GB1570236A - Method and apparatus for liquid chromatography - Google Patents

Method and apparatus for liquid chromatography Download PDF

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Publication number
GB1570236A
GB1570236A GB967877A GB967877A GB1570236A GB 1570236 A GB1570236 A GB 1570236A GB 967877 A GB967877 A GB 967877A GB 967877 A GB967877 A GB 967877A GB 1570236 A GB1570236 A GB 1570236A
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United Kingdom
Prior art keywords
light
tube
detector
eluent
source
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GB967877A
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National Research Development Corp UK
National Research Development Corp of India
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National Research Development Corp UK
National Research Development Corp of India
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Priority to GB967877A priority Critical patent/GB1570236A/en
Priority to US05/884,621 priority patent/US4233030A/en
Publication of GB1570236A publication Critical patent/GB1570236A/en
Expired legal-status Critical Current

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    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N30/00Investigating or analysing materials by separation into components using adsorption, absorption or similar phenomena or using ion-exchange, e.g. chromatography or field flow fractionation
    • G01N30/02Column chromatography
    • G01N30/62Detectors specially adapted therefor
    • G01N30/74Optical detectors
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N21/00Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
    • G01N21/62Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
    • G01N21/63Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
    • G01N21/631Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited using photolysis and investigating photolysed fragments

Description

(54) IMPROVEMENTS IN OR RELATING TO METHODS AND APPARATUS FOR LIQUID CHROMATOGRAPHY (71) We, NATIONAL RESEARCH DE VELOPMENT CORPORATION, a British Corporation, established by statute of Kingsgate House, 6S74, Victoria Street, London SW1E 6SL, do hereby declare the invention, for which I pray that a patent may be granted to me, and the method by which it is to be performed, to be particularly described in and by the following statement: Background of the Invention This invention relates to methods of and apparatus for liquid chromatography, in particular high-pressure liquid chromatography (HPLC), sometimes known as highperformance or high-speed liquid chromatography, though also applicable to traditional liquid chromatography.
In HPLC, a solution containing one or more constituents is forced rapidly through a chromatographic column. The retention volume (in practice the time at constant flow-rate) after which a constituent arrives at the column output in the eluent is characteristic of the constituent. Known techniques for detecting this arrival include measuring optical absorption (using UV or visible light), fluorescence, refractive index or electrochemical behaviour, e.g. electrooxidation or reduction potential.
Some substances are inherently suitable for such detection but others may not possess a suitable detectable property. For example they may not fluoresce at all, or not to a degree or at a wavelength which gives the required degree of selectivity or sensitivity. Some substances can, however, be modified photochemically by irradiation with light of a suitable wavelength, and the present invention utilises this fact to enable substances otherwise unsuitable for detection by HPLC to be detected thereby.
Examples of such substances are cannabinoids, whose detection in body fluids is of forensic importance; Bowd et al have shown (Talanta, 1971, pp. 697-705) that cannabis has constituents, for example CBN (cannabinol), which can be modified photochemically by irradiation with UV to yield a substance with an enhanced UV fluorescence at a wavelength suitable for detection.
Summat of the Invention According to the present invention, in a method of liquid chromatography wherein the eluent from a chromatographic column enters a detector adapted to detect a known or suspected constituent by means of a given property, the eluent while flowing between the column and the detector is irradiated in order to convert the constituent photochemically to a species which possesses this property, or in which said property is changed in magnitude to a substantial degree.
Preferably the method is high-pressure liquid chromatography. The irradiation may be by UV or visible light. Additional reactants may be added to the eluent either before or after its passage through the column, to take part in the photochemical reaction.
The property may be fluorescence. The constituent may be converted from a species giving little or no fluorescence with UV or visible light to a species giving an enhanced degree thereof. Alternatively, the constituent may be converted to a species giving reduced or no fluorescence. Such enhancement or reduction may also involve a change in the wavelength of the fluorescence.
As an alternative to fluorescence the property may be light absorbance, the constituent being converted by irradiation either to a species having enhanced light absorbance at a particular wavelength, or to a species having reduced light absorbance at a particular wavelength. The light absorbance may be visible or UV absorbance.
Irradiation may serve to increase the sensitivity and/or the selectivity of detection.
For example, to increase the selectivity, a non-fluorescent substance can be converted to a fluorescent species, or a fluorescent substance to a non-fluorescent species, whereas any interfering substances present may not react in the same way. Similarly, irradiation may allow detection by light absorbance at a wavelength where the converted species of interest has high absorbance but where any interfering substances present have low absorbance, or alternatively where the converted species of interest has low absorbance but the interfering substances have high absorbance.
The selectivity may be increased by comparing measurements made on the irradiated and non-irradiated eluent, e.g. by temporarily discontinuing the irradiation or causing the eluent to by-pass the irradiation, or causing the eluent to pass through a further detector prior to irradiation and comparing the outputs of the two detectors.
Such procedures are applicable to both fluorescence and absorbance detection, and to both enhancement and reduction of the detected property by irradiation.
Also according to the present invention, in apparatus for liquid chromatography there is connected between a chromatographic column and a detector arranged to receive eluent from the column a photochemical reactor comprising a translucent duct for passage of the eluent and a lightsource arranged to irradiate the eluent flowing in the duct. Preferably the apparatus is high-pressure liquid chromatography ap Apparatus The duct may comprise a long, translucent, small-bore tube, e.g. of fused silica, shaped to a configuration which at least partially surrounds the light-source.
In one configuration the tube is bent back upon itself repetitively to form an arc of generally straight tube-portions each generally parallel to the axis of the arc and a linear light-source is located along said axis.
Alternatively the tube may form a multiturn helix surrounding the light source.
The duct may be enclosed within a liquidtight jacket having an inlet and outlet for a liquid coolant. The jacket may be of an: nular shape, having an) inner cylindrical wall which is translucent to allow entry of light from an axially located light-source.
The jacket may have an outer cylindrical wall whose inner surface is light-reflecting.
The present invention also provides, for use in liquid chromatography apparatus, preferably in high-pressure liquid chromatography apparatus, a photochemical reactor constructed and adapted to be connected as aforesaid.
In performing the method the coolant may be adapted, e.g. by the inclusion of a solute, to act as an optical filter which selects light of a desired wavelength from the light-source. Alternative ways of obtaining light of desired wavelengths include the use of different light-sources (e.g. Xe arc, high pressure Hg arc, etc.), and making the eluent duct or the translucent inner cylindrical wall (or equivalent wall in other jacket configurations) of a material which transmits only the desired wavelengths.
The temperature at which the photochemical reaction is carried out may be varied by varying the temperature of the liquid in the jacket.
Description of the Drawings To enable the nature of the present invention to be more readily understood, attention is directed, by way of example, to the accompanying drawings wherein: Fig. 1 is a block schematic diagram of HPLC apparatus embodying the present invention.
Fig. 2 is a sectional perspective view of a photochemical reactor suitable for use in the present invention.
Fig. 3 shows chromatograms of cannabinol (CBN) obtained with a fluorescence detector: (a) without eluent irradiation, and (b) with eluent irradiation in accordance with the present invention.
Fig. 4 shows chromatograms of lysergic acid diethylamide (LSD) obtained with a fluorescence detector: (a) without eluent irradiation, and (b) with UV irradiation of the eluent Fig. 5 shows chromatograms of cannabinol (CBN) obtained with an absorbance detector: (a) without eluent irradiation, and (b) with UV irradiation of the eluent.
Description of Preferred Embodiments In Fig. 1 a pump 1 feeds a liquid eluent via an injector 2 to a chromatographic column 3 in a known manner. Substances to be separated are introduced on to the column via the injector 2. Hitherto the eluent from column 3 has generally been fed directly to a detector, e.g. of the fluorescence type. In the present invention the eluent - flows to detector 5 via a photo chemical reactor 4. The eluent from detector 5 goes to waste (arrow 7) and the electrical output from the detector 5 is fed to a chart-recorder 6, as hitherto.
Fig. 2 shows one form of photochemical reactor 4. It comprises a long, small-bore, fused-silica tube 8 bent back upon itself repetitively to provide a plurality of straight tubeportions 9 arranged in an arc along whose axis is located a light-source 10. The tube 8 is located within an annular liquidtight coolant jacket comprising an inner tube 11 of fused silica and an outer tube 12 of aluminium alloy whose inner surface is polished to reflect light from source 10.
Tube 11 is sealed to metal end-plates 13 by O-ring seals. Inlet and outlet connections 14 for tube 8 are provided in one of the end-plates 13, and inlet and outlet connections 15 for the coolant in tube 12. In one embodiment tube 8 is 70 cm long, OD 2 mm, ID 0-25 mm. Alternatively the tube can form a multiturn helix located in the coolant jacket.
In use the constituents of interest are separated chromatographically by column 3 (Fig. 1) in the usual way and pass in sequence to the reactor 4 where they are irradiated by the light source 10. For detecting the CBN component of cannabis, this source is suitably a medium-pressure Hg arc lamp and the detector 5 is a conventional fluorescence detector. If -CBN is present in the solution, it reacts photochemically in the reactor to yield a fluorescent species which is detected by the detector. By contrast, the fluorescence of non-irradiated CBN is generally insufficient to allow of sensitive detection thereby. The effect is illustrated by Fig. 3, which shows chromatograms of cannabinol (10 ng), (a) without irradiation and (b) with irradiation.
Compensation can be made for naturally fluorescent substances in the eluent by injecting a further quantity of the substances to be separated on to the column with the light-source switched off, or with the reactor by-passed. Only naturally fluorescent substances are now detected and the output due solely to the substance converted to the fluorescent species by irradiation can be determined by comparing the two chromatograms. The same effect can be achieved with a single injection of solution by connecting a further fluorescence detector (not shown) between column 3 and reactor 4 (Fig. 1), and comparing the chromatograms from the two detectors.
Referring now to Fig. 4 it is seen that the naturally fluorescent LSD is converted by Lw irradiation to a species which is nonfluorescent. This chromatogram was performed using an aqueous methanolic eluent, the water present acting both as a component of the eluent and also as a reagent in the photochemical reaction with LSD.
(The LSD molecule is known to undergo photoaddition of water to form the nonfluorescent lumi-LSD). Interfering fluorescent materials present may not so react and thus the method may be used to discriminate between LSD and non-photolabile substances which have fluorescent and chromatographic characteristics similar to LSD.
In the exemplary apparatus and measure- ments described above, the detector or detectors are of the fluorescence type. However the invention is not limited to the use of this type of detector, and the irradiation may serve to convert a constituent or constituents to species suitable for other types of detection. Fig. 5 shows results obtained using an absorbance detector, for example.
In Fig. 5 the absorbance was measured at 360 nm. It is seen that the effect of Lw irradiation is to convert CBN to a species having enhanced absorbance at this wavelength. Although unirradiated CBN can be detected by its absorbance at 280 nm, interference due to other substances present may be reduced if 360 nm detection is used.
An important consideration in HPLC is to minimise the "dead volume", i.e. the volume of the flow-lines, detector cell, etc., so that the resolution obtained on the column is not lost. The form of reactor shown in Fig. 2 has been devised to be of low dead volume and therefore to have a minimal effect on resolution.
WHAT I CLAIM IS:- 1. A method of liquid chromatography wherein the eluent from a chromatographic column enters a detector adapted to detect a known or suspected constituent by means of a given property, wherein the eluent while flowing between the column and the detector is irradiated in order to convert the constituent photochemically to a species which possesses this property or in which said property is changed in magnitude to a substantial degree.
2. A method as claimed in claim 1 wherein the method is high-pressure liquid chromatography.
3. A method as claimed in claim 1 or claim 2 wherein the irradiation is by UV or visible light.
4. A method as claimed in any preceding claim wherein at least one additional reactant is added to the eluent either before or after its passage through the column, to take part in the photo chemical reaction.
5. A method as claimed in any-preceding claim wherein the constituent is converted to a species which possesses said property or in which said property is enhanced.
6. A method - as claimed in claim 5 wherein the property is fluorescence.
**WARNING** end of DESC field may overlap start of CLMS **.

Claims (28)

**WARNING** start of CLMS field may overlap end of DESC **. detector 5 goes to waste (arrow 7) and the electrical output from the detector 5 is fed to a chart-recorder 6, as hitherto. Fig. 2 shows one form of photochemical reactor 4. It comprises a long, small-bore, fused-silica tube 8 bent back upon itself repetitively to provide a plurality of straight tubeportions 9 arranged in an arc along whose axis is located a light-source 10. The tube 8 is located within an annular liquidtight coolant jacket comprising an inner tube 11 of fused silica and an outer tube 12 of aluminium alloy whose inner surface is polished to reflect light from source 10. Tube 11 is sealed to metal end-plates 13 by O-ring seals. Inlet and outlet connections 14 for tube 8 are provided in one of the end-plates 13, and inlet and outlet connections 15 for the coolant in tube 12. In one embodiment tube 8 is 70 cm long, OD 2 mm, ID 0-25 mm. Alternatively the tube can form a multiturn helix located in the coolant jacket. In use the constituents of interest are separated chromatographically by column 3 (Fig. 1) in the usual way and pass in sequence to the reactor 4 where they are irradiated by the light source 10. For detecting the CBN component of cannabis, this source is suitably a medium-pressure Hg arc lamp and the detector 5 is a conventional fluorescence detector. If -CBN is present in the solution, it reacts photochemically in the reactor to yield a fluorescent species which is detected by the detector. By contrast, the fluorescence of non-irradiated CBN is generally insufficient to allow of sensitive detection thereby. The effect is illustrated by Fig. 3, which shows chromatograms of cannabinol (10 ng), (a) without irradiation and (b) with irradiation. Compensation can be made for naturally fluorescent substances in the eluent by injecting a further quantity of the substances to be separated on to the column with the light-source switched off, or with the reactor by-passed. Only naturally fluorescent substances are now detected and the output due solely to the substance converted to the fluorescent species by irradiation can be determined by comparing the two chromatograms. The same effect can be achieved with a single injection of solution by connecting a further fluorescence detector (not shown) between column 3 and reactor 4 (Fig. 1), and comparing the chromatograms from the two detectors. Referring now to Fig. 4 it is seen that the naturally fluorescent LSD is converted by Lw irradiation to a species which is nonfluorescent. This chromatogram was performed using an aqueous methanolic eluent, the water present acting both as a component of the eluent and also as a reagent in the photochemical reaction with LSD. (The LSD molecule is known to undergo photoaddition of water to form the nonfluorescent lumi-LSD). Interfering fluorescent materials present may not so react and thus the method may be used to discriminate between LSD and non-photolabile substances which have fluorescent and chromatographic characteristics similar to LSD. In the exemplary apparatus and measure- ments described above, the detector or detectors are of the fluorescence type. However the invention is not limited to the use of this type of detector, and the irradiation may serve to convert a constituent or constituents to species suitable for other types of detection. Fig. 5 shows results obtained using an absorbance detector, for example. In Fig. 5 the absorbance was measured at 360 nm. It is seen that the effect of Lw irradiation is to convert CBN to a species having enhanced absorbance at this wavelength. Although unirradiated CBN can be detected by its absorbance at 280 nm, interference due to other substances present may be reduced if 360 nm detection is used. An important consideration in HPLC is to minimise the "dead volume", i.e. the volume of the flow-lines, detector cell, etc., so that the resolution obtained on the column is not lost. The form of reactor shown in Fig. 2 has been devised to be of low dead volume and therefore to have a minimal effect on resolution. WHAT I CLAIM IS:-
1. A method of liquid chromatography wherein the eluent from a chromatographic column enters a detector adapted to detect a known or suspected constituent by means of a given property, wherein the eluent while flowing between the column and the detector is irradiated in order to convert the constituent photochemically to a species which possesses this property or in which said property is changed in magnitude to a substantial degree.
2. A method as claimed in claim 1 wherein the method is high-pressure liquid chromatography.
3. A method as claimed in claim 1 or claim 2 wherein the irradiation is by UV or visible light.
4. A method as claimed in any preceding claim wherein at least one additional reactant is added to the eluent either before or after its passage through the column, to take part in the photo chemical reaction.
5. A method as claimed in any-preceding claim wherein the constituent is converted to a species which possesses said property or in which said property is enhanced.
6. A method - as claimed in claim 5 wherein the property is fluorescence.
7. A method as claimed in claim 6
wherein the constituent is converted from a species giving little or no fluorescence with Lw or visible light to a species giving an enhanced degree thereof.
8. A method as claimed in claim 6 wherein the constituent is converted from a species giving substantial fluorescence with UV or visible light to a species giving reduced or no fluorescence.
9. A method as claimed in any of claims 1 to 4 wherein the property is either visible or UV light absorbance, the constituent being converted by irradiation either to a species having enhanced light absorbance at a particular wavelength, or to a species having reduced light absorbance at a particular wavelength.
10. A method as claimed in any of claims 1, 2 or 3 wherein the eluent under irradiation includes a reactant, additional to the known or suspected constituent, which takes part in the photochemical reaction.
11. Apparatus for liquid chromatography in which there is connected between a chromatographic column and a detector arranged to receive eluent from the column a photochemical reactor comprising a translucent duct for passage of the eluent and a light-source arranged to irradiate the eluent flowing in the duct.
12. Apparatus as claimed in claim 11 comprising high-pressure liquid chromatography apparatus.
13. Apparatus as claimed in claim 11 or claim 12 wherein the duct comprises a long translucent small-bore tube shaped to a configuration which at least partially surrounds the light-source.
14. Apparatus as claimed in claim 13 wherein the duct is enclosed within a liquid-tight jacket having an inlet and outlet for a liquid coolant.
15. Apparatus as claimed in claim 14 wherein the jacket is of annular shape having an inner cylindrical wall which is translucent to allow entry of light from an axially located light-source.
16. Apparatus as claimed in claim 15 wherein the jacket has an outer cylindrical wall whose inner surface is light-reflecting.
17. Apparatus as claimed in any of claims 13 to 16 wherein the tube is bent back upon itself repetitively to form an are of generally straight tube-portions each generally parallel to the axis of the are and a linear light-source is located along said axis.
18. Apparatus as claimed in any of claims 13 to 16 wherein the tube is wound as a multi-turn helix surrounding said light source.
19. A photochemical reactor suitable for use in apparatus as claimed in claim 12 comprising a single long translucent smallbore tube having a bore not substantially greater than about 0-25mm and having one end adapted for connection to the eluentend of the chromatographic column of a high-pressure liquid chromatography apparatus and the other end adapted for connection to a detector adapted to detect a known or suspected constituent of the eluent by means of a given property, and a light-source for irradiating eluent flowing in the tube, said tube being shaped to a configuration which at least partially surrounds said light-source.
20. A reactor as claimed in claim 19 wherein the duct is enclosed within a liquidtight jacket having an inlet and outlet for a liquid coolant.
21. A reactor as claimed in claim 20 wherein the jacket is of annular shape having an inner cylindrical wall which is translucent to allow entry of light from said light-source, said light-source being located within the space bounded by said inner cylindrical wall.
22. A reactor as claimed in claim 21 wherein the jacket has an outer cylindrical wall whose inner surface is light-reflecting.
23. A reactor as claimed in any of claims 19 to 22 wherein the tube is bent back upon itself repetitively to form an arc of generally straight tube-portions each generally parallel to the axis of the arc, and wherein said light-source is linear and is located along said axis.
24. A reactor as claimed in any of claims 19 to 22 wherein the tube is wound as a multi-turn helix surrounding said light source.
25. A method of liquid chromatography substantially as hereinbefore described with reference to Figs. 1 and 3 of the accompany drawings.
26. A method of liquid chromatography substantially as hereinbefore described with reference to Figs. 4 or 5 of the accompanying drawings.
27. Apparatus for liquid chromatography substantially as hereinbefore described with reference to Fig. 1 or to Figs.
1 and 2 of the accompanying drawings.
28. A photochemical reactor substantially as hereinbefore described with reference to Fig. 2 of the accompanying drawings.
GB967877A 1977-03-08 1977-03-08 Method and apparatus for liquid chromatography Expired GB1570236A (en)

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GB967877A GB1570236A (en) 1977-03-08 1977-03-08 Method and apparatus for liquid chromatography
US05/884,621 US4233030A (en) 1977-03-08 1978-03-06 Methods and apparatus for liquid chromatography

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Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP2271932A2 (en) * 2008-04-30 2011-01-12 Waters Technologies Corporation Apparatus and methods for performing photoreactions and analytical methods and devices to detect photo-reacting compounds

Cited By (3)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
EP2271932A2 (en) * 2008-04-30 2011-01-12 Waters Technologies Corporation Apparatus and methods for performing photoreactions and analytical methods and devices to detect photo-reacting compounds
EP2271932A4 (en) * 2008-04-30 2011-06-29 Waters Technologies Corp Apparatus and methods for performing photoreactions and analytical methods and devices to detect photo-reacting compounds
US8524502B2 (en) 2008-04-30 2013-09-03 Waters Technologies Corporation Apparatus and methods for performing photoreactions and analytical methods and devices to detect photo-reacting compounds

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