CA2315474A1 - Micro extraction technique - Google Patents
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- CA2315474A1 CA2315474A1 CA 2315474 CA2315474A CA2315474A1 CA 2315474 A1 CA2315474 A1 CA 2315474A1 CA 2315474 CA2315474 CA 2315474 CA 2315474 A CA2315474 A CA 2315474A CA 2315474 A1 CA2315474 A1 CA 2315474A1
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- support
- sample
- analytes
- coating
- solid
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N1/00—Sampling; Preparing specimens for investigation
- G01N1/28—Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
- G01N1/40—Concentrating samples
- G01N1/405—Concentrating samples by adsorption or absorption
Abstract
The invention disclosed relates to a method and apparatus for solid phase microextraction of target analytes from solid or fluid samples. The apparatus comprises gas tight enclosure means, means for introducing a sample including target analytes into the enclosure means, and means located within the enclosure means for extracting the target analytes from the sample, wherein the extraction means either samples a head space near the sample or samples the sample directly.
Description
Micro Extraction Technique BACKGROUND OF THE INVENTION
Field of the Invention This invention relates to the method for solid phase micro extraction and analysis and in particular to the micro extraction and analysis using various types of solid supports which can be coated with various materials.
Description of the Prior Art The analysis of environmental, food, biomedical and pharmaceutical samples involves the separation of components or analytes of interest from the sample matrix such as soil, water, food, tissue or other material. Liquid/liquid extraction is a traditional method of sample extraction and separation- an example is the extraction of a water sample with an immiscible organic solvent such as hexane. Solid samples can be mixed with anhydrous sodium sulfate, ground to a free flowing powder, packed into a chromatography column and then extracted with an organic solvent. Solvent-based extraction methods are frequently time consuming and expensive since high purity solvents must be purchased and properly disposed. Also, many solvents are relatively toxic and should be handled only under proper laboratory conditions. Solvent extraction is not very selective so further analyte isolation is usually accomplished by other chromatographic techniques before the analytes can be quantitated. This increases the cost and complexity of the analysis.
Solid phase extraction is an alternative to liquid/liquid extraction. This involves the selective adsorption of the analytes of interest onto a solid substrate/sorbent (typically a chemically modified silica surface) while other co-extractives are unretained.
Pre-made solid phase extraction cartridges are available but there is significant variation between manufacturers products. The analytes of interest are then eluted from the sorbent by the use of selective solvent or solvent mixtures. The analyte(s) can then be analyzed. Many different types of sorbents are available so that a wide range of selectivities are possible.
Although solvent use is reduced relative to liquid/liquid extraction, purchase and disposal costs remain and the procedure is still time consuming.
S US Patent no. 5,691,206 describes a prior solid phase micro extraction apparatus and method. The method consists of two process steps - partitioning of analytes between the coating (sorbent) and sample, and desorption of the collected analytes into an analytical instrument. This is accomplished by exposing the coated substrate, typically in the form of a fibre, to the sample, allowing the target analytes to be extracted e.g.
adsorbed into the coating from either the head space above the sample or from the sample directly.
Various coatings are available to adjust selectivity of the extraction and no solvent is used for the extraction. After exposure, the fibre (now containing concentrated analytes) is then typically moved to a thermal desorption instrument, where the analyte is thermally desorbed, followed by separation and quantitation of the analytes. The method is simple, inexpensive and eliminates some of the disadvantages of solid phase extraction including:
solvent consumption, extract preconcentration and high blank values. However, it has a significant limitation of low sample throughput which has been only partially overcome by expensive automation options.
SUMMARY OF THE INVENTION
According to the invention, an apparatus and method for carrying out solid phase micro extraction of analytes contained within a fluid or a solid sample, is provided.
In one embodiment of the invention, an apparatus for carrying out solid phase microextraction of analytes included in a fluid or a solid sample is provided, comprising gas tight enclosure means, means for introducing a sample including target analytes into the enclosure means, and means located within the enclosure means for extracting the target analytes from the sample, wherein the extraction means either samples a head space near the sample or samples the sample directly.
Field of the Invention This invention relates to the method for solid phase micro extraction and analysis and in particular to the micro extraction and analysis using various types of solid supports which can be coated with various materials.
Description of the Prior Art The analysis of environmental, food, biomedical and pharmaceutical samples involves the separation of components or analytes of interest from the sample matrix such as soil, water, food, tissue or other material. Liquid/liquid extraction is a traditional method of sample extraction and separation- an example is the extraction of a water sample with an immiscible organic solvent such as hexane. Solid samples can be mixed with anhydrous sodium sulfate, ground to a free flowing powder, packed into a chromatography column and then extracted with an organic solvent. Solvent-based extraction methods are frequently time consuming and expensive since high purity solvents must be purchased and properly disposed. Also, many solvents are relatively toxic and should be handled only under proper laboratory conditions. Solvent extraction is not very selective so further analyte isolation is usually accomplished by other chromatographic techniques before the analytes can be quantitated. This increases the cost and complexity of the analysis.
Solid phase extraction is an alternative to liquid/liquid extraction. This involves the selective adsorption of the analytes of interest onto a solid substrate/sorbent (typically a chemically modified silica surface) while other co-extractives are unretained.
Pre-made solid phase extraction cartridges are available but there is significant variation between manufacturers products. The analytes of interest are then eluted from the sorbent by the use of selective solvent or solvent mixtures. The analyte(s) can then be analyzed. Many different types of sorbents are available so that a wide range of selectivities are possible.
Although solvent use is reduced relative to liquid/liquid extraction, purchase and disposal costs remain and the procedure is still time consuming.
S US Patent no. 5,691,206 describes a prior solid phase micro extraction apparatus and method. The method consists of two process steps - partitioning of analytes between the coating (sorbent) and sample, and desorption of the collected analytes into an analytical instrument. This is accomplished by exposing the coated substrate, typically in the form of a fibre, to the sample, allowing the target analytes to be extracted e.g.
adsorbed into the coating from either the head space above the sample or from the sample directly.
Various coatings are available to adjust selectivity of the extraction and no solvent is used for the extraction. After exposure, the fibre (now containing concentrated analytes) is then typically moved to a thermal desorption instrument, where the analyte is thermally desorbed, followed by separation and quantitation of the analytes. The method is simple, inexpensive and eliminates some of the disadvantages of solid phase extraction including:
solvent consumption, extract preconcentration and high blank values. However, it has a significant limitation of low sample throughput which has been only partially overcome by expensive automation options.
SUMMARY OF THE INVENTION
According to the invention, an apparatus and method for carrying out solid phase micro extraction of analytes contained within a fluid or a solid sample, is provided.
In one embodiment of the invention, an apparatus for carrying out solid phase microextraction of analytes included in a fluid or a solid sample is provided, comprising gas tight enclosure means, means for introducing a sample including target analytes into the enclosure means, and means located within the enclosure means for extracting the target analytes from the sample, wherein the extraction means either samples a head space near the sample or samples the sample directly.
In another embodiment of the invention, an apparatus is provided comprising, an assembly for carrying out solid phase microextraction of analytes contained within a fluid or a solid sample, and a gas tight sampling enclosure. The assembly is arranged such that it either samples the head space above the sample or samples the sample matrix directly, within the gas tight enclosure. The assembly includes a solid support, which may be in the form of a fibre which may be coated or uncoated. The fibre and/or the coating material is selected, based upon selectivity of the fibre and/or coating for at least one of the analytes present in the sample.
In a further embodiment of the invention, a method for solid phase micro extraction of analytes included in a fluid or a solid sample is provided, comprising (a) exposing a fluid or a solid sample including target analytes, to a solid support which may be coated or uncoated, the support and/or the coating being selected based upon selectivity of the support and/or coating for at least one of the analytes in the sample, for a sufficient time to permit chemical extraction of the analytes by the support to occur, and (b) ending said contact and then placing said solid support into a micro volume of solvent where chemical desorption of the analytes from the support occurs.
In yet another embodiment of the invention, a method is provided for solid phase micro extraction of analytes contained within a fluid or a solid sample, comprising exposing a solid support, which may be in the form of a fibre, which may be coated or uncoated, the fibre and/or the coating material being selected based upon selectivity of the fibre andlor coating for at least one of the analytes in the sample, for a sufficient time to permit chemical extraction of the analytes to occur, ending said contact and then placing said solid support into a suitable micro volume of solvent where desorption of the analytes from the support occurs. Quantitation of the analytes in the extracting solvent can then proceed by conventional means.
In a further embodiment of the invention, a method for solid phase micro extraction of analytes included in a fluid or a solid sample is provided, comprising (a) exposing a fluid or a solid sample including target analytes, to a solid support which may be coated or uncoated, the support and/or the coating being selected based upon selectivity of the support and/or coating for at least one of the analytes in the sample, for a sufficient time to permit chemical extraction of the analytes by the support to occur, and (b) ending said contact and then placing said solid support into a micro volume of solvent where chemical desorption of the analytes from the support occurs.
In yet another embodiment of the invention, a method is provided for solid phase micro extraction of analytes contained within a fluid or a solid sample, comprising exposing a solid support, which may be in the form of a fibre, which may be coated or uncoated, the fibre and/or the coating material being selected based upon selectivity of the fibre andlor coating for at least one of the analytes in the sample, for a sufficient time to permit chemical extraction of the analytes to occur, ending said contact and then placing said solid support into a suitable micro volume of solvent where desorption of the analytes from the support occurs. Quantitation of the analytes in the extracting solvent can then proceed by conventional means.
BRIEF DESCRIPTION OF THE DRAWINGS
Figure 1 is a schematic side view of a fibre assembly according to the invention;
S Figure 2 is an enlarged end view of a fibre assembly according to the invention;
Figure 3 is a schematic side view of a shielded fibre assembly according to the invention;
Figure 4 is a schematic side view of a fibre assembly installed in a typical sampling enclosure according to the invention;
Figure Sa illustrates the reproducibility of multiple extractions of tetraethyltin, tetraethyllead, di-n-propyl mercury and decane using the present technique from an aqueous solution;
Figure Sb illustrates the reproducibility of multiple extractions of ionic butyltin compounds (ethylated in situ) from a complex biological matrix using the present technique;
Figure 6 is a chromatogram of the extraction of a chlorinated pesticide mixture containing 1) gamma-BHC (lindane), 2) heptachlor, 3) aldrin, 4) dieldrin, 5) endrin and 6) 4,4'-DDT from an aqueous sample; and Figure 7 is a chromatogram of the extraction of a BTEX mixture containing 1) benzene, 2) toluene, 3) ethylbenzene, 4) p-xylene, 5) m-xylene and 6) o-xylene from an aqueous solution.
DETAILED DESCRIPTION OF THE INVENTION
Referring to figures 1 and 2, in detail, an assembly 1 for carrying out solid phase micro extraction is shown, comprising a cylindrical support lA, which may be in the form of a fibre, and which may have a length of coating 2 of which various types of organic compounds could be used. The diameter of the fibre may vary, but would generally be between 0.5 to 2 mm and it may be solid or hollow.
As seen in figure 3, a cylindrical support lA which has a length of coating, is mounted through a Teflon~ faced silicone septum 4. Stainless steel tubing 3 , which acts as a shield, of slightly longer length than the coating is mounted over the support lA. If the fibre is pulled up through the silicone septum, until the fibre coating is inside the stainless steel sleeve 3, the extracted analytes are shielded from volatizing into the atmosphere.
This permits short term storage or transport of the fibre assembly without having to immediately desorb the analytes into a solvent.
The coating is typically provided on the outside of solid fibres, and may be on the outside and/or the inside of hollow fibres.
In figure 4., the assembly 1 is mounted in a gas tight enclosure 2, typically but not exclusively a hypo-vial (trade mark) with an open top, closed by a crimp top (as illustrated) 3A, or screw cap and Teflon-faced seal 4A. Generally, a Teflon coated magnetic stir bar S is included to permit agitation of the sample 6 during extraction of the analytes by the fibre lA. The assembly 1 is positioned for head space sampling but can also used for direct (aqueous layer) sampling as well. Fibres can be manufactured with various coating lengths but 10 mm is the typical length used. Although longer lengths of coating can result in a greater amount of extracted analyte, for our purpose, a 10 mm length completely submerged in a 1 SO ~L volume of solvent is sufficient for adequate desorption. For multiple extraction chemistries or to increase the extraction efficiency, we would use mixed chemistry coatings or multiple fibres.
Fibres can be constructed with fused silica or other support material chemically or mechanically modified e.g. by roughening of the fibre surface to improve adhesion of the coating, followed by chemical attachment of the desired coating. Although there are both absorption and adsorption-type SPME coatings available, our fibres with a silicone coating would extract analytes by absorption, while porous polymer coatings (such as CarboxenTM) can extract suitable analytes by adsorption within the pore structure.
Alternatively, the support can be constructed from silicone (such as Dow Corning Silastic~ Q7-4750 (0.51 mm ID, 0.94 mm OD) that was used in our studies) or other polymer tubing lengths, swelled by solvent and then dried (to a tight fit) over metal wire or other cylindrical support material. Polymer tubing used for the support is exhaustively extracted by solvent to virtually eliminate background levels of extractives prior to use, and then heated to 100 ° C for 30 min before use to eliminate any volatiles that may have been absorbed during storage.
The micro extraction technique consists of several simple steps. For example, when a water sample is to be analyzed for certain analytes, it is placed in a hypo-vial (trade-mark) or other suitable gas tight enclosure. The assembly 1 is inserted through the Teflon face of the vial seal into the silicone backing. If a shielded fibre assembly (Fig. 3) is used, the support material extends through the vial seal . Single or multiple fibres can be provided with identical or different coatings. The vial is then made gas tight by crimping the seal into position. Other sealing techniques such as screw cap enclosures can be used.
A magnetic stir bar S which was enclosed with the sample prior to sealing the vial may be included. The sample may also be heated during extraction. The time required for extraction depends on many factors including the analytes being extracted as well as the thickness and type, if any, of coating on the support. However, extraction times would normally range from several to 60 minutes. The vial is then opened and the analytes contained in the fibre desorbed by immersion in a micro volume of solvent (typically 150 ~L) contained in a small conical shaped vial, such as a gas chromatograph autosampler vial. The fibre can remain in the autosampler vial.
If a shielded fibre is used (Fig. 3), the coating is retracted into the stainless steel tubing by pulling the cylindrical support lA( Fig. 3) into the tube before opening the vial. The fibre assembly is then extended out from the shield into a micro volume of solvent. The extracted analytes are analyzed by injecting portions of the solvent extract into a chromatograph through injection ports. Various injection ports would include "
programmable temperature", "split-splitless", "on-column" and "large solvent volume"
types.
Careful construction and the typical one- time use of the fibres allows low variation of extraction efficiencies amongst fibres.
Example 1 Salmon (Sg), was spiked with monobutyltin, dibutyltin and tributyltin (final concentration 100 ng/g salmon tissue). The sample was then hydrolyzed with tetramethylammonium hydroxide, derivatized with sodium tetraethylborate, and the resulting ethylated analytes then collected by fibre assembly for 60 minutes at room temperature. Analytes were then desorbed into 150 uL of isoctane. Analysis was by capillary gas chromatography-atomic emission spectrometry monitoring the Sn line 326 nm.
Figure Sa illustrates that relative standard deviations of extraction for tetraethyllead, tetraethyltin, di-n-propyl mercury and decane (from an aqueous solution spiked at a low ppb level) in two trials of five individual extractions ranged from only 3.5 to 8.8%.
Figure Sb demonstrates that even in the presence of a complex matrix (salmon hydrolysate) low ppb levels of ionic butyltins (derivatized in situ with sodium tetraethylborate) can be reproducibly extracted (11-15% RSD) using the described technique. These results, which are typical for the micro extraction technique, are comparable or superior to other analytical techniques. This consistency enables multiple simultaneous extractions to be conducted without costly automation, greatly enhancing sample throughput and quantitation. Further, since the analytes are desorbed into solvent, the extracts can be easily stored or collected until a convenient time for analysis. Solid phase micro extraction, however, is usually a sequential technique requiring the same device to be used repeatedly- this reduces sample throughput and analysis normally proceeds immediately after sampling. Also, since the analytes are usually thermally desorbed, there is no extract to archive or analyse by alternative analytical instrumentation.
The extraction process of the micro extraction technique is essentially that which occurs with solid phase micro extraction. The simple geometry of the fibre resists clogging from particulates which may be present in the sample matrix. Further, extraction is usually not exhaustive but rather an equilibrium described by the partition coefficient between the water and organic stationary phase for the analytes. Selectivity of the technique can be altered by the appropriate choice of stationary phase for the analytes of interest. The partitioning between the aqueous phase and the organic coating is described by the distribution constant, K:
K= CS/Caq ( 1 ) where CS is the concentration in the stationary phase (coating) and Caq is the concentration of analyte present in the water. Further, assuming a liquid polymeric coating, equation 2 shows that the amount of analyte extracted by the coating at equilibrium can be related directly to its concentration in the sample n=(KrSVeCoVs)/(KfSVr+VS) (2) where n is the mass of the analyte extracted by the coating, Vf and VS are the volumes of the coating and sample respectively, Kfs is the partition coefficient between the coating and the sample matrix, and Co is the initial concentration of the analyte in the sample.
However, headspace solid phase micro extraction is a three-phase system (equation 3) where n can be expressed as:
n=(~,KnsVtCoVs)/(K~,KnsVr~'KnsVh+VS) (3) when K,~, is the coating/gas distribution constant, Khs is the gas/sample matrix constant and V,, is the volume of the headspace. A linear relationship therefore exists between the amount of analytes extracted by the coating on the fibre and the initial concentration of these analytes in the sample.
The limit of quantitation depends on the partition coefficient and the thickness of the coating and can extend down to sub part per billion. The rate of the extraction process is S essentially the same as for solid phase micro extraction, where initially, the amount of analyte extracted by the coating (stationary phase) increases with increased extraction times until a point of steady state is achieved where the amount of analyte extracted remains relatively constant. At this point a state of equilibrium exists between the concentration of the analyte in the coating, headspace (if present) and in the sample matrix.
Example 2 The micro extraction technique is very versatile and can be used for a variety of analytes.
A 50 mL aqueous solution was spiked with a pesticide spike mixture (20-50 ng/uL) containing 1 ) gamma-BHC (lindane), 2) heptachlor, 3) aldrin, 4) dieldrin, 5) endrin and 6) 4,4'-DDT made up in methanol (final concentration 4-10 ng/mL water).
The sample was heated to 70°C and the analytes collected by fibre assembly for 4 hours.
The analytes were then desorbed into 150 uL of issoctane. Analysis was by capillary gas chromatography with electron capture detection.
Figure 6 shows a chromatogram of a chlorinated pesticide mixture (containing of 1 ) gamma-BHC (lindane), 2) heptachlor, 3) aldrin, 4) dieldrin, 5) endrin and 6) 4,4'-DDT, ) extracted from a low ppb-spiked aqueous solution, and analyzed from an aqueous solution by the micro extraction technique with an unshielded silicone coated fibre . The vapour pressure of these compounds range down to 1.5 x 10'' mm Hg at room temperature, demonstrating that even a relatively nonvolatile compound can be readily quantitated by this technique. A gas chromatograph equipped with an electron capture detector was used for the analysis.
Figure 1 is a schematic side view of a fibre assembly according to the invention;
S Figure 2 is an enlarged end view of a fibre assembly according to the invention;
Figure 3 is a schematic side view of a shielded fibre assembly according to the invention;
Figure 4 is a schematic side view of a fibre assembly installed in a typical sampling enclosure according to the invention;
Figure Sa illustrates the reproducibility of multiple extractions of tetraethyltin, tetraethyllead, di-n-propyl mercury and decane using the present technique from an aqueous solution;
Figure Sb illustrates the reproducibility of multiple extractions of ionic butyltin compounds (ethylated in situ) from a complex biological matrix using the present technique;
Figure 6 is a chromatogram of the extraction of a chlorinated pesticide mixture containing 1) gamma-BHC (lindane), 2) heptachlor, 3) aldrin, 4) dieldrin, 5) endrin and 6) 4,4'-DDT from an aqueous sample; and Figure 7 is a chromatogram of the extraction of a BTEX mixture containing 1) benzene, 2) toluene, 3) ethylbenzene, 4) p-xylene, 5) m-xylene and 6) o-xylene from an aqueous solution.
DETAILED DESCRIPTION OF THE INVENTION
Referring to figures 1 and 2, in detail, an assembly 1 for carrying out solid phase micro extraction is shown, comprising a cylindrical support lA, which may be in the form of a fibre, and which may have a length of coating 2 of which various types of organic compounds could be used. The diameter of the fibre may vary, but would generally be between 0.5 to 2 mm and it may be solid or hollow.
As seen in figure 3, a cylindrical support lA which has a length of coating, is mounted through a Teflon~ faced silicone septum 4. Stainless steel tubing 3 , which acts as a shield, of slightly longer length than the coating is mounted over the support lA. If the fibre is pulled up through the silicone septum, until the fibre coating is inside the stainless steel sleeve 3, the extracted analytes are shielded from volatizing into the atmosphere.
This permits short term storage or transport of the fibre assembly without having to immediately desorb the analytes into a solvent.
The coating is typically provided on the outside of solid fibres, and may be on the outside and/or the inside of hollow fibres.
In figure 4., the assembly 1 is mounted in a gas tight enclosure 2, typically but not exclusively a hypo-vial (trade mark) with an open top, closed by a crimp top (as illustrated) 3A, or screw cap and Teflon-faced seal 4A. Generally, a Teflon coated magnetic stir bar S is included to permit agitation of the sample 6 during extraction of the analytes by the fibre lA. The assembly 1 is positioned for head space sampling but can also used for direct (aqueous layer) sampling as well. Fibres can be manufactured with various coating lengths but 10 mm is the typical length used. Although longer lengths of coating can result in a greater amount of extracted analyte, for our purpose, a 10 mm length completely submerged in a 1 SO ~L volume of solvent is sufficient for adequate desorption. For multiple extraction chemistries or to increase the extraction efficiency, we would use mixed chemistry coatings or multiple fibres.
Fibres can be constructed with fused silica or other support material chemically or mechanically modified e.g. by roughening of the fibre surface to improve adhesion of the coating, followed by chemical attachment of the desired coating. Although there are both absorption and adsorption-type SPME coatings available, our fibres with a silicone coating would extract analytes by absorption, while porous polymer coatings (such as CarboxenTM) can extract suitable analytes by adsorption within the pore structure.
Alternatively, the support can be constructed from silicone (such as Dow Corning Silastic~ Q7-4750 (0.51 mm ID, 0.94 mm OD) that was used in our studies) or other polymer tubing lengths, swelled by solvent and then dried (to a tight fit) over metal wire or other cylindrical support material. Polymer tubing used for the support is exhaustively extracted by solvent to virtually eliminate background levels of extractives prior to use, and then heated to 100 ° C for 30 min before use to eliminate any volatiles that may have been absorbed during storage.
The micro extraction technique consists of several simple steps. For example, when a water sample is to be analyzed for certain analytes, it is placed in a hypo-vial (trade-mark) or other suitable gas tight enclosure. The assembly 1 is inserted through the Teflon face of the vial seal into the silicone backing. If a shielded fibre assembly (Fig. 3) is used, the support material extends through the vial seal . Single or multiple fibres can be provided with identical or different coatings. The vial is then made gas tight by crimping the seal into position. Other sealing techniques such as screw cap enclosures can be used.
A magnetic stir bar S which was enclosed with the sample prior to sealing the vial may be included. The sample may also be heated during extraction. The time required for extraction depends on many factors including the analytes being extracted as well as the thickness and type, if any, of coating on the support. However, extraction times would normally range from several to 60 minutes. The vial is then opened and the analytes contained in the fibre desorbed by immersion in a micro volume of solvent (typically 150 ~L) contained in a small conical shaped vial, such as a gas chromatograph autosampler vial. The fibre can remain in the autosampler vial.
If a shielded fibre is used (Fig. 3), the coating is retracted into the stainless steel tubing by pulling the cylindrical support lA( Fig. 3) into the tube before opening the vial. The fibre assembly is then extended out from the shield into a micro volume of solvent. The extracted analytes are analyzed by injecting portions of the solvent extract into a chromatograph through injection ports. Various injection ports would include "
programmable temperature", "split-splitless", "on-column" and "large solvent volume"
types.
Careful construction and the typical one- time use of the fibres allows low variation of extraction efficiencies amongst fibres.
Example 1 Salmon (Sg), was spiked with monobutyltin, dibutyltin and tributyltin (final concentration 100 ng/g salmon tissue). The sample was then hydrolyzed with tetramethylammonium hydroxide, derivatized with sodium tetraethylborate, and the resulting ethylated analytes then collected by fibre assembly for 60 minutes at room temperature. Analytes were then desorbed into 150 uL of isoctane. Analysis was by capillary gas chromatography-atomic emission spectrometry monitoring the Sn line 326 nm.
Figure Sa illustrates that relative standard deviations of extraction for tetraethyllead, tetraethyltin, di-n-propyl mercury and decane (from an aqueous solution spiked at a low ppb level) in two trials of five individual extractions ranged from only 3.5 to 8.8%.
Figure Sb demonstrates that even in the presence of a complex matrix (salmon hydrolysate) low ppb levels of ionic butyltins (derivatized in situ with sodium tetraethylborate) can be reproducibly extracted (11-15% RSD) using the described technique. These results, which are typical for the micro extraction technique, are comparable or superior to other analytical techniques. This consistency enables multiple simultaneous extractions to be conducted without costly automation, greatly enhancing sample throughput and quantitation. Further, since the analytes are desorbed into solvent, the extracts can be easily stored or collected until a convenient time for analysis. Solid phase micro extraction, however, is usually a sequential technique requiring the same device to be used repeatedly- this reduces sample throughput and analysis normally proceeds immediately after sampling. Also, since the analytes are usually thermally desorbed, there is no extract to archive or analyse by alternative analytical instrumentation.
The extraction process of the micro extraction technique is essentially that which occurs with solid phase micro extraction. The simple geometry of the fibre resists clogging from particulates which may be present in the sample matrix. Further, extraction is usually not exhaustive but rather an equilibrium described by the partition coefficient between the water and organic stationary phase for the analytes. Selectivity of the technique can be altered by the appropriate choice of stationary phase for the analytes of interest. The partitioning between the aqueous phase and the organic coating is described by the distribution constant, K:
K= CS/Caq ( 1 ) where CS is the concentration in the stationary phase (coating) and Caq is the concentration of analyte present in the water. Further, assuming a liquid polymeric coating, equation 2 shows that the amount of analyte extracted by the coating at equilibrium can be related directly to its concentration in the sample n=(KrSVeCoVs)/(KfSVr+VS) (2) where n is the mass of the analyte extracted by the coating, Vf and VS are the volumes of the coating and sample respectively, Kfs is the partition coefficient between the coating and the sample matrix, and Co is the initial concentration of the analyte in the sample.
However, headspace solid phase micro extraction is a three-phase system (equation 3) where n can be expressed as:
n=(~,KnsVtCoVs)/(K~,KnsVr~'KnsVh+VS) (3) when K,~, is the coating/gas distribution constant, Khs is the gas/sample matrix constant and V,, is the volume of the headspace. A linear relationship therefore exists between the amount of analytes extracted by the coating on the fibre and the initial concentration of these analytes in the sample.
The limit of quantitation depends on the partition coefficient and the thickness of the coating and can extend down to sub part per billion. The rate of the extraction process is S essentially the same as for solid phase micro extraction, where initially, the amount of analyte extracted by the coating (stationary phase) increases with increased extraction times until a point of steady state is achieved where the amount of analyte extracted remains relatively constant. At this point a state of equilibrium exists between the concentration of the analyte in the coating, headspace (if present) and in the sample matrix.
Example 2 The micro extraction technique is very versatile and can be used for a variety of analytes.
A 50 mL aqueous solution was spiked with a pesticide spike mixture (20-50 ng/uL) containing 1 ) gamma-BHC (lindane), 2) heptachlor, 3) aldrin, 4) dieldrin, 5) endrin and 6) 4,4'-DDT made up in methanol (final concentration 4-10 ng/mL water).
The sample was heated to 70°C and the analytes collected by fibre assembly for 4 hours.
The analytes were then desorbed into 150 uL of issoctane. Analysis was by capillary gas chromatography with electron capture detection.
Figure 6 shows a chromatogram of a chlorinated pesticide mixture (containing of 1 ) gamma-BHC (lindane), 2) heptachlor, 3) aldrin, 4) dieldrin, 5) endrin and 6) 4,4'-DDT, ) extracted from a low ppb-spiked aqueous solution, and analyzed from an aqueous solution by the micro extraction technique with an unshielded silicone coated fibre . The vapour pressure of these compounds range down to 1.5 x 10'' mm Hg at room temperature, demonstrating that even a relatively nonvolatile compound can be readily quantitated by this technique. A gas chromatograph equipped with an electron capture detector was used for the analysis.
Example 3 A 50 mL aqueous solution was spiked with a BTEX mixture (200 ng/uL) containing benzene, ethylbenzene, toluene, m-xylene, o-xylene, andp-xylene made up in methanol (final concentration 40 ng/mL water). The analytes were collected by fibre assembly at room temperature for 60 minutes. The analytes were then desorbed with 150 uL of issoctane. Analysis was by capillary gas chromatography using flame ionization detection.
Figure 7 shows the chromatogram of a BTEX mixture containing 1) benzene, 2) toluene, 3) ethylbenzene, 4) p-xylene, 5) m-xylene and 6) o-xylene extracted from a low ppb-spiked aqueous solution, and analysed by the micro extraction technique using a unshielded silicone coated fibre. All of the components are present and readily quantitated by FID detector, illustrating that significant sample preconcentration is 1 S possible with micro solvent volume desorption of the fibres.
The micro extraction technique can be applied to any analysis suited to solid phase micro extraction since it can be transported for remote sampling, is amenable to existing analytical instrumentation and is quite flexible in terms of coatings. The ability to use multiple fibre assemblies would permit different coating chemistries to simultaneously extract a single sample. Further, since multiple samples can be extracted simultaneously, sample throughput is very high, permitting faster calibration and quantitation of samples.
Fibres of various materials can be used depending upon the intended use, includng fused silica, graphite, various solid polymers and metals.
Examples of fibre coatings include: Carbowax (trade mark for polyethyleneglycols and methoxypolyethyleneglycols), silicone, polyimide, divinylbenzene, polyacrylate, carbon-based sorbents, ion-exchange materials and other materials readily apparent to skilled chemical analysts including those described in US Patent no. 5,691,206, the disclosure of which is incorporated herein by reference.
The solvent may be any suitable organic solvent known to those skilled in the art of chemical analysis e.g. isoctane.
The micro extraction technique can be used with many different analytical methods, including gas, liquid or supercritical fluid chromatography, atomic absorption or emission, mass spectrometry, and infrared absorption spectrometry.
It will also be appreciated that the method and apparatus according to the invention can be used for analysing not only environmental, biomedical and pharmaceutical samples, but also industrial process streams, chemical reactions, and air monitoring.
Further applications will be readily apparent to those skilled in the art.
Figure 7 shows the chromatogram of a BTEX mixture containing 1) benzene, 2) toluene, 3) ethylbenzene, 4) p-xylene, 5) m-xylene and 6) o-xylene extracted from a low ppb-spiked aqueous solution, and analysed by the micro extraction technique using a unshielded silicone coated fibre. All of the components are present and readily quantitated by FID detector, illustrating that significant sample preconcentration is 1 S possible with micro solvent volume desorption of the fibres.
The micro extraction technique can be applied to any analysis suited to solid phase micro extraction since it can be transported for remote sampling, is amenable to existing analytical instrumentation and is quite flexible in terms of coatings. The ability to use multiple fibre assemblies would permit different coating chemistries to simultaneously extract a single sample. Further, since multiple samples can be extracted simultaneously, sample throughput is very high, permitting faster calibration and quantitation of samples.
Fibres of various materials can be used depending upon the intended use, includng fused silica, graphite, various solid polymers and metals.
Examples of fibre coatings include: Carbowax (trade mark for polyethyleneglycols and methoxypolyethyleneglycols), silicone, polyimide, divinylbenzene, polyacrylate, carbon-based sorbents, ion-exchange materials and other materials readily apparent to skilled chemical analysts including those described in US Patent no. 5,691,206, the disclosure of which is incorporated herein by reference.
The solvent may be any suitable organic solvent known to those skilled in the art of chemical analysis e.g. isoctane.
The micro extraction technique can be used with many different analytical methods, including gas, liquid or supercritical fluid chromatography, atomic absorption or emission, mass spectrometry, and infrared absorption spectrometry.
It will also be appreciated that the method and apparatus according to the invention can be used for analysing not only environmental, biomedical and pharmaceutical samples, but also industrial process streams, chemical reactions, and air monitoring.
Further applications will be readily apparent to those skilled in the art.
Claims (19)
1. An apparatus for carrying out solid phase microextraction of analytes included in a fluid or a solid sample, comprising gas tight enclosure means, means for introducing a sample including target analytes into the enclosure means, and means located within the enclosure means for extracting the target analytes from the sample, wherein the extraction means either samples a head space near the sample or samples the sample directly.
2. An apparatus according to Claim 1, wherein the extraction means includes a solid support, which may be coated or uncoated, the solid support and/or the coating being selected, based upon selectivity of the support and/or coating for at least one of the analytes present in the sample.
3. An apparatus according to Claim 2, wherein the support is a cylindrical support.
4. An apparatus according to Claim 3, wherein the cylindrical support is in the form of a fibre.
5. An apparatus according to Claim 3, additionally comprising means for shielding the cylindrical support from the atmosphere.
6. An apparatus according to Claim 2, additionally comprising means for desorbing the target analytes, located outside of the gas tight enclosure means.
7. An apparatus according to Claim 4, wherein the coating is an organic material selected from the group consisting of Carbowax~, silicone, polyimide, divinylbenzene, polyacrylate, carbon-based sorbents and ion-exchange materials.
8. An apparatus according to Claim 4, wherein the solid support is of a material selected from the group consisting of fused silica, graphite, solid polymers and metals .
9. An apparatus according to Claim 4, wherein the fibre is of fused silica, and the coating is of silicone.
10. A method for solid phase micro extraction of analytes included in a fluid or a solid sample, comprising (c) exposing a fluid or a solid sample including target analytes, to a solid support which may be coated or uncoated, the support and/or the coating being selected based upon selectivity of the support and/or coating for at least one of the analytes in the sample, for a sufficient time to permit chemical extraction of the analytes by the support to occur, and (d) ending said contact and then placing said solid support into a micro volume of solvent where chemical desorption of the analytes from the support occurs.
11. A method according to Claim 10, wherein the support is in the form of a fibre.
12. A method according to Claim 11, wherein the method is effected within a gas tight enclosure.
13. A method according to Claim 12, wherein the solvent is a suitable organic solvent.
14. A method according to Claim 10, wherein the chemical extraction is by absorption or adsorption of the target analyte by the solid support or coating.
15. A method according to Claim 10, wherein the sample is in an aqueous solution.
16. A method according to Claim 10 wherein the support is uncoated.
17. A method according to Claim 16, wherein the support is of fused silica.
18. A method according to Claim 10, wherein the support is coated with an organic material selected from the group consisting of Carbowax~, silicone, polyimide, divinylbenzene, polyacrylate, carbon-based sorbents and ion-exchange materials.
19. A method according to Claim 18, wherein the coating is silicone.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CA 2315474 CA2315474A1 (en) | 1999-08-12 | 2000-08-10 | Micro extraction technique |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CA2,280,418 | 1999-08-12 | ||
| CA002280418A CA2280418A1 (en) | 1999-08-12 | 1999-08-12 | Micro extraction technique |
| CA 2315474 CA2315474A1 (en) | 1999-08-12 | 2000-08-10 | Micro extraction technique |
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| Publication Number | Publication Date |
|---|---|
| CA2315474A1 true CA2315474A1 (en) | 2001-02-12 |
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA 2315474 Abandoned CA2315474A1 (en) | 1999-08-12 | 2000-08-10 | Micro extraction technique |
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| CA (1) | CA2315474A1 (en) |
Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| GB2401174A (en) * | 2003-04-30 | 2004-11-03 | Ecolab Sevices Ltd | Microextraction device for trace volatiles |
| CN102489105A (en) * | 2011-11-29 | 2012-06-13 | 南昌航空大学 | Air treatment device |
| WO2016045030A1 (en) * | 2014-09-25 | 2016-03-31 | 深圳粤网节能技术服务有限公司 | Graphene material-based dispersive solid phase extraction method |
-
2000
- 2000-08-10 CA CA 2315474 patent/CA2315474A1/en not_active Abandoned
Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| GB2401174A (en) * | 2003-04-30 | 2004-11-03 | Ecolab Sevices Ltd | Microextraction device for trace volatiles |
| GB2401174B (en) * | 2003-04-30 | 2007-02-21 | Ecolab Sevices Ltd | Method and apparatus for detection of trace volatiles |
| CN102489105A (en) * | 2011-11-29 | 2012-06-13 | 南昌航空大学 | Air treatment device |
| WO2016045030A1 (en) * | 2014-09-25 | 2016-03-31 | 深圳粤网节能技术服务有限公司 | Graphene material-based dispersive solid phase extraction method |
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