combination of

adsorbent and eluting solvent that will result in the acceptable separation of a particular mixture can be

determined only by trial.

Table 2. Eluting solvents for chromatography

Least Eluting Power (alumina as adsorbent) Petroleum ether (hexane; pentane)

Cyclohexane

Carbon tetrachloride

Benzene

DichIoromethane

Chloroform

Ether (anhydrous)

Ethyl acetate (anhydrous)

Acetone (anhydrous)

Ethanol

Methanol

Water

Pyridine

Greatest Eluting Power (alumina as adsorbent) Organic acids

If the substances in the mixture differ greatly in adsorbability, it will be much easier to separate them.

Often, when this is so, a succession of solvents of increasing eluting power is used. One substance may be

eluted easily while the other stays at the top of the column, and then the other can be eluted with a solvent

of greater eluting power. Table 3 indicates an approximate order of adsorbability by functional group.

Table 3. Adsorbability of organic compounds by functional group

Least Strongly Adsorbed Saturated hydrocarbons; alkyl halides

Unsaturated hydrocarbons; aIkenyl halides

Aromatic hydrocarbons; aryl halides

Polyhalogenated hydrocarbons

Ethers

Esters

Aldehydes and ketones

Alcohols

Most Strongly Adsorbed Acids and bases (amines)

Technique of Thin-layer Chromatography

The sample is applied to the layer of adsorbent, near one edge, as a small spot of a solution. After the

solvent has evaporated, the adsorbent-coated sheet is propped more or less vertically in a closed container,

with the edge to which the spot was applied down. The spot on the thin layer plate must be positioned

above the level of the solvent in the container (Figure 24). If it is below the level of the solvent, the spot

will be washed off the plate into the developing solvent. The solvent, which is in the bottom of the

container, creeps up the layer of adsorbent, passes over the spot, and, as it continues up, effects a separation

of the materials in the spot ("develops" the chromatogram). When the solvent front has nearly reached

nearly the top of the adsorbent, the thin layer plate is removed from the container (Figure 25).

Figure 24. Position of the spot on a thin layer plate.

Since the amount of adsorbent involved is relatively small, and the ratio of adsorbent to sample must

be high, the amount of sample must be very small, usually much less than a milligram. For this reason,

thin-layer chromatography (TLC) is usually used as an analytical technique rather than a preparative

method. With thicker layers (about 2 mm) and large plates with a number of spots or a stripe of sample, it

can be used as a preparative method. The separated substances are recovered by scraping the adsorbent off

the plate (or cutting out the spots if the supporting material can be cut) and extracting the substance from

the adsorbent.

Figure 25. TLC plate showing distances traveled by the spot and the solvent after solvent front nearly

reached the top of the adsorbent.

Because the distance traveled by a substance relative to the distance traveled by the solvent front

depends upon the molecular structure of the substance, TLC can be used to identify substances as well as to

separate them. The relationship between the distance traveled by the solvent front and the substance is

usually expressed as the Rf value:

Rf value = distance traveled by substance

distance traveled by solvent front)

The Rf values are strongly dependent upon the nature of the adsorbent and solvent. Therefore,

experimental Rf values and literature values do not often agree very well. In order to determine whether an

unknown substance is the same as a substance of known structure, it is necessary to run the two substances

side by side in the same chromatogram, preferably at the same concentration.

Application of the Sample

The sample to be separated is generally applied as a small spot (1 to 2 mm diameters) of solution about

1 cm from the end of the plate opposite the handle. The addition may be made with a micropipet prepared

by heating and drawing out a melting point capillary. As small a sample as possible should be used, since

this will minimize tailing and overlap of spots; the lower limit is the ability to visualize the spots in the

developed chromatogram. If the sample solution is very dilute, make several small applications in the same

place, allowing the solvent to evaporate between additions. Do not disturb the adsorbent when you make

the spots, since this will result in an uneven flow of the solvent. The starting position can be indicated by

making a small mark near the edge of the plate.

Development of thin layer plates

The chamber used for development of the chromatogram (Figure 26) can be as simple as a beaker

covered with a watch glass, or a cork-stoppered bottle. The developing solvent (an acceptable solvent or

mixture of solvents must be determined by trial) is poured into the container to a depth of a few

millimeters. The spotted plate is then placed in the container, spotted end down; the solvent level must be

below the spots (see figure below). The solvent will then slowly rise in the adsorbent by capillary action.

Figure 26. Developing chamber for thin layer chromatogram.

In order to get reproducible results, the atmosphere in the development chamber must be saturated with

the solvent. This can be accomplished by sloshing the solvent around in the container before any plates

have been added. The atmosphere in the chamber is then kept saturated by keeping the container closed all

the time except for the brief moment during which a plate is added or removed.

Visualization

When the solvent front has moved to within about 1 cm of the top end of the adsorbent (after 15 to 45

minutes), the plate should be removed from the developing chamber, the position of the solvent front

marked, and the solvent allowed to evaporate. If the components of the sample are colored, they can be

observed directly. If not, they can sometimes be visualized by shining ultraviolet light on the plate (Figure

27) or by allowing the plate to stand for a few minutes in a closed container in which the atmosphere is

saturated with iodine vapor. Sometimes the spots can be visualized by spraying the plate with a reagent

that will react with one or more of the components of the sample.

Figure 27. Two ways of using UV light to visualize the spots

General preparation of materials

• The thin layer chromatography plates are commercial pre-prepared ones with a silica gel layer on a glass,

plastic, or aluminum backing. Use the wide plates for spotting several compounds on the same plate. This

allows for more precise comparison of the behavior of the compounds.

• The samples are spotted on the thin layer plates using fine capillaries drawn from melting point

capillaries. You will need to draw several spotters. Your teaching assistant will demonstrate the technique

(mystical art?) of drawing capillaries.

• Samples for spotting are prepared by dissolving approximately 0.1 g (the amount on the tip of a spatula)

of the compound in less than 0.5 mL of a solvent (ethyl acetate, dichloromethane, or ether work well).

• When spotting samples on the TLC plates, it is a good idea to check if enough sample has been spotted

on the plate. Allow the solvent to evaporate and then place the plate under a short wavelength ultraviolet

lamp. A purple spot on a background of green should be clearly visible. If the spot is faint or no spot is

apparent, more sample will have to be applied to the plate.

• The chromatograms are developed in a 150-mL beaker or jar containing the developing solvent. The

beaker is covered with a small watch glass. A wick made from a folded strip of filter paper is used to keep

the atmosphere in the beaker saturated with solvent vapor.

• When the plates are removed from the developing solvent, the position of the solvent front is marked, and

the solvent is allowed to evaporate. The positions of the spots are determined by placing the plates under a

short wavelength ultraviolet lamp. The silica gel is mixed with an inorganic phosphor which fluoresces

green in the UV light. Where there are compounds on the plates, the fluorescence is quenched and a dark

purple spot appears.