EP1680212A2 - Membranen und laminate enthaltende reagenzien sowie verfahren zu ihrer herstellung - Google Patents

Membranen und laminate enthaltende reagenzien sowie verfahren zu ihrer herstellung

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Publication number
EP1680212A2
EP1680212A2 EP04786030A EP04786030A EP1680212A2 EP 1680212 A2 EP1680212 A2 EP 1680212A2 EP 04786030 A EP04786030 A EP 04786030A EP 04786030 A EP04786030 A EP 04786030A EP 1680212 A2 EP1680212 A2 EP 1680212A2
Authority
EP
European Patent Office
Prior art keywords
membrane
reagent
laminate
sample
hdl
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Withdrawn
Application number
EP04786030A
Other languages
English (en)
French (fr)
Inventor
Ronald M. Jones
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Cholestech Corp
Original Assignee
Cholestech Corp
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Cholestech Corp filed Critical Cholestech Corp
Publication of EP1680212A2 publication Critical patent/EP1680212A2/de
Withdrawn legal-status Critical Current

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Classifications

    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/92Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving lipids, e.g. cholesterol, lipoproteins, or their receptors
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K9/00Medicinal preparations characterised by special physical form
    • A61K9/70Web, sheet or filament bases ; Films; Fibres of the matrix type containing drug
    • A61K9/7007Drug-containing films, membranes or sheets
    • BPERFORMING OPERATIONS; TRANSPORTING
    • B01PHYSICAL OR CHEMICAL PROCESSES OR APPARATUS IN GENERAL
    • B01DSEPARATION
    • B01D67/00Processes specially adapted for manufacturing semi-permeable membranes for separation processes or apparatus
    • B01D67/0081After-treatment of organic or inorganic membranes
    • B01D67/0088Physical treatment with compounds, e.g. swelling, coating or impregnation

Definitions

  • the present invention relates to a method of impregnating a membrane or membrane laminate with a uniform and controlled amount of reagent.
  • the invention relates to preparing membrane laminates containing impregnated reagents, where the reagents are limited to a single respective layer of the laminate, and to such reagent-containing membranes and laminates and assay devices containing them.
  • Diagnostic assays employing a strip format, where a porous material such as a fibrous strip or membrane is impregnated with diagnostic reagents, are in common use due to convenience, speed and reduced need for manipulation of reagents by the user. Uniform and reproducible application of reagents is important in the production of such devices, to ensure consistency and accuracy of test results.
  • a porous membrane can be impregnated with a reagent simply by contacting the membrane with a solution of the reagent.
  • a saturating amount of solution is typically used.
  • this approach often produces non-uniform distribution of reagents.
  • it is unsatisfactory for laminated membranes, since it generally does not limit dispersion of the reagent to a single layer, particularly if the layers are of similar materials.
  • Spray coating or syringe coating of reagent to a surface of a membrane or lami- can provide better control of the amount of reagent applied, thus reducing the risk of dispersion to underlying layers in a laminate.
  • coating by these methods also tends to be non-uniform, producing concentration gradients with more reagent in the center of the application area.
  • HDL high-density lipoprotein
  • Said reagent pad is produced by dispensing aqueous solution containing dextrane sulfate onto an asymmetric membrane in a certain dispensing rate.
  • the HDL-reaction membrane is impregnated with an aqueous formulation.
  • the two impregnated membranes are separately or simultaneously attached by ultrasonic welding.
  • the invention provides a method of applying a reagent to a membrane in a membrane laminate, comprising first and second laminated membranes.
  • the method comprises: (a) providing a laminate of the first and second membranes, having an outer first membrane surface, a laminated first membrane surface, a laminated second membrane surface, and an outer second membrane surface; (b) applying a controlled volume of a solution of a first reagent to the outer first membrane surface, by contacting the surface with a support having a surface containing a pattern, and (c) drying the first membrane in the laminate, to produce a laminate containing the first membrane impregnated with the first reagent, wherein the first reagent does not contact the second membrane in the laminate.
  • the method applies said solution by means of a pattern comprising recesses filled with said solution, or by means of a pattern comprising projections applying said solution.
  • said support preferably comprises a planar or cylindrical shape.
  • the method further comprises impregnating the second layer with a second reagent, by (d) applying a controlled volume of a solution of the second reagent to the outer second membrane surface, by contacting the surface with a solid support containing recesses filled with the solution, and (e) drying the second membrane in the laminate, to produce a laminate containing the second membrane impregnated with the second reagent, wherein the second reagent does not contact the first membrane in the laminate.
  • a second reagent by (d) applying a controlled volume of a solution of the second reagent to the outer second membrane surface, by contacting the surface with a solid support containing recesses filled with the solution, and (e) drying the second membrane in the laminate, to produce a laminate containing the second membrane impregnated with the second reagent, wherein the second reagent does not contact the first membrane in the laminate.
  • the solid support is a rotating gravure cylinder, having a plurality of recesses or cells formed in the surface, as discussed further below.
  • said applying occurs simultaneously across the entire width of the first membrane outer surface, to produce a uniform application across the width of the membrane.
  • the "controlled volume" of solution is generally no more than a saturating amount of the solution, with respect to the absorptive capacity of the respective membrane, and is typically a subsaturating amount, as defined below.
  • a given (first or second) reagent does not contact the laminated surface of the respective membrane in the finished laminate; that is, it penetrates only partially through the depth of the respective membrane.
  • a given (first or second) reagent contacts the laminated surface of the respective membrane in the finished laminate; that is, it impregnates the full thickness of the respective membrane, but it does not contact the other membrane in the laminate.
  • the first membrane is an asymmetric membrane, i.e. having a small pored surface and a large pored surface.
  • the second membrane may also be an asymmetric membrane, h selected embodiments, the outer first membrane surface is the large pored surface of the first membrane. In a further embodiment, the outer second membrane surface is the small pored surface of the second membrane.
  • Fig. 1 shows a laminate 10 of first membrane 12 and second layer 14, having outer first membrane surface 16, laminated first membrane surface 18, laminated second membrane surface 20, and outer second membrane surface 22. The laminated first membrane surface and laminated second membrane surface jointly form a laminate interface.
  • At least one of the reagents may be a heat sensitive reagent, such that laminating a membrane containing said reagent to a further membrane would produce a detrimental change in the reagent.
  • the first reagent comprises reagents effective to selectively remove non-HDL lipoproteins from a blood fluid sample passing through the first membrane
  • the second reagent comprises reagents effective to produce an optically detectable signal proportional to a quantity of HDL- associated cholesterol in the second membrane.
  • the invention provides a method of applying a reagent to a membrane, by applying a controlled volume of a solution of said reagent to a first surface of the membrane, by contacting the surface with a planar or cylindrical support having a surface containing a pattern of recesses filled with the solution.
  • the support is typically a rotating gravure cylinder.
  • the techniques and apparatus are preferably used which are described for applying reagents to a membrane in a membrane laminate.
  • the controlled amount of reagent may be a subsaturating amount.
  • the reagent does not contact the opposite surface of said membrane; that is, it penetrates only partially through the depth of the membrane.
  • the application of reagent preferably occurs simultaneously across the entire width of the first surface of the membrane. Accordingly, the concentration of the reagent is preferably uniform across the length and width of said membrane.
  • the membrane may be an asymmetric membrane, having a small pored surface and a large pored surface; in one embodiment, the first surface, to which reagent is applied, is the large pored surface. In other embodiments, the first surface is the small pored surface.
  • the reagent comprises reagents effective to selectively remove non-HDL lipoproteins from a blood fluid sample passing through the membrane; alternatively, the reagent includes reagents effective to selectively precipitate non-HDL (LDL and VLDL) lipoprotein particles in the sample, and the precipitated LDL and VLDL particles are prevented by filtration from passing through the membrane. In this embodiment, when the membrane is an asymmetric membrane, the reagent is applied to the large pored surface.
  • the reagent comprises reagents effective to produce an optically detectable signal proportional to a quantity of HDL-associated choleste- rol in the membrane.
  • the reagent is applied to the small pored surface.
  • the invention provides a membrane laminate for use in a diagnostic assay, comprising first and second laminated membranes which are joined at a laminate interface, wherein the first membrane in said laminate is im- pregnated with a first reagent, the second membrane is impregnated with a second reagent, and the reagent in at least one of the membranes is absent in a laminar region of that membrane adjacent the laminate interface, such that the reagents in the two membranes are physically separated by at least that laminar region.
  • the concentration of each reagent or reagent system is uniform across the length and width of the respective membrane.
  • At least one said reagent is heat sensitive, such that laminating a membrane containing said reagent to a further membrane would produce a detrimental change in the reagent.
  • the first membrane is an asymmetric membrane, having a small pored surface and a large pored surface.
  • the small pored surface faces the laminate interface.
  • the second membrane may also be an asymmetric membrane; in selected embodiments, its large pored surface faces the laminate interface.
  • the first reagent comprises reagents effective to selectively remove non-HDL lipoproteins from a blood fluid sample passing through said first membrane; alternatively, the first reagent includes reagents effective to selectively precipitate non-HDL (LDL and VLDL) lipoprotein particles in the sample, and the precipitated LDL and VLDL particles are prevented by filtration from passing through the laminate interface.
  • the second reagent comprises reagents effective to produce an optically detectable signal proportional to a quantity of HDL-associated cholesterol in the second membrane.
  • the reagent in the second membrane is absent in a laminar region of that membrane adjacent the laminate interface.
  • the invention provides an assay device for assaying HDL in a blood or serum sample, comprising (a) a substrate having a sample-receiving well for receiving an aliquot of the sample, (b) a membrane laminate comprising first and second laminated membranes which are joined at a laminate interface, wherein (i) the first membrane is impregnated with reagents effective to selectively precipitate LDL and VLDL lipoprotein particles in the sample, and the precipitated LDL and VLDL particles are prevented by filtration from passing through the laminate interface; (ii) the second membrane is impregnated with reagents effective to produce an optically detectable signal proportional to a quantity of HDL-associated cholesterol in the second membrane; and (iii) the reagent in at least one of the membranes, and preferably the second membrane, is absent in a laminar region of that membrane adjacent the laminate interface, such that the reagents in the two membranes are physically separated by at least that laminar region.
  • the concentration of each reagent is preferably uniform across the length and width of the membrane.
  • the device also comprises (c) a filter between the sample-receiving well and the first membrane of the laminate, for removing red blood cells in the sample as the sample migrates from the sample-receiving well to the laminate, wherein the well, filter and laminate are or can be placed in fluid communication with each other.
  • Figure 1 is a cross section view of two laminated asymmetric membranes to which reagents may be applied in accordance with one embodiment of the invention
  • Figure 2 is a schematic diagram showing a coating system for application of reagents to a laminate, in accordance with one embodiment of the invention
  • Figure 3 is a side view of an assay device incorporating a membrane laminate, in accordance with one embodiment of the invention.
  • the invention provides methods of impregnating or coating a laminate of at least two membranes with at least one reagent, such that each reagent is confined to its respective membrane.
  • the laminate includes at least two membranes, each containing a different reagent or reagent system.
  • a laminate used in a device designed for measuring the concentration of HDL-associated cholesterol in a blood sample which also containing LDL and VLDL particles. See, for example, Jones et ah, US Appn. Pubn. No. 20030166291 and US Appn. Serial No. 10/410,671, which are incorporated herein by reference.
  • the invention is useful for any application employing a laminate as described above, having reagents impregnated in at least one, and preferably two, membrane layers, where each reagent must be confined to its respective layer.
  • the exemplary HDL assay laminate includes an HDL test membrane, in which HDL concentration is measured, and a reagent membrane, containing a binding and/or precipitation reagent, such that the membrane is effecti- ve to selectively remove non-HDL lipoproteins from the fluid sample, before the sample contacts the test membrane.
  • each of the membranes in the laminate is a porous asymmetric membrane; that is, a membrane having a pore size gradient across its thickness.
  • An e- xemplary two-membrane layer 10 comprising two asymmetric membranes 12 and 14 is shown in cross section in Fig. 1, with the preferred orientation shown, with larger pores at 24 and smaller pores at 26 in membrane 12.
  • the HDL test reagent In order for the HDL assay to function accurately, the HDL test reagent must be restricted to it respective layer. If the HDL reagent is present in the reagent layer, the color developed in the assay reaction will generally represent some fraction of non-HDL cholesterol in addition to the analyte, HDL-associated cholesterol.
  • a gravure printing process in which fluid is applied to a substrate from recesses in a solid plate having planar or arbitrary shape, or, typically, a rotating cylinder, allows controlled- volume deposition of different reagents to opposite surfaces of a laminated membrane. By controlling the deposition volume, each reagent can be limited to its respective layer in the laminate.
  • the rea- gents are applied to separate membranes or membrane laminates by a letterpress technique.
  • the support has a planar or arbitrary suitable configuration, preferably the configuration of a cylinder.
  • Said support comprises a pattern of projections applying the reagents to the membrane.
  • said reagents are provided having a consistency to temporarily adhere to said projections so that they are applied in a controlled manner.
  • a network of depressions is etched on the surface of a metal cylinder.
  • the cells are loaded with fluid, and the rotating cylinder transfers the fluid to a substrate.
  • the cells have a defined volu- me, thus limiting the amount of liquid that can be transferred to the substrate.
  • a cylinder has a volume of about 30-50 ⁇ l per square inch of cylinder sur- face (about 4.5 - 8 ⁇ l per cm 2 ).
  • cylinder surface assumes a smooth surface, corresponding to the surface area of the substrate contacted by the cylinder. It does not include the additional surface area provided by the recesses themselves.
  • Other volume capacities can also be used.
  • the recesses are generally uni- formly sized and closely spaced, such that, upon transfer of liquid drops to the membrane, they coalesce into a uniform layer of liquid.
  • a gravure coating system that may be used in carrying out the processes described herein is shown at 30 in Fig. 2.
  • coating includes applying a reagent such that it penetrates beyond the surface and may impregnate the entire thickness of the membrane.
  • the laminated membrane or "web” 32 is fed from a roll 34.
  • the gravure cylinder 36 is typically copper or copper-plated steel or aluminum; a thin layer of chrome is often applied for durability.
  • the surface of the cylinder is etched with a plurality of small cells effective to hold a defined quantity of liquid.
  • a cylinder is chosen with a pattern of wells that is effective to apply a uniform coating with the given coating system.
  • the cylinder may be partially submerged in a bath or tray of the fluid to be applied.
  • a reagent chamber 38 may be used to deliver reagent solution to the cylinder via conduits 40. The chamber reduces exposure of the reagents to the atmosphere.
  • the excess solution is wiped off the cylinder by a flexible doctor blade 41 which contacts the cylinder between the reagent chamber or tray and the membrane 32. Solution remaining in the recessed cells is then transferred to the desired surface of the membrane.
  • the membrane 32 is held in tangential contact (i.e., contacting a few degrees of the circumference of the cylinder) with the gravure cylinder by a takeup cylinder 42, a process referred to as "kiss" gravure .
  • a takeup cylinder 42 a process referred to as "kiss" gravure .
  • the web ay pass between the gravure cylinder 36 and an impression or "backup" cylinder, as shown at 42'.
  • takeup cylinder 42 is generally absent.
  • fluid is transferred from the gravure cylinder to a rubber coated transfer roll, which then applies the solution to the substrate.
  • the substrate is then passed through a dryer 44, preferably an TR dryer blower, and taken up on takeup roll 46.
  • a dryer 44 preferably an TR dryer blower
  • takeup roll 46 The other surface of the laminate is then coated in a similar manner.
  • the gravure coating process may be carried out in a direct mode, where the cylinder rotates in the same direction as the membrane feed.
  • the rotational direction of the cylinder is opposite to the travel direction of the membrane. This arrangement results in a shearing force being applied to the solution as it is transferred to the substrate, which can result in a smoother coating.
  • the volume of reagent solution applied to the membrane as it contacts the gravure roll is limited by the volume of the cells on the cylinder surface, as noted above.
  • the amount actually transferred from the cells to the membrane depends on addi- tional factors, such as cylinder speed, roll pressure, web speed, and solution components. Accordingly, the amount transferred to the membrane can be further controlled by proper selection of the system configuration, contact time between the membrane and cylinder (determined by web speed and direction relative to gravure rotation speed and direction) and surfactant level.
  • Surfactant is included to facilitate transfer of the solution to the membrane surface, which might otherwise repel an aqueous solution, depending on the hydrophobicity of the membrane material.
  • the penetration of reagent into the membranes is also dependent on pore size and distribution.
  • solution applied to surface 16 large pored
  • solution applied to surface 22 small pored
  • a controlled volume of reagent solution to one side of a membrane on the outer surface of a laminate, followed by drying, produces a laminate in which the reagent does not penetrate beyond that membrane.
  • the controlled amount may be a subsaturating amount; that is, a volume of the solution which is less than that which would, if applied to a selected membrane, penetrate the entire membrane by capillary flow. In some cases, a saturating or near-saturating volume may be used.
  • an amount of reagent solution is applied to the membrane to give the desired amount of penetration into the thickness or depth of the membrane.
  • the application method also provides a uniform concentration of reagent across the length and width of the membrane.
  • uniform is meant that there are no significant concentration gradients or changes across the length or width of the membrane. This uniformity is effective to give consistent assay readings for sample presented to different points on the surface of the laminate.
  • the amount of reagent present at different points on the surface of a membrane in the laminate, or at different points on a given laminar surface parallel to this surface varies by no more than a- bout 5%.
  • the application method is useful for heat sensitive reagents, where lamination of a membrane containing the reagent, under normal thermal lamination conditions, would produce a detrimental change in the reagent and/or its function in an assay carried out on the laminate. Such a change could include a change in the morphology or distribution of the reagent as well as chemical changes in the reagent.
  • the application method may also be advantageously used to apply a controlled a- mount of reagent in a uniform manner to a single membrane, by contacting the surface of the membrane with a planar or cylindrical support having a surface containing a pattern of recesses filled with the solution. Again, the support is typi- cally a rotating gravure cylinder, as described above.
  • the application of reagent by this method preferably occurs simultaneously across the entire width of the first surface of the membrane; accordingly, the concentration of the reagent is substantially uniform across the length and width of the membrane.
  • the controlled amount of reagent may be a subsaturating amount.
  • the reagent following application of reagent and, preferably, drying, the reagent does not contact the opposite surface of the membrane; that is, it penetrates only partially through the depth of the membrane.
  • the method is advantageous even when a saturating amount is to be applied, in that it produces a membrane in which reagents are impregnated more uniformly, as compared to prior art methods such as submersion in a saturating amount of solution or spray coating.
  • the invention also provides membranes impregnated with reagents in accordance with this method.
  • membranes for use in diagnostic assays.
  • the membrane may be an asymmetric membrane, having a small pored surface and a large pored surface; the reagent may be applied to either surface.
  • the reagent comprises reagents effective to selectively remove non-HDL lipoproteins from a blood fluid sample passing through the membrane; alternatively, the reagent includes reagents effective to selectively precipitate non-HDL (LDL and VLDL) lipoprotein particles in the sample, and the precipitated LDL and VLDL particles are prevented by filtration from passing through the membrane.
  • the reagent is preferably applied to the large pored surface.
  • the reagent comprises reagents effective to produce an optically detectable signal proportional to a quantity of HDL-associated cholesterol in the membrane.
  • the reagent is preferably applied to the small pored surface.
  • the invention provides laminated membranes having reagents impregnated in at least one, and preferably two, membrane layers, where each reagent (or reagent system) is confined to its respective layer.
  • each reagent or reagent system
  • different layers contain different reagent systems.
  • the reagent is applied to a laminated membrane in accordance with the methods described above.
  • membrane laminates for use in diagnostic assays.
  • Such a laminate comprises first and second laminated membranes, impregnated with first and second reagents, respectively, which are joined at a laminate interface. At least one of the first and second reagents is absent in a laminar region of the respective membrane adjacent the laminate interface, such that the reagents in the two membranes are physically separated by at least that laminar region.
  • the concentration of each said reagent is uniform across the length and width of the respective membrane containing that reagent. This uniformity is effective to give consistent assay readings for sample presented to different points on the surface of the laminate.
  • the amount of reagent present at different points on the surface of a membrane in the laminate, or at different points on a given laminar surface parallel to this surface varies by no more than about 5%.
  • the laminate is one designed for use in determining the level of HDL-associated cholesterol in a fluid sample. See, for example, Jones et al, US Appn. Pubn. No. 20030166291 and US Appn. Serial No. 10/410,671, cited above.
  • the first membrane contains reagents effective to selectively remove non-HDL lipoproteins from a blood fluid sample passing through the membrane.
  • the non-HDL lipoproteins may be removed, for example, by selective binding to a reagent contained or immobilized within the membrane.
  • these components are removed by selective precipitation by the reagent and are pre- vented by filtration from passing through the laminate interface into the second membrane.
  • Such reagents include polyanionic compounds, such as sulfonated polysaccharides, heparin, or phosphotungstate, in combination with a group LI cation, such as Mg 2+ , Mn 2+ , or Ca 2+ .
  • a preferred reagent is a sulfonated polysaccharide, such as dextran sulfate, having a typical molecular weight of 50-500 KDa, in combination with magnesium acetate or chloride, optionally buffered to maintain neutral pH.
  • the reagents may also be immobilized to the membrane.
  • the HDL test membrane contains reagents for quantification of HDL-associated cholesterol, as is known in the art. See, for example, co-owned U.S. Patent Nos. 5,213,964, 5,213,965, 5,316,196 and 5,451,370, each of which is incorporated herein by reference.
  • the assay reagents include cholesterol esterase, for releasing free cholesterol from HDL, cholesterol oxidase, for producing H 2 O 2 by reaction with free cholesterol, peroxidase, and a coupled dye system which is converted, in the presence of peroxidase and H 2 O 2 , to a distinctively colored signal reaction product.
  • Assay reagents are known in the art for quantification of other blood components, e.g. total cholesterol, triglycerides, or glucose, and frequently comprise similar enzyme/coupled dye systems.
  • the first membrane is an asymmetric membrane, having a small pored surface and a large pored surface.
  • the small pored surface preferably faces the laminate interface, such that the large pored surface is on the outer surface of the laminate. This orientation allows free access of sample into the membrane through the larger pores, and prevents passage of any precipitated or other solid material through the smaller pores.
  • the second membrane may also be an asymmetric membrane, preferably having its large pored surface facing the laminate interface, and the small pored surface on the other surface of the laminate. This orientation presents the more uniform surface of the membrane for optical scanning and quanti- tation of assay results.
  • Materials of fabrication include polysulfones, polyethersulfones, polyamides, polyether amides, polyurethanes, cellulose acetate, polyvinyl pyrrolido- ne, polystyrenes and modified polystyrenes, as well as blends, copolymers, and laminar composites.
  • preferred membrane types see e.g. US Appn. Pubn. No. 20030166291 and US Appn. Serial No. 10/410,671, cited above.
  • An exemplary asymmetric membrane is a polysulfone or polyethersulfone membrane, such as BTS 83 membranes provided by Pall Corporation (San Diego, CA).
  • each membrane typically has a thickness of about 100-150 ⁇ m and an absorption capacity of about 80 ⁇ l/sq in (about 12.4 ⁇ l/cm 2 ).
  • Minimum pore sizes typically range from 0.01 to 10 ⁇ m, with maximum/minimum pore size ratios up to 100 or more.
  • the laminate includes at least one reagent which is heat sensitive, such that laminating a membrane containing the reagent to a further membrane produces a detrimental change in the reagent.
  • the detrimental change could include any or all or a change in morphology, distribution or the actual chemical structure of the reagent.
  • an assay device for assaying HDL in a blood or serum sample comprises: (a) a substrate having a sample-receiving well for receiving an aliquot of a blood fluid sample, (b) a membrane laminate comprising first and second laminated membranes which are joined at a laminate interface, and (c) a filter between the sample-receiving well and the first membrane of the laminate, for removing red blood cells in the sample, as the sample migrates from the sample-receiving well to the laminate.
  • the membrane laminate of (b) is a laminate as described above, where the first membrane is impregnated with reagents effective to selectively precipitate non-HDL (LDL and VLDL) lipoprotein particles in said sample, and the precipitated LDL and VLDL particles are prevented by filtration from passing through the laminate interface; the second membrane is impregnated with reagents effective to produce an optically detectable signal proportional to a quantity of HDL-associated cholesterol in said second membrane; and the reagent in at least one of these membranes is absent in a laminar region of that membrane adjacent the laminate interface, such that the reagents in the two membranes are physically separated by at least that laminar region. It is particularly preferred that the HDL assay reagents are absent in a laminar region of the second membrane adjacent the laminate interface.
  • the concentration of each reagent is uniform across the length and width of the membrane containing the reagent, as described above.
  • the membranes are preferably asymmetric membranes, oriented as described above, where the outer surface of the reagent membrane is the large pored (dull) surface and the outer surface of the assay membrane is the small pored (shiny) surface.
  • the sample well, filter and laminate of (a)-(c) above are or can be placed in fluid communication with each other.
  • these elements may reside on a common substrate, or they may reside on one or more separate substrates and be brought into fluid communication during the course of the assay.
  • Different embodiments of such an assay device include those described in Jones et ah, US Appn. Pubn. No. 20030166291 and US Appn. Serial No. 10/410,671, cited above.
  • the apparatus 50 includes a main body or sup- port 52 which defines the sample well 54.
  • the well is in fluid contact with a sieving pad 60, which maybe carried in a notched region 58 formed in the upper edge of the support.
  • the fluid contact may be direct, or as in the device shown in Fig. 3, provided by a capillary conduit 56 formed in the plate at the base of the well.
  • the support is preferably a plastic plate, with the well, notched region and or capillary formed by standard molding or machining methods.
  • Sieving pad 60 carried in region 58 functions to partially remove large particulate matter (including blood cells) as the sample migrates through the pad matrix in a bottom-to-top direction as shown in the figure.
  • Pad 60 is preferably formed of a glass fibrous matrix of material designed to draw aqueous fluid by surface wetting, and to retard the movement of blood cells as the blood sample is drawn through the matrix.
  • One exemplary pad is a glass fiber filter, such as a GF/D or PD008 filter supplied by Whatman.
  • the pad is dimensioned to absorb a defined volume of sample fluid, e.g. about 15-25 ⁇ .
  • Sieving pad 60 may additionally contain red blood cell capture rea- gents, such as lectins, antibodies specific for red blood cell surface membrane proteins, thrombin, or ion exchange agents.
  • the sieving pad, 60 contacts an elongate strip or sample distribution matrix
  • Matrix 62 which extends along the upper edge of plate 52. This strip may also be supported by foam cushions or other supports.
  • Matrix 62 serves to distribute sample fluid from a central sample-application region 64, which is in fluid contact with pad 60, to sam- pie-collection regions such as 66, 68 within the matrix.
  • the matrix is preferably formed of glass fibers. The packing density and thickness of the matrix are such as to absorb and distribute volumes of sample fluid, e.g., 10-25 ⁇ , supplied to the sample- application region of the strip to the sample-collection regions of the strip.
  • One e- xemplary strip material is a F- 165-25 A glass fiber filter available from Whatman, having a packing density of about 0.2 gm/cm 3 and a thickness of about 0.12 mm.
  • Device 50 also includes a reaction bar 70 composed of an elongate support 72, and one or more multiple wettable, absorbent reaction test strips, shown as 74, 76, 78 and 80, carried on the lower surface of the support, as shown. Elements 74 and 86 form a membrane laminate as described herein, where 74 is the HDL assay membrane and 86 is the reagent membrane.
  • Support 72 is transparent or has windows or openings which allow the pads to be viewed through the support.
  • Each test pad used in a particular assay contains analy- te-dependent reagents effective to produce an analyte-dependent change in the pad which can be detected in a known manner.
  • the reaction bar is mounted on support 52 by mounting means effective to (a) maintain the device in a sample-distribution position, wherein the test membrane/reagent membrane laminate is spaced apart from the sample distribution matrix, and to (b) transfer the device to a test position, where the test membrane/reagent membrane laminate and the sample distribution matrix are in fluid communication.
  • the mounting means can also be used to break such fluid communication after a desired amount of sample has entered the test pads, and/or after a determined contact time, by transferring the device from the test position to a position in which the test strip(s) are not in fluid communication with the sample distribution matrix (which may be the same as the "sample-distribution" position).
  • Such transferring can be controlled by monitoring the reflectance at the top surface of the test pad, which re- fleets extent of wetting, as described in co-owned U.S. Patent No. 5,114,350.
  • the quantity of sample can be controlled with sufficient accuracy by u- sing a predetermined contact time.
  • the mounting means can include, for example, a pair of resilient members, such as elastomeric blocks 82, 84, which act to bias the test membrane/reagent membrane laminate toward a non-transfer or sample-distribution position, at which the laminate is spaced apart from the sample distribution matrix.
  • resilient members such as elastomeric blocks 82, 84
  • fluid communication between sample distribution matrix 62 and the laminate can be selectively established and separated.
  • the fluid communication may be via direct contact or through an intermediate element.
  • the support blocks could be compressed by means of springs or a piston-like action.
  • external mechanical devices could engage the main body 52 and/or support 62 and move one towards the other.
  • An exemplary system is the Cholestech LDX® A- nalyzer, a self-contained, automated analyzer advantageous for use with assay devices such as described herein.
  • Exemplary HDL assay laminates were prepared by gravure coating, as disclosed herein, and HDL assays on known standards were run using the laminates. The data showed excellent precision, demonstrating the effectiveness of the disclosed process for applying controlled and uniform quantities of the assay reagents.
  • the membrane laminate employed was a laminate of two BTS-83 polysulfone asymmetric membranes, laminated with the small pored (shiny) side of one membrane contacting the large pored (dull) side of the second membrane, prepared by Pall Corporation, San Diego CA. Widths of up to about 5 inches were used for coating.
  • Standard precipitation and HDL assay reagent mixtures were used.
  • the precipitation solution included 3.9 mg/ml dextran sulfate (500,000 MW) and 7.9 mM Mg(OAc) 2 in water.
  • a surfactant (Pluronic L64, produced by BASF, at a level of 0.05%) was also added to facilitate uptake onto the membrane. .
  • the HDL assay reagent solution contained 80.3 U/ml cholesterol oxidase, 473 U/ml cholesterol esterase, 440 U/ml horseradish peroxidase, 4.14 mg/ml 4-aminoantipyrine, and 26.5 mg ml TOOS (3-[ethyl(3-methylphenyl)amino]-2-hydroxy propanesulfonic acid) in water, with 3 mg/ml CHAPS added as surfactant.
  • TOOS 3-[ethyl(3-methylphenyl)amino]-2-hydroxy propanesulfonic acid
  • a flexo graphic press with gravure cylinder was used to apply a constant volume of reagent solution to a rubber roller which was in contact with the membrane laminate (offset gravure process).
  • the cylinder used for this experiment was a 65 line/inch, 30 BCM roll, where BCM refers to billion cubic microns, or microliters, per square inch of surface.
  • the precipitation reagents were first applied to the dull side of the first membrane. Following application, the membrane was dried with an IR dryer blower. The HDL colorimetric assay reagents were then applied to the shiny side of the second membrane of the laminate, in a similar manner, and dried with an TR dryer blower.
  • HDL assay data was from laminated membranes prepared as described above, cut into 0.22 inch sections and assembled into assay cassettes, such as described in US Appn. Pubn. No. 20030166291 and US Appn. Serial No. 10/410,671, cited above. Assays were carried out according to standard procedures. The samples (eight HDL standards) were analyzed in an LDX ® analyzer, and the mean of eight cassettes was taken for each standard. Excellent precision and correlation with the standard values were obtained.
  • the gravure cylinder spins in a direction opposite to the web feed direction (i.e., reverse gravure, as shown in Fig. 2), and the web contacts the cylinder without an impression cylinder ("kiss" gravure, as shown at 42 in Fig. 2).
  • a cylinder is chosen with a pattern of wells that is effective to apply a uniform coating with the given coating system.
  • Membranes were coated using the reverse/kiss gravure process, with web speeds of 5-10 ft/min and cylinder rotation speeds of about twice the web speed for the precipitation reagent coating and about the same as the web speed for the HDL assay reagent coating.
  • the quantity of solution applied to the membrane in these runs was generally about 65% of the saturating volume for the precipitation reagents, and about 45% of the saturating volume for the HDL assay reagents.

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EP04786030A 2003-11-10 2004-07-29 Membranen und laminate enthaltende reagenzien sowie verfahren zu ihrer herstellung Withdrawn EP1680212A2 (de)

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DE2003152384 DE10352384A1 (de) 2003-11-10 2003-11-10 Reagenzien enthaltende Membrane und Laminate und Verfahren zu ihrer Herstellung
PCT/IB2004/003704 WO2005044429A2 (en) 2003-11-10 2004-07-29 Reagent-containing membranes and laminates and methods of their prepration

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USRE37701E1 (en) * 1994-11-14 2002-05-14 W. L. Gore & Associates, Inc. Integral composite membrane
US6451396B1 (en) * 1998-02-13 2002-09-17 Gore Enterprise Holdings, Inc. Flexure endurant composite elastomer compositions
EP1322407A4 (de) * 2000-09-05 2004-07-28 Miox Corp Umkehrosmosemembrane und verfahren zu deren herstellung
DE10204606C1 (de) * 2002-01-18 2003-10-16 Cholestech Corp Vorrichtung und Verfahren für Lipoproteine hoher Dichte
ATE309544T1 (de) * 2002-04-09 2005-11-15 Cholestech Corp Verfahren und vorrichtung zur quantifizierung von lipoprotein-cholesterol hoher dichte

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