Chromatography is a family of analytical chemistry techniques for the separation of mixtures. It involves passing the sample, a mixture which contains the analyte, in the "mobile phase", often in a stream of solvent, through the "stationary phase." The stationary phase retards the passage of the components of the sample. When components pass through the system at different rates they become separated in time, like runners in a mass-start foot race. Each component has a characteristic time of passage through the system, called a "retention time." Chromatographic separation is achieved when the retention time of the analyte differs from that of other components in the sample. Analytical chemistry is the analysis of material samples to gain an understanding of their chemical composition and structure. ... In chemistry and chemical engineering, a separation process is a process that transforms a mixture of substances into two or more compositionally-distinct products. ... An Analyte is the substance or chemical constituent that is undergoing analysis. ... A solvent is a liquid that dissolves a solid, liquid, or gaseous solute, resulting in a solution. ... An Analyte is the substance or chemical constituent that is undergoing analysis. ...

A chromatograph takes a chemical mixture carried by liquid or gas and separates it into its component parts as a result of differential distributions of the solutes as they flow around or over a stationary liquid or solid phase. Various techniques for the separation of complex mixtures rely on the differential affinities of substances for a gas or liquid mobile medium and for a stationary absorbing medium through which they pass; such as paper, gelatin, or magnesium silicate gel. A liquid will assume the shape of its container. ... A gas is one of the four main phases of matter (after solid and liquid, and followed by plasma), that subsequently appear as a solid material that is subjected to increasingly higher temperatures. ... A substance is soluble in a fluid if it dissolves in the fluid. ... Absorption has a number of meanings: In physics, absorption is a process in which particles of some sort encounter another material and are taken up by or even disappear in it. ... This article needs to be cleaned up to conform to a higher standard of quality. ... Gelatin (also gelatine) is a translucent brittle solid substance, colorless or slightly yellow, nearly tasteless and odorless, which is created by prolonged boiling of animal skin and connective tissue. ...

Analytical chromatography is used to determine the identity and concentration of molecules in a mixture. Preparative chromatography is used to purify larger quantities of a molecular species. Most of the following refers to analytical chromatography.

History

It was the Russian botanist Mikhail Tsvet (Mikhail Semyonovich Tsvet) who invented the first chromatography technique in 1901 during his research on chlorophyll. He used liquid-adsorption columns to separate plant pigments. The method was described on December 30, 1901 at the XI Congress of Naturalists and Doctors (XI съезд естествоиспытателей и врачей) in St.Petersburg. The first printed description was in 1903, in the Proceedings of the Warsaw Society of Naturalists, section of biology. He first used the term chromatography in print in 1906 in his two papers about chlorophyll in the German botanical journal, Berichte der Deutschen botanischen Geselschaft. In 1907 he demonstrated his chromatogaph for the German Botanical Society. The phenomenon of precipitational separation was observed before Tsvet as well. His contribution was turning the phenomenon into the method of scientific analysis. Botany is the scientific study of plant life. ... Mikhail Semyonovich Tsvet (Михаил Семенович Цвет, also spelt Tsvett, Tswett, Tswet, Zwet, and Cvet) (1872-1919) was a Russian botanist who invented adsorption chromatography. ... 1901 (MCMI) was a common year starting on Tuesday (see link for calendar). ... Chlorophyll is a green photosynthetic pigment found in plants, algae, and cyanobacteria. ... In biology, pigment is any material resulting in color in plant or animal cells which is the result of selective absorption. ... 1903 has the latest occurring solstices and equinoxes for 400 years, because the Gregorian calendar hasnt had a leap year for seven years or a century leap year since 1600. ... Warsaw (Polish Warszawa, (?), in full The Capital City of Warsaw, Polish: Miasto StoÅ‚eczne Warszawa) is the capital of Poland and its largest city. ... 1906 was a common year starting on Monday (see link for calendar). ... 1907 was a common year starting on Tuesday (see link for calendar). ...

The Greek word chroma in chromatography means color in English and refers both to Tsvet's name that is literally translated from Russian as color and to the color of the plant pigments he was separating at that time.

In 1952 Archer John Porter Martin and Richard Laurence Millington Synge were awarded the Chemistry Nobel Prize "for their invention of partition chromatography". [1] 1952 was a leap year starting on Tuesday (link will take you to calendar). ... Archer John Porter Martin was a British chemist and Nobel Prize winner. ... Richard Laurence Millington Synge (born Liverpool, October 28, 1914, died Norwich, August 18, 1994) was a British biochemist, and winner of the 1952 Nobel Prize in Chemistry for the invention of partition chromatography. ...

The technology of chromatography advanced rapidly throughout the 20th century. Researchers found that the principles underlying Tsvet's chromatography could be applied in many different ways, giving rise to the different varieties of chromatography described below. Simultaneously, advances continually improved the technical performance of chromatography, allowing increasingly similar molecules to be resolved.

Chromatography theory

Chromatography is a separation method that exploits the differences in partitioning behavior between a mobile phase and a stationary phase to separate the components in a mixture. Components of a mixture may be interacting with the stationary phase based on charge, relative solubility or adsorption. There are two theories of chromatography, the plate and rate theories.

Retention

The retention is a measure of the speed at which a substance moves in a chromatographic system. In continuous development systems like HPLC or GC, where the compounds are eluted with the eluent, the retention is usually measured as the retention time R_t or t_R, the time between injection and detection. In interrupted development systems like TLC the retention is measured as the retention factor R_f, the run length of the compound divided by the run length of the eluent front:

The retention of a compound often differs considerably between experiments and laboratories due to variations of the eluent, the stationary phase, temperature, and the setup. It is therefore important to compare the retention of the test compound to that of one or more standard compounds under absolutely identical conditions.

Plate theory

The plate theory of chromotography was developed by Archer John Porter Martin and Richard Laurence Millington Synge. The plate theory describes the chromotography system, the mobile and stationary phases, as being in equilibrium. The partition coefficient K is based on this equilibrium, and is defined by the following equation: Archer John Porter Martin was a British chemist and Nobel Prize winner. ... Richard Laurence Millington Synge (born Liverpool, October 28, 1914, died Norwich, August 18, 1994) was a British biochemist, and winner of the 1952 Nobel Prize in Chemistry for the invention of partition chromatography. ...

K is assumed to be independent of concentration, and can change if experimental conditions are changed, for example temperature is increased or decreased. As K increases, it takes longer for solutes to separate. For a column of fixed length and flow, the retention time (t_R) and retention volume (V_r) can be measured and used to calculate K.

Paper chromatography

See the article paper chromatography Paper chromatography is an analytical technique for separating and identifying pigmentIt is one of the frequently used forms of chromatography. ...

In paper chromatography, chemical interactions with the paper make compounds travel at different rates.

A small spot of solution containing the sample is applied to a strip of chromatography paper about one centimeter from the base. This sample is adsorbed onto the paper. This means that the sample will contact the paper and may form interactions with it. Any substance that will react with (and thus bond to) the paper cannot be measured using this technique. The paper is then dipped in to a suitable solvent (such as ethanol or water) and placed in a sealed container. As the solvent rises through the paper it meets the sample mixture which starts to travel up the paper with the solvent. Different compounds in the sample mixture travel different distances according to how strongly they interact with the paper. Paper chromatography takes some time and the experiment is usually left to complete for some hours. Diagram of TLC tank drawn by Theresa Knott. ... Diagram of TLC tank drawn by Theresa Knott. ... This page is a candidate for speedy deletion. ... A solvent is a liquid that dissolves a solid, liquid, or gaseous solute, resulting in a solution. ... Ethanol, also known as ethyl alcohol or grain alcohol, is a flammable, colorless chemical compound, one of the alcohols that is most often found in alcoholic beverages. ... Water (from the Old English word wæter; c. ... A chemical compound is a chemical substance formed from two or more elements, with a fixed ratio determining the composition. ...

The final chromatogram can be compared with other known mixture chromatograms to identify sample mixes. Two-way paper chromatography involves using two solvents and rotating the paper 90^o inbetween. This is useful for separating complex mixtures of similar compounds.

Thin layer chromatography (TLC)

Separation of black ink on a TLC plate.

In thin layer chromatography or TLC the stationary phase consists of a thin layer of adsorbent like silica gel, alumina, or cellulose on a flat carrier like a glass plate, a thick aluminum foil, or a plastic sheet. Separation of black ink on TLC plate. ... Separation of black ink on TLC plate. ... Some examples of silica gel sachets Silica gel is a granular, porous form of silica made synthetically from sodium silicate. ... Aluminium oxide or aluminum oxide is a chemical compound of aluminium and oxygen with the chemical formula Al2O3. ... Cellulose (C6H10O5)n is a long-chain polymer polysaccharide carbohydrate, of beta-glucose. ... For eyeglasses, see glasses. ...

The process is similar to paper chromatography with the advantage of faster runs, better separations, and the choice between different adsorbents. TLC is a standard laboratory method in organic chemistry. Because of its simplicity and speed TLC is often used for monitoring chemical reactions and for the qualitative analysis of reaction products. Organic chemistry is the scientific study of the structure, properties, composition, reactions, and synthesis of organic compounds that by definition contain carbon. ... A chemical reaction is a process involving one, two, or more substances, such as compounds or atoms. ...

TLC plates are made by mixing the adsorbent with a small amount of inert binder like calcium sulfate (gypsum) and water, spreading the a thick slurry on the carrier, drying the plate, and activation of the adsorbent by heating in an oven. The thickness of the adsorbent layer is typically around 0.1–0.25 mm for analytical purposes and around 1–2 mm for preparative TLC. Inert is the state of doing little or nothing. ... Calcium sulfate is a common laboratory and industrial chemical. ...

Several methods exists to make colorless spots visible:

• Often a small amount of a fluorescent dye is added to the adsorbent that allows the visualization of UV absorbing spots under a blacklight ("UV₂₅₄").
• Iodine vapors are a general unspecific color reagent.
• Specific color reagents exist into which the TLC plate is dipped or which are sprayed onto the plate.

Once visible, the spots can be quantified by way of calculating their R_f values. These values should be the same regardless of the extent of travel of the solvent, and in theory are independent of a single experimental run. They do depend on the solvent used, and the type of TLC plate. Fluorescence induced by exposure to ultraviolet light in vials containing various sized cadmium selenide (CdSe) quantum dots. ... Note: Ultraviolet is also the name of a 1998 UK television miniseries about vampires. ... Note: Ultraviolet is also the name of a 1998 UK television miniseries about vampires. ... General Name, Symbol, Number iodine, I, 53 Chemical series halogens Group, Period, Block 17, 5, p Appearance violet-dark gray, lustrous Atomic mass 126. ...

Column chromatography

Column chromatography utilizes a vertical glass column filled with some form of solid support with the sample to be separated placed on top of this support. The rest of the column is filled with a solvent which, under the influence of gravity, moves the sample through the column. Similarly to other forms of chromatography, differences in rates of movement through the solid medium are translated to different exit times from the bottom of the column for the various elements of the original sample.

A picture of a standard column chromatography and a flash column chromatography setup

In 1978, W. C. Stills introduced a modified version of column chromatography called flash column chromatography ("flash"). The technique is very similar to the traditional column chromatography, except for that the solvent is driven through the column by applying positive pressure. Image File history File links Columnchromatography. ... Image File history File links Columnchromatography. ...

When applying positive pressure on top of the column, most separations could be performed in less than 20 minutes with improved separations compared to the old method. This makes flash column chromatography the method of choice for most synthetic organic chemists when purifying organic compounds.

In the modern Flash chromatography systems which can be purchased, the glass columns are replaced with pre-packed plastic cartridges. Solvent is pumped through the cartridge, which is much quicker. Systems may also be linked with detectors and fraction collectors providing automation. The introduction of gradient pumps means quicker separations and less solvent usage.

Gas-liquid chromatography

Gas-liquid chromatography is based on a partition equilibrium of analyte between a liquid stationary phase and a mobile gas. It is useful for a wide range of non-polar analytes, but poor for thermally labile molecules. Gas-liquid chromatography (GLC), or simply gas chromatography (GC) is a type of chromatography in which the mobile phase is a carrier gas, usually an inert gas such as helium, hydrogen or nitrogen, and the stationary phase is a microscopic layer of liquid on an inert solid support. ...

Ion exchange chromatography

Ion exchange chromatography is a column chromatography that uses a charged stationary phase. It is used to separate charged compounds including amino acids, peptides, and proteins. The stationary phase is usually an ion exchange resin that carries charged functional groups which interact with oppositely charged groups of the compound to be retained: In chemistry, an amino acid is any molecule that contains both amino and carboxylic acid functional groups. ... Peptides (from the Greek πεπτος, digestible), are the family of molecules formed from the linking, in a defined order, of various amino acids. ... A representation of the 3D structure of myoglobin, showing coloured alpha helices. ... An ion exchange resin is an insoluble matrix (or support structure) normally in the form of small (1-2mm diameter) beads, fabricated from an organic polymer substrate on the surface of which are sites with easily trapped and released ions in a process called ion exchange. ... In ecology functional groups are collections of organisms based on morphological, physiological, behavioral, biochemical, or environmental responses or on trophic criteria. ...

• Positively charged ion exchanger (anion exchanger) interacts with anions
• Negatively charged ion exchanger (cation exchanger) interacts with cations.

Bound compounds can be eluted from the column by gradient elution with an increasing concentration of salts, acid, or base in the eluent. An anion is an ion with negative charge. ... A cation is an ion with positive charge. ... In chemistry, salt is a term used for ionic compounds composed of positively charged cations and negatively charged anions, so that the product is neutral and without a net charge. ... An acid (often represented by the generic formula AH) is typically a water-soluble, sour-tasting chemical compound. ... The common (Arrhenius) definition of a base, also known as an alkaline compound, is a chemical compound that either donates hydroxide ions or absorbs hydrogen ions when dissolved in water. ...

Immobilized metal ion affinity chromatography

IMAC is a popular and powerful way to purify proteins. It is based on the specific coordinate covalent binding between histidine or other unique amino acids (either naturally present on the surface of the protein or grafted with recombinant DNA techniques) and various immobilized metal ions, such as copper, nickel, zinc, or iron. A representation of the 3D structure of myoglobin, showing coloured alpha helices. ... A coordinate covalent bond (also known as dative covalent bond) is a special type of covalent bond in which the shared electrons come from one of the atoms only. ... Histidine is one of the 20 most common natural amino acids, coded for in DNA. Nutritionally, in humans, histidine is considered an essential amino acid, but mostly only in children. ... In chemistry, an amino acid is any molecule that contains both amino and carboxylic acid functional groups. ... Recombinant DNA technology adds/replaces DNA in an organism resulting in the recipient organism containing exogenous DNA. Recombinant proteins are proteins that are produced by different genetically modified organisms following insertion of the relevant DNA into their genome. ...

Salt concentration is increased to produce later fractions.

High performance liquid chromatography (HPLC)

High performance liquid chromatography, usually referred to simply as HPLC, is a form of column chromatography used frequently in biochemistry and Analytical Chemistry. The analyte is forced through a column by liquid (mobile phase) at high pressure, which decreases the time the separated components remain on the stationary phase and thus the time they have to diffuse within the column. Diffusion within the column leads to broad peaks and loss of resolution. Less time on the column then translates to narrower peaks in the resulting chromatogram and thence to better resolution (it's easier to differentiate one peak from another) and sensitivity (tall, narrow peaks can be easier to discriminate from noise than shorter, broader peaks). High performance liquid chromatography, also known as high pressure liquid chromatography and usually abbreviated as HPLC, is a form of column chromatography used frequently in biochemistry and analytical chemistry. ... Column chromatography in chemistry is the preparative application of chromatography. ... Biochemistry is the chemistry of life, a bridge between biology and chemistry that studies how complex chemical reactions give rise to life. ... Analytical chemistry is the analysis of material samples to gain an understanding of their chemical composition and structure. ... This article is about the physical mechanism of diffusion. ...

Reversed phase (RP) liquid chromatography

Traditionally HPLC stationary phases are polar, whereas so-called "reverse" phase (RP-HPLC) stationary phases are hydrophobic. On an RP-HPLC column, then, hydrophobic analytes would tend to be retained on the column, eluting more readily as the proportion of the hydrophobic component of the mobile phase is increased. RP-HPLC has lower resolution than GC.

Gel permeation chromatography

Gel permeation chromatography, also known as size exclusion chromatography or Sephadex gel chromatography, separates molecules on basis of size. Smaller molecules enter a porous media and take longer to exit the column, hence larger particles leave the column first. GPC is good for determining polymer molecular weight distribution, but is low resolution. Gel permeation chromatography (GPC) also known as size exclusion chromatography (SEC) is a chromatographic method in which molecules are separated based on their size. ... The word resolution has several meanings, depending on context. ...

Affinity chromatography

Affinity chromatography is based on selective non-covalent interaction between an analyte and specific molecules. It is very specific, but not very robust. It is often used in biochemistry in the purification of proteins (or better: protein constructs). These constructs can be of fusion proteins with a so-called His-tag, biotinylated or possibly antigens. After purification some of these tags are usually removed and the pure protein is obtained. Affinity chromatography is a biochemical separation method that combines size fractionation capability of gel permeation chromatography with the ability to design a stationary phase that reversibly binds to a known subset of molecules. ... Robust means healthy, strong, and durable. ... A representation of the 3D structure of myoglobin, showing coloured alpha helices. ... A fusion protein is a protein created through genetic engineering from two or more proteins/peptides. ... A His-tag is an amino acid motif in proteins that consists of six histidine (His) residues, often at the N- or C-terminus of the protein. ... Biotin, also known as vitamin H or B7 and C10H16N2O3S (Biotin; Coenzyme R, Biopeiderm), is a water-soluble B-complex vitamin which is composed of an ureido ring fused with a tetrahydrothiophene ring. ... An antigen is a molecule that stimulates the production of antibodies. ... Tag (also known as it, had, he, tig, or other names) is an informal sport or game (see also playground games) that usually involves one or more players attempting to tag other players by touching them with their hands. ...

Countercurrent chromatography

Countercurrent chromatography This article is in need of attention from an expert on the subject. ...

See also

• Paper chromatography of amino acids

This page is a candidate to be moved to Wikibooks. ...

External links

• Library 4 Science online books about chromatography.