Method for adding an apparent non-signal line to a rapid diagnostic assay

Abstract

A test device and method for determining the presence or absence of one or more analytes in a fluid sample, the test device including a support or member bearing a mark thereon, and a matrix or member containing a capture zone. In operation, an observation area in the test device becomes transparent, thereby allowing the user to view a mark that is present on a support that is disposed beneath the observation area. Typically, the mark on the underlying support is configured as a minus (−) sign. In the absence of analyte in the sample, the test device presents a negative result as a minus (−) signal. In the presence of analyte in the sample, however, the mark operates in concert with a perpendicular test line on the observation area to present a positive result as a plus (+) signal that is visible to the user.

Description

BACKGROUND OF THE INVENTION

[0002] The present invention relates generally to devices and methods for detection of analytes in test samples. More specifically, the present invention provides solid phase test devices and methods that combine an internal indicator on the test with an external mark located on a support.

[0003] Various analytical procedures and devices are commonly employed in detection assays to determine the presence and/or amount of substance of interest or clinical significance which may be present in biological or non-biological fluids. Such substances are generally termed “analytes” and can include antibodies, antigens, drugs, or hormones.

[0004] The present invention includes, but is not limited to, lateral flow chromatography assay formats. Generally, these assays have an extended base layer on which a differentiation can be made between a sample application region and an evaluation region. In typical use, the sample is applied to the sample application region, flows along a liquid transport path which runs parallel to the base layer, and then flows into the evaluation region. A capture reagent is present in the evaluation region, and the captured analyte can be detected by a variety of protocols to detect visible moieties associated with the captured analyte. For example, the assay may produce a visual signal, such as color change, fluorescence, luminescence, and the like, when indicating the presence or absence of an analyte in a biological sample.

[0005] Vertical flow devices and assays are also contemplated herein. Generally, these assays, similar to those described in U.S. Pat. No. 4,632,901, involve the introduction of a liquid sample to a device and allowing the fluid sample to pass through one or more layers to generate a result. Results, similar to the assays described above and below, may be in the form a visual signal.

[0006] Optimally, such test devices will provide a characteristic signal when the analyte is present in a sample, and a different signal when the analyte is absent from a sample. Most typically, the test device will display a “plus” (+) signal in the presence of analyte, and a “minus” (−) signal in the absence of analyte. The plus/minus test result format has enjoyed enthusiastic customer response and wide commercial success.

[0007] Test devices of this kind are well known in the art, and play an important role in areas such as clinical chemistry. They are used by skilled clinicians and lay person alike. Thus, there is a strong impetus to provide devices that are simple and reliable. Desirably, the assays are single-step devices wherein the user need only apply the sample prior to viewing the result. Single-step devices obviate the necessity of performing complicated and time consuming processing steps that may introduce errors in the end result.

[0008] Examples of such assays include pregnancy tests, ovulation tests, various urine, saliva, spinal, and blood tests, as well as other clinical or diagnostic assays.

[0009] Test devices typically use materials that specifically bind with an analyte of interest. A homologous pair of specific binding pair members (“sbp members”), usually an immunological pair comprising a ligand and a receptor (antiligand), is involved, wherein one of the sbp members is labeled with a label that provides a detectable signal. The immunoassay methodology results in a distribution of the signal label between signal label bound in a complex of the sbp members and unbound signal label. The differentiation between bound and unbound signal label can be a result of physical separation of bound from unbound signal label or modulation of the detectable signal between bound and unbound signal label.

[0010] In developing an assay device, there are many considerations. One consideration is to provide substantial differentiation between the observed signal resulting from signal label when bound as compared to unbound. Another consideration is the ease with which the observed signal can be detected and serve to differentiate between the presence or absence of analyte of interest. Other factors include the precision with which the test devices must be manufactured. In factoring this consideration it is important to include registration or indexing capabilities in vertical flow test devices of the present invention. These capabilities, as described in detail below, are important for testing accuracy, reproducibility and ease of use and reading results. Therefore, in developing an assay that can be used by untrained personnel, such as assays to be performed in the home, medical offices and the like, the technique for performing the assay should be simple, and the method of manufacturing the assay should be straightforward.

[0011] Plus/Minus Assays

[0012] Of particular interest to the present invention are test devices of the type described in U.S. Pat. No. 5,145,789 to Corti et al., the disclosure of which is incorporated herein by reference. Corti et al. discuss a built-in positive control to indicate successful operation of a pregnancy test device. The positive control is envisaged as a horizontal tract that always stains, independent of the presence of hCG in the urine, and is described as an area on a membrane that contains immobilized hCG. Regardless of whether hCG is present in the biological sample, it is intended that during operation, the upstream mobile labeled hCG binding reagents will always bind to the immobilized hCG, thereby forming a horizontal line, or minus sign, in the reading area.

[0013] A similar approach for providing a minus sign in a test device is described in U.S. Pat. Nos. 4,916,056, 5,008,080 and 5,160,701 to Brown, III et al., the disclosures of which are incorporated herein by reference. As illustrated, the positive control is formed by providing a binding substance within the test strip matrix, and is formed in the shape of a rectangular bar, or minus sign. The binding substance of the minus sign is intended to bind the labeled material regardless of the presence or absence of the analyte of interest in the test sample.

[0014] Another approach for providing a positive control in a test device is described in EP Patent Publication No. 0 249 418 to Graham, Jr., the disclosure of which is incorporated herein by reference. As described, the control zone has anti-human IgG or IgM immobilized thereon, for nonspecifically capturing human immunoglobulin ubiquitously present in all similar human aqueous samples. The immobilized antibody is intended to provide a signal in a “minus” pattern, regardless of the presence or absence of the analyte of interest in the test sample.

[0015] Osikowicz et al., in U.S. Pat. No. 5,075,078, describe yet another approach for providing a positive control in a plus/minus test device. The positive control is disposed on a test strip in a rectangular bar configuration. The control bar is oriented on the strip so that it lies neither perpendicular nor parallel to the direction of fluid flow, but rather lies at an intermediate orientation, i.e., at a 45 degree angle.

[0016] Still yet another approach for providing a positive control in a test device is provided in U.S. Pat. No. 5,401,667 to Koike. As described, the test device provides a plus/minus format, but considers alternative geometric symbols as well. A portion of the chromatographic medium is removed, or otherwise partially blocked, thereby affecting the flow path of the liquid. It is suggested that this modification enhances the signal of the device.

[0017] Wong et al., in EP Patent No. 0 260 965, describe another test device that utilizes the plus/minus format. Wong et al. discuss a multiple-step diagnostic assay with a horizontal positive control line sprayed onto a test membrane.

[0018] The previous methods discussed above accomplish the “appearance” of a minus sign (−) by placing an indicator (positive control) line perpendicular to the test line, directly onto the test strip. Typically, the control line develops with any sample flow, while the test line develops only with a positive sample flow. Thus, the previous assays involve a control mechanism inherent to the matrix membrane test strip, and require a specific manufacturing step to apply the control line to the strip.

[0019] Other previous devices display a printed minus sign positioned on the matrix and across the test line. These devices typically incorporate a positive control line downstream from, and parallel to, the test line. Such devices are limited as the test strips may present a line that is visible before the sample is added.

[0020] Previous methods are further disadvantaged as the additional manufacturing step involves a difficult placement procedure to orient the perpendicular line directly in the center of the viewing window. Whether the perpendicular line is a printed minus sign, or a reagent-based control line, this approach is particularly ill suited for certain matrix construction procedures, including web processing methods that involve a continuous flow or continuous roll application approach.

[0021] Therefore, it would be desirable to provide a test device that does not require this extra processing step of depositing a perpendicular line onto the test strip, or does not leave a line that is visible before the sample is added to the device. This invention fulfills these and other needs.

[0022] Transparent Membranes

[0023] The use of transparent test strips in diagnostic assays is known in the art. In U.S. Pat. No. 4,824,640, Hildebrand et al. discuss a transparent reagent carrier layer suitable for evaluation by transmission photometry. As described, the transparent nature of the film of plastic provides a suitable carrier material as compared to opaque films.

[0024] The use of a transparent test strip is also discussed in U.S. Pat. No. 5,110,550 to Schlipfenbacher et al. As described, this test device includes a white non-transparent covering layer situated above a color-forming layer. During operation of the test device, the covering layer becomes transparent in the moist state. Through the transparent covering layer, the user is then able to observe any reaction occurring in the color-forming layer below.

[0025] The use of a clearing agent in an immunochromatographic assay is discussed in U.S. Pat. No. 6,165,798 to Brooks. As described, the test strip membrane is rendered transparent by wetting the membrane with a clearing agent, thus reducing the amount of light scattered by the membrane fibers.

[0026] In U.S. Pat. No. 6,187,268, Albarella et al. describe a transparent flow through membrane for use in test devices, but do not suggest a control feature to indicate a positive or negative test result. The membrane described in Albarella et al. is not configured to become transparent only when wet. The membrane is transparent whether wet or dry.

[0027] While conceivably workable in some circumstances, the previous detection systems that employ transparent membranes are of limited utility. There is no teaching or suggestion in current art for a test device with a transparent membrane that utilizes a control feature to indicate a positive or negative test result as provided by a mark on the underlying support.

[0028] In view of the foregoing, there remains a need in the art for a simple, efficient method for adding a positive control to a solid phase assay that does not require the manufacturing step of fixing a positive control binding member to the assay test strip, and that does not leave a substantially visible signal before the sample is added to the device. It would further be desirable to achieve improved test device formats that incorporate transparent membranes as part of a control or display feature.

[0029] Additionally, the assay of the present invention should overcome the disadvantages described above in connection with the previous test device systems.

BRIEF SUMMARY OF THE INVENTION

[0030] The present invention includes devices, methods, and kits for visually detecting the presence or absence of an analyte in a sample. For example, the present invention provides a test device for determining the presence or absence of an analyte in a fluid sample. In a particular embodiment, testing devices are contemplated that are capable of measuring multiple analytes in a given sample. The test device may be a vertical flow test device, or a lateral flow test device, or any other solid phase test device that comprises a matrix disposed above a support, e.g., a dipstick-type testing device.

[0031] In one embodiment, the matrix defines an axial flow path, and typically contains three zones. First, a sample receiving zone is located at an upstream end of the flow path. The test sample suspected of containing an analyte of interest is applied to the sample receiving zone. Second, a label zone is located on the flow path downstream from the sample receiving zone. As the test sample flows through the label zone, it contacts a detectable mobile labeled reagent. This labeled reagent is specific for, and binds to, the analyte of interest. Third, an observation area is located at the downstream end of the flow path. A capture zone is situated in the area, and contains immobilized capture reagents that are specific for, and bind with, the analyte of interest. Generally, the binding is achieved by either a direct or an indirect binding approach. Optionally, an absorbent zone is disposed downstream of the observation area.

[0032] The sample fluid travels from the sample receiving zone, through the label zone, and then across the observation area and capture zone. The observation area, now moistened from the sample fluid, becomes transparent. The user can then view a mark displayed on the underlying support.

[0033] In another embodiment, a test device is provided useful for determining the presence or absence of an analyte in a fluid sample, the test device composed of a matrix comprising a porous first member comprising a defined capture zone and an observation area, and a second member disposed below and contacting said first member. In one aspect, the capture zone contains an immobilized capture reagent that restrains the analyte, and the first member is comprised of a material that is opaque in a dry state and transparent in a moist state. In another aspect, the second member bears one or more marks thereon, and is comprised of a porous material. The second member generally allows fluid flow through the first member when a fluid sample is introduced. And, the mark on the second member becomes visible through the observation area on the first member when the first member is in a moist state. The mark may have a shape such that, in the presence or absence of the analyte in the sample, a first symbol may be displayed to represent a negative result, and the capture zone may have a shape such that, taken together with the first symbol in the presence of the analyte in the sample, a second symbol is formed to represent a positive result.

[0034] In another embodiment, methods of manufacturing and using the testing devices are provided. In manufacturing vertical flow assays, it is important to include registration or indexing capabilities in vertical flow test devices. These capabilities, as described in detail below, are important for testing accuracy, reproducibility and ease of use and reading results.

[0035] The present invention is simple, effective, and solves the problems of previous devices and methods, by providing a test device with a transparent membrane and an underlying support that bears a mark.

[0036] This invention utilizes a property of nitrocellulose, or a similar membrane, in that it becomes transparent when it is wet. By placing a detectable line or symbol directly underneath the nitrocellulose capture zone, that marking will be mostly invisible until a liquid sample is added. When the membrane becomes wet, the markings underneath it become instantaneously visible and appear to be a part of the displayed results.

[0037] The invention described herein allows the mark to be placed in a precisely controlled location within the window and can be printed directly on the plastic housing or on an intermediate member disposed between the housing and the test strip. This allows for the actual test strip to be processed continuously in that there is no need to manufacture a control line or minus symbol that is perpendicular to the processing flow. This feature is particularly desirable in web processing procedures. With appropriate indexing of the printing equipment, the mark can also be printed on the transparent backing material that may be used to support the membrane on which the assay takes place.

[0038] The invention does not require any chemical interaction between a label component and a capture component to produce the appearance of a line or symbol in any shape or color. The invention imparts a very distinct look and operability characteristic to a lateral flow device.

[0039] The present invention achieves the “appearance” of a minus sign (−) by placing an indicator mark perpendicular to the test line, directly on the underlying support. The mark typically manifests with any sample flow, while the test line develops only with a positive sample flow. A further advantage of the present invention is the avoidance of a line that is substantially visible before the sample is added to the device.

[0040] Other objects and advantages will become apparent from the following detailed description taken in conjunction with the drawings in which:

BRIEF DESCRIPTION OF THE DRAWINGS

[0041] FIG. 1 is an exploded perspective view of a test device of the present invention.

[0042] FIG. 2 is an exploded perspective view of a test device of the present invention showing a negative test result.

[0043] FIG. 3 is an exploded perspective view of a test device of the present invention showing a positive test result.

[0044] FIG. 4 is an exploded perspective view of a test device of the present invention showing a positive test result, and a procedural control line.

[0045] FIG. 5 shows a top view of a vertical flow device, looking down into the chamber into which the sample and other components are poured.

[0046] FIG. 6 shows a top view of a porous positive control membrane support in a vertical flow device.

[0047] FIG. 7 shows a top view of a filter/membrane including a capture/test zone in a vertical flow device.

[0048] FIG. 8 shows an illustration of a negative test result in a vertical flow device of the present invention. The positive control line is visible but the dotted invisible test line is not formed.

[0049] FIG. 9 shows an illustration of a positive test result in a vertical flow device of the present invention. Both the positive control line and the test line are visible.

[0050] FIG. 10 shows a side view of a vertical flow device of the present invention.

DETAILED DESCRIPTION OF THE INVENTION

[0051] Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. If a definition set forth in this section is contrary to or otherwise inconsistent with a definition set forth in the patents, applications, published applications and other publications that are herein incorporated by reference, the definition set forth in this section prevails over the definition that is incorporated herein by reference. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, the preferred methods and materials are now described. All publications mentioned herein are incorporated herein by reference to disclose and describe the methods and/or materials in connection with which the publications are cited.

[0052] In describing the various aspects of the present invention, a number of terms will be generally defined or abbreviated as follows.

[0053] Definitions

[0054] As used herein, “a” or “an” means “at least one” or “one or more.”

[0055] “Fluid sample” refers to a material suspected of containing the analyte of interest. The fluid sample can be used as obtained directly from the source or following a pretreatment so as to modify its character. Such samples can include human, animal or man-made samples. The sample can be prepared in any convenient medium which does not interfere with the assay. Typically, the sample is an aqueous solution or biological fluid as described in more detail below.

[0056] The fluid sample can be derived from any source, such as a physiological fluid, including blood, serum, plasma, saliva, sputum, ocular lens fluid, sweat, urine, milk, ascites fluid, mucous, synovial fluid, peritoneal fluid, transdermal exudates, pharyngeal exudates, bronchoalveolar lavage, tracheal aspirations, cerebrospinal fluid, semen, cervical mucus, vaginal or urethral secretions, amniotic fluid, and the like. Herein, fluid homogenates of cellular tissues such as, for example, hair, skin and nail scrapings, meat extracts and skins of fruits and nuts are also considered biological fluids. Pretreatment may involve preparing plasma from blood, diluting viscous fluids, and the like. Methods of treatment can involve filtration, distillation, separation, concentration, inactivation of interfering components, and the addition of reagents. Besides physiological fluids, other samples can be used such as water, food products, soil extracts, and the like for the performance of industrial, environmental, or food production assays as well as diagnostic assays. In addition, a solid material suspected of containing the analyte can be used as the test sample once it is modified to form a liquid medium or to release the analyte. The selection and pretreatment of biological, industrial, and environmental samples prior to testing is well known in the art and need not be described further.

[0057] “Specific pair binding member” refers to a member of a specific binding pair, i.e., two different molecules wherein one of the molecules specifically binds with the second molecule through chemical or physical means. The two molecules are related in the sense that their binding with each other is such that they are capable of distinguishing their binding partner from other assay constituents having similar characteristics. The members of the specific binding pair are referred to as ligand and receptor (antiligand), sbp member and sbp partner, and the like. A molecule may also be a sbp member for an aggregation of molecules; for example an antibody raised against an immune complex of a second antibody and its corresponding antigen may be considered to be an sbp member for the immune complex.

[0058] In addition to antigen and antibody specific binding pair members, other specific binding pairs include, as examples without limitation, biotin and avidin, carbohydrates and lectins, complementary nucleotide sequences, complementary peptide sequences, effector and receptor molecules, enzyme cofactors and enzymes, enzyme inhibitors and enzymes, a peptide sequence and an antibody specific for the sequence or the entire protein, polymeric acids and bases, dyes and protein binders, peptides and specific protein binders (e.g., ribonuclease, S-peptide and ribonuclease S-protein), and the like. Furthermore, specific binding pairs can include members that are analogs of the original specific binding member, for example an analyte-analog or a specific binding member made by recombinant techniques or molecular engineering.

[0059] An sbp member is analogous to another sbp member if they are both capable of binding to another identical complementary sbp member. Such an sbp member may, for example, be either a ligand or a receptor that has been modified by the replacement of at least one hydrogen atom by a group to provide, for example, a labeled ligand or labeled receptor. The sbp members can be analogous to or complementary to the analyte or to an sbp member that is complementary to the analyte.

[0060] If the specific binding member is an immunoreactant it can be, for example, an antibody, antigen, hapten, or complex thereof. If an antibody is used, it can be a monoclonal or polyclonal antibody, a recombinant protein or antibody, a chimeric antibody, a mixture(s) or fragment(s) thereof, as well as a mixture of an antibody and other specific binding members. The details of the preparation of such antibodies and their suitability for use as specific binding members are well-known to those skilled in the art.

[0061] When an immunoreactive specific binding member is attached to the chromatographic material of the present invention, the device is referred to as an “immunochromatograph”, and the corresponding method of analysis is referred to as “immunochromatography”. Immunochromatography, as used herein, encompasses both sandwich and competitive immunoassay techniques.

[0062] “Ligand” refers to any compound for which a receptor naturally exists or can be prepared.

[0063] “Receptor” refers to any compound or composition capable of recognizing a particular spatial or polar orientation of a molecule, e.g., epitopic or determinant site. Illustrative receptors include: antibodies, enzymes, thyroxine binding globulin, intrinsic factor, lectins, nucleic acids, protein A, complement, complement Clq, and the like. Receptors are also referred to as antiligands.

[0064] “Antigen” shall mean any compound capable of binding to an antibody, or against which antibodies can be raised.

[0065] “Antibody” refers to a polypeptide substantially encoded by an immunoglobulin gene or immunoglobulin genes, or fragments thereof. The recognized immunoglobulin genes include the kappa, lambda, alpha, gamma, delta, epsilon, and mu constant regions, as well as myriad immunoglobulin variable region genes. Light chains are classified as either kappa or lambda. Heavy chains are classified as gamma, mu, alpha, delta, or epsilon, which in turn define the immunoglobulin classes, IgG, IgM, IgA, IgD, and IgE, respectively. Typically, an antibody is an immunoglobulin having an area on its surface or in a cavity that specifically binds to and is thereby defined as complementary with a particular spatial and polar organization of another molecule. The antibody can be polyclonal or monoclonal. Antibodies may include a complete immunoglobulin or fragments thereof. Fragments thereof may include Fab, Fv and F(ab′)2, Fab′, and the like. Antibodies may also include chimeric antibodies made by recombinant methods.

[0066] “Analyte” or “analyte of interest” refers to the compound or composition to be detected or measured and which has at least one epitope or binding site. The analyte can be any substance for which there exists a naturally occurring analyte specific binding member or for which an analyte-specific binding member can be prepared. e.g., carbohydrate and lectin, hormone and receptor, complementary nucleic acids, and the like. Further, possible analytes include virtually any compound, composition, aggregation, or other substance which may be immunologically detected. That is, the analyte, or portion thereof, will be antigenic or haptenic having at least one determinant site, or will be a member of a naturally-occurring binding pair.

[0067] Analytes include, but are not limited to, toxins, organic compounds, proteins, peptides, microorganisms, bacteria, viruses, amino acids, nucleic acids, carbohydrates, hormones, steroids, vitamins, drugs (including those administered for therapeutic purposes as well as those administered for illicit purposes), pollutants, pesticides, and metabolites of or antibodies to any of the above substances. The term analyte also includes any antigenic substances, haptens, antibodies, macromolecules, and combinations thereof. A non-exhaustive list of exemplary analytes is set forth in U.S. Pat. No. 4,366,241, at column 19, line 7 through column 26, line 42, the disclosure of which is incorporated herein by reference. Further descriptions and listings of representative analytes are found in U.S. Pat. Nos. 4,299,916; 4,275,149; and 4,806,311, all incorporated herein by reference.

[0068] “Label reagent” refers to a substance comprising a detectable label attached with a specific binding member. The attachment may be covalent or non-covalent binding, but the method of attachment is not critical to the present invention. The label allows the label reagent to produce a detectable signal that is related to the presence of analyte in the fluid sample. The specific binding member component of the label reagent is selected to directly bind to the analyte or to indirectly bind the analyte by means of an ancillary specific binding member, which is described in greater detail hereinafter. The label reagent can be incorporated into the test device at a site upstream from the capture zone, it can be combined with the fluid sample to form a fluid solution, it can be added to the test device separately from the test sample, or it can be predeposited or reversibly immobilized at the capture zone. In addition, the specific binding member may be labeled before or during the performance of the assay by means of a suitable attachment method.

[0069] “Label” refers to any substance which is capable of producing a signal that is detectable by visual or instrumental means. Various labels suitable for use in the present invention include labels which produce signals through either chemical or physical means. Such labels can include enzymes and substrates, chromogens, catalysts, fluorescent compounds, chemiluminescent compounds, and radioactive labels. Other suitable labels include colloidal metallic particles such as gold, colloidal non-metallic particles such as selenium or tellurium, dyed or colored particles such as a dyed plastic or a stained microorganism, organic polymer latex particles and liposomes, colored beads, polymer microcapsules, sacs, erythrocytes, erythrocyte ghosts, or other vesicles containing directly visible substances, and the like. Typically, a visually detectable label is used as the label component of the label reagent, thereby providing for the direct visual or instrumental readout of the presence or amount of the analyte in the test sample without the need for additional signal producing components at the detection sites.

[0070] The selection of a particular label is not critical to the present invention, but the label will be capable of generating a detectable signal either by itself, or be instrumentally detectable, or be detectable in conjunction with one or more additional signal producing components, such as an enzyme/substrate signal producing system. A variety of different label reagents can be formed by varying either the label or the specific binding member component of the label reagent; it will be appreciated by one skilled in the art that the choice involves consideration of the analyte to be detected and the desired means of detection. As discussed below, a label may also be incorporated used in a control system for the assay.

[0071] For example, one or more signal producing components can be reacted with the label to generate a detectable signal. If the label is an enzyme, then amplification of the detectable signal is obtained by reacting the enzyme with one or more substrates or additional enzymes and substrates to produce a detectable reaction product.

[0072] In an alternative signal producing system, the label can be a fluorescent compound where no enzymatic manipulation of the label is required to produce the detectable signal. Fluorescent molecules such as fluorescein, phycobiliprotein, rhodamine and their derivatives and analogs are suitable for use as labels in such a system.

[0073] The use of dyes for staining biological materials, such as proteins, carbohydrates, nucleic acids, and whole organisms is documented in the literature. It is known that certain dyes stain particular materials preferentially based on compatible chemistries of dye and ligand. For example, Coomassie Blue and Methylene Blue for proteins, periodic acid-Schiffs reagent for carbohydrates, Crystal Violet, Safranin O, and Trypan Blue for whole cell stains, ethidium bromide and Acridine Orange for nucleic acid staining, and fluorescent stains such as rhodamine and Calcofluor White for detection by fluorescent microscopy. Further examples of labels can be found in, at least, U.S. Pat. Nos. 4,695,554; 4,863,875; 4,373,932; and 4,366,241, all incorporated herein by reference.

[0074] “Signal producing component” refers to any substance capable of reacting with another assay reagent or with the analyte to produce a reaction product or signal that indicates the presence of the analyte and that is detectable by visual or instrumental means. “Signal production system”, as used herein, refers to the group of assay reagents that are needed to produce the desired reaction product or signal.

[0075] “Ancillary specific binding member” refers to any member of a specific binding pair which is used in the assay in addition to the specific binding members of the conjugate or capture reagent. One or more ancillary specific binding members can be used in an assay. For example, an ancillary specific binding member can be capable of binding the conjugate with the analyte of interest, in instances where the analyte itself could not directly attach to the conjugate. Optionally, the ancillary binding member may be capable of binding the analyte with the capture reagent, in instances where the analyte itself could not directly attach to the capture reagent. The ancillary specific binding member can be incorporated into the assay device or it can be added to the device as a separate reagent solution.

[0076] “Solid phase” refers to any solid material to which analyte, analyte complexes, or assay reagents become bound and which can be separated from unreacted assay reagents, test sample, or test solutions. For example, the solid phase may involve beads, magnetic particles, latex particles, test tubes, microtiter plates, or any other solid material. Generally, the solid phase is any suitable chromatographic, bibulous, porous, isotropic, or capillary material, hereinafter referred to as porous material, which forms the basis of the test device.

[0077] “Capture reagent” refers to a specific binding member that is attached within or upon a portion of the solid phase to form a “capture zone”. The method of attachment is not critical to the present invention. The capture reagent is selected to bind the analyte, the conjugate, or a complex thereof.

[0078] “Ancillary material” shall mean any material that may be employed in an assay in accordance with the present invention. For example, buffer will normally be present in the labeling means, the neutralization means, as well as stabilizers for the assay medium and assay components. Frequently, in addition to these additives, additional protein, such as albumin, or surfactant, non-ionic or ionic, binding enhancer, for example, polyalkylene glycol, or the like, may be present, including free antibody, analyte analog, or other unrelated ligand, for the purpose of removing or adding material or to modify the amount, position, partitioning, or appearance of the analyte or other compound used in the invention.

[0079] “Observable signal” as used herein refers to a signal produced in the claimed devices and methods that is detectable by visual inspection. Without limitation, the type of signal produced depends on the label reagents and marks used (described herein). Generally, observable signals indicating the presence or absence of an analyte in a sample may be evident of their own accord, e.g., plus or minus signs or particularly shaped symbols, or may be evident through the comparison with a panel such as a color indicator panel.

[0080] “Axial flow” as used herein refers to lateral, vertical or transverse flow through a particular matrix. The type of flow contemplated in a particular device, assay or method varies according to the structure of the device. Without being bound by theory, lateral, vertical or transverse flow may refer to flow of a fluid sample from the point of fluid contact on one end or side of a particular matrix to an area downstream of this contact. The downstream area may be on the same side or on the opposite side of the matrix from the point of fluid contact. For example, in vertical flow devices of the present invention, axial flow may progress vertically from and through a first member (top to bottom) to a second member and from there on to an absorbent medium.

[0081] “Porous material” refers to any material that may be employed in the lateral assays described herein that are opaque in a dry state and transparent or semi-transparent in a moist state (e.g., nitrocellulose).

[0082] “Absorbent material” as used herein refers to material used in vertical flow devices and assays that allows and promotes sample flow through the first and second members. Such materials may be as described in, e.g., U.S. Pat. No. 4,632,901, such as, for example, fibrous materials such as cellulose acetate fibers, cellulose or cellulose derivatives, polyester, or polyolefin. Generally, the absorbent material, as used herein, should maintain direct or intimate contact with the second member in order to promote fluid flow therethrough. Contemplated absorbent materials having fluid absorptive qualities are generally compressible and may be compressed in devices of the present invention to ensure contact with the second member or positive control element.

[0083] “Registration means” or “indexing means” refers to physical means useful for placement of the first and second members in the vertical flow devices of the present invention. These means may involve the use of rails contained in the outer wall of a device coupled with notches or slots located in the first and second members. Without limitation, these means are useful for providing an orientation of control markings in relation to capture zones such that in the presence or absence of an analyte of interest and detectable reagent coupled thereto, all markings and zones may be separately distinguishable. Occasionally, these means may also equally apply to placement of the absorbent medium in the vertical assay devices of the present invention.

[0084] “Orientation indicia” refers to a separate marking located on a vertical flow device of the present invention that permits the user of the device to quickly and accurately determine the correct reading orientation of the device to determine a positive and/or negative result after use of such device in accordance with the presently described methods.

[0085] Introduction

[0086] The present invention relates generally to devices and methods for detection of analytes in test samples. More specifically, the present invention provides solid phase test strip devices and methods that combine an internal indicator on the test strip with an external mark located on a support.

[0087] Test Devices

[0088] In a particular aspect, the present invention provides a test device for determining the presence or absence of an analyte in a fluid sample. The test device includes a support bearing a mark thereon, and a matrix defining an axial flow path. Typically, the matrix further includes a sample receiving zone, a label zone, and an observation area that contains a capture zone. In a related embodiment, the matrix further includes an absorbent zone disposed downstream of the observation area.

[0089] In a preferred embodiment, the sample receiving zone accepts a fluid sample that may contain an analyte of interest. In another embodiment, the sample receiving zone is dipped into a fluid sample. A label zone is located downstream of the sample receiving zone, and contains a mobile label reagent that recognizes the analyte of interest. Further, an observation area is disposed downstream of from the label zone, and contains an immobilized capture reagent that binds to the analyte of interest. Thus, as the fluid sample flows along the matrix, the analyte of interest will first bind with the mobile label reagent in the label zone, and then bind to the immobile capture reagent in the capture zone of the observation area. The observation area is made of a material that is opaque in a dry state and transparent in a moist state. Thus, the mark on the support is visible through the observation area when the observation area is in the moist state.

[0090] In another preferred embodiment, the fluid sample flows along a flow path running from the sample receiving zone (upstream), through the label zone (midstream), and then to the observation area (downstream). Optionally, the fluid may thereafter flow to the absorbent zone.

[0091] In a preferred embodiment, the sample receiving zone is made of an absorbent application pad. Suitable materials for manufacturing absorbent application pads include, but are not limited to, hydrophilic polyethylene materials or pads, glass fiber filter paper or pads, desiccated paper, paper pulp, fabric, and the like. In a related embodiment, the sample receiving zone is constructed from any material that absorbs water.

[0092] In a preferred embodiment, the absorbent application pad is made of any material from which the fluid sample can pass to the label zone. Further, the absorbent application pad may be constructed to act as a filter for cellular components, hormones, particulate, and other certain substances that may occur in the fluid sample. Application pad materials suitable for use by the present invention also include those application pad materials disclosed in U.S. Pat. No. 5,075,078, incorporated herein by reference.

[0093] In yet another preferred embodiment, the absorbent application pad may incorporate other reagents such as ancillary specific binding members, fluid sample pretreatment reagents, and signal producing reagents.

[0094] In a particularly preferred embodiment, the analyte of interest is from the group including heartworm antigens, hCG (human chorionic gonadotropin), streptococcus A, and other bacterial antigens.

[0095] In another preferred embodiment, the test device is configured to perform an immunological analysis process. In yet another embodiment, the liquid transport along the matrix is based upon capillary action, whereby the liquid transport path can be formed not only by one or more layers of absorbent material, for example paper or fleece, but also by a gap which is sucked full by capillary action.

[0096] In a preferred embodiment, the label zone is capable of non-bibulous lateral flow. By “non-bibulous lateral flow” is meant liquid flow in which all of the dissolved or dispersed components of the liquid are carried at substantially equal rates and with relatively unimpaired flow laterally through the membrane, as opposed to preferential retention of one or more components as would occur, e.g., in materials capable of adsorbing or imbibing one or more components.

[0097] In a further preferred embodiment, the label zone is made of a typical non-bibulous material such as high density polyethylene sheet material manufactured by Porex Technologies Corp. of Fairburn, Ga., USA. The sheet material has an open pore structure with a typical density, at 40% void volume, of 0.57 gm/cc and an average pore diameter of 1 to 250 micrometers, the average generally being from 3 to 100 micrometers. The optimum pore diameter for the membrane for use in the invention is about 10 to about 50μm. The membranes typically are from about 1 mil to about 15 mils in thickness, typically in the range of from 5 or 10 mils, but may be up to 200 mils and thicker. The membrane may be backed by a generally water impervious layer, such as mylar. When employed, the backing is generally fastened to the membrane by an adhesive, such as 3M 444 double-sided adhesive tape. Typically, a water impervious backing is used for membranes of low thickness. A wide variety of polymers may be used provided that they do not bind nonspecifically to the assay components and do not interfere with flow of the sample. Illustrative polymers include polyethylene, polypropylene, polystyrene and the like. Alternatively, the membrane may be self supporting. Other non-bibulous membranes, such as polyvinyl chloride, polyvinyl acetate, copolymers of vinyl acetate and vinyl chloride, polyamide, polycarbonate, polystyrene, and the like, can also be used.

[0098] In yet another preferred embodiment, the label zone is made of a material such as untreated paper, cellulose blends, nitrocellulose, polyester, an acrylonitrile copolymer, and the like. The label zone may be constructed to provide either bibulous or non-bibulous flow. In an especially preferred embodiment, the label zone is made of a nonwoven fabric such as Rayon or glass fiber. Other label zone materials suitable for use by the present invention include those chromatographic materials disclosed in U.S. Pat. No. 5,075,078, which is herein incorporated by reference. In a preferred embodiment, the label zone material may be treated with labeled solution that includes blocking and stabilizing agents. Blocking agents include bovine serum albumin (BSA), methylated BSA, casein, nonfat dry milk. Stabilizing agents are readily available and well known in the art, and may be used, for example, to stabilize colored labels.

[0099] In all of the above, employment of the selected blocking and stabilizing agents together with colored moieties in the labeling zone followed by the immobilization of the blocking and stabilizing agents on the support (by, e.g., a freeze-drying process, or a forced air heat drying process) is of utmost importance for improved performance of the device. It is well known that visible moieties, especially particles, aggregate upon air-drying and do not readily rehydrate in contact with a liquid sample. Therefore, absent conversion to the nonbibulous surface, instead of being transported to the capture zone with the sample, the visible moieties will remain trapped in the labeling zone.

[0100] In a particularly preferred embodiment, the observation area will be made of a material that is opaque when in a dry state, and transparent when in a moistened state, examples of which include nitrocellulose, nylon, and hydrophilic polyvinylidene difluoride (PVDF). Hydrophilic polyvinylidene difluoride (PVDF) is commercially available form the firm Millipore, Bedford, U.S.A. under trademark Immobilon AV. However, on the basis of the present description, the expert can also select other materials and especially synthetic material membranes which fulfill the above-mentioned conditions. It is believed that the refractive index of the synthetic material is of major influence to this characteristic. It is to be assumed that porous materials, the refractive index of which is close to that of the sample liquid, have the property of becoming transparent in a moist state.

[0101] In a particularly preferred embodiment, the observation area is a nitrocellulose web assembly made of Millipore nitrocellulose roll laminated to a clear Mylar backing. In another embodiment, the observation area is made of nylon.

[0102] Those skilled in the art will appreciate that various methods could be used to test the desired property of the observation area, and whether it is sufficiently opaque in the dry state, and sufficiently transparent in the moist state. For example, one could put a mark on a piece of plastic, and then place the test strip on top of the plastic and visually determine if it is opaque or transparent. Other methods include the use of scanner devices, or other means for determining optical density of the apparent line.

[0103] The artisan will appreciate the whole of the observation area, or only a portion thereof, may become transparent when moistened. In either embodiment, the portion of the observation area that is disposed above the mark should become transparent when moistened. In a related embodiment, the observation area will contain one or more distinct areas that are opaque in the dry state, and transparent in the moist state.

[0104] In a preferred embodiment, the capture zone may be constructed from any of the materials as listed above for the observation zone. In a particularly preferred embodiment, the capture zone is made of the same material as the observation zone. The artisan will recognize that the present invention envisages a test device with one or more capture zones.

[0105] Further embodiments include capture zones that include microporous materials made from nitrocellulose, by which term is meant any nitric acid ester of cellulose. Thus suitable materials may include nitrocellulose in combination with carboxylic acid esters of cellulose. The pore size of nitrocellulose membranes may vary widely, but is preferably within 5 to 20 microns, preferably 8 to 15 microns. To provide non-bibulous flow, these materials may be treated with blocking agents that can block the forces which account for the bibulous nature of bibulous membranes. Suitable blocking agents include bovine serum albumin, methylated bovine serum albumin, whole animal serum, casein, and non-fat dry milk.

[0106] In a preferred embodiment, the observation area further includes a procedural control line, to verify that the sample flow is as expected. The control line is a spatially distinct region that includes an immobilized binding member which reacts with a labeled reagent. In a preferred embodiment, the procedural control line contains an authentic sample of the analyte of interest, or a fragment thereof. In another preferred embodiment, the control line contains antibody that is specific for, or otherwise provides for the immobilization of, the labeled reagent. In operation, a labeled reagent binds to the control line, even when the analyte of interest is absent from the test sample.

[0107] In a related embodiment, a control conjugate is introduced into the flow sample upstream from the control line. For example, the control conjugate may be added to the fluid sample before the sample is applied to the assay device. Alternatively, the control conjugate may be diffusively bound in the sample receiving zone, or in the label zone.

[0108] In a preferred embodiment, the control conjugate includes a control label and a control reagent. Typically, a control reagent is chosen to be different from the reagent that is recognized by the capture reagent. Further, the control agent is generally not specific for the analyte. In a preferred embodiment, the control reagent binds to a control capture partner that is immobilized on the procedural control line. Thus the control conjugate is directly detected in the control line.

[0109] In yet another embodiment, the detectable control label is the same label used for the label reagent. In a preferred embodiment, the control label is different from the test label, so that the user can more easily determine the results of the assay. In a particularly preferred embodiment, the control label and the test label include colored beads, where the control and test beads are of different colors.

[0110] In a preferred embodiment, the control label includes streptavidin, and the control capture partner includes biotin, which couples to the avidin specifically. In a particularly preferred embodiment, the control label includes biotin, and the control capture partner includes streptavidin. The artisan will appreciate that other “irrelevant” binding pairs can also be used-such as antigen/antibody reactions unrelated to analyte.

[0111] The use of a control line is helpful in that appearance of a signal in the control line indicates the time at which the test result can be read, even for a negative result. Thus, when the expected signal appears in the control line, the presence or absence of a signal in the capture zone can be noted.

[0112] In another preferred embodiment, the matrix may further incorporate an absorbent zone. The absorbent zone can act to increase the amount of fluid sample that travels through the capture zone.

[0113] In this embodiment, the absorbent zone is located downstream from the capture zone and can be a means for removing excess sample and free label other than the analyte of interest from the matrix of the device. Generally, the absorbent zone will consist of an absorbent material such as filter paper, a glass fiber filter, or the like.

[0114] In a preferred embodiment, the device may also contain an end of assay control zone indicator. The control zone indicator may consist of a pH indicating reagent (such as bromocresol green) impregnated in the absorbent zone or at a location downstream of the capture zone. Upon contact with the sample, a pH change occurs in the processed matrix. This pH shift converts the pH indicator to a different color (for instance, bromocresol green may be converted from yellow to blue) which is seen in an observation window over the control zone. This technology may also serve as an internal assay control.

[0115] In a related embodiment, the end of assay control zone may be constructed by applying a line of soluble ink on the capture zone (at the interface with the absorbent zone). The liquid front moving through the capture zone will solubilize the ink and transfer it into the absorbent. The resulting color change will be seen in an observation window above the absorbent zone, signifying end of assay.

[0116] In a preferred embodiment, the capture reagent binds with the analyte for the completion of a sandwich complex. The capture reagent can be chosen to directly bind the analyte or indirectly bind the analyte by binding with an ancillary specific binding member which is bound to the analyte. In addition, the capture reagent may be immobilized on the solid phase before or during the performance of the assay by means of any suitable attachment method. Typically, the capture site of the present invention is a delimited or defined portion of the solid phase such that the specific binding reaction of the capture reagent and analyte is localized or concentrated in a limited site, thereby facilitating the detection of label that is immobilized at the capture site in contrast to other portions of the solid phase. In a related embodiment, the capture reagent can be applied to the solid phase by dipping, inscribing with a pen, dispensing through a capillary tube, or through the use of reagent jet-printing or other techniques. In addition, the capture zone can be marked, for example with a dye, such that the position of the capture zone upon the solid phase can be visually or instrumentally determined even when there is no label immobilized at the site.

[0117] Those of skill in the art will recognize that a variety of direct and indirect assay formats may be employed in the present invention. In a preferred embodiment, a direct assay format is used. Direct assays are exemplified by those that detect the presence of an antigen in a sample, as well as those that detect the presence of an antibody in a sample. A direct assay that detects the presence or absence of an antigen in a sample generally includes a label zone that contains at least one antibody label reagent that is specific for the antigen. In a preferred embodiment, the antibody is coated on colored beads. Likewise, a direct assay that detects the presence or absence of an antigen in a sample generally includes a label zone that contains at least one antigen that is reactive with an antibody-analyte of interest. In this embodiment, the antigen is coated on colored beads.

[0118] As provided above, particular devices of the present invention include a support. The support in these devices provides a convenient platform for performance of the assay. However, the composition and shape of the support are not critical and may vary. Occasionally, the support may be comprised of a plastic or nylon material.

[0119] In another embodiment the present devices may be in the form of a dipstick. Generally, dipsticks of the present invention are functionally analogous to the lateral assays described herein excepting the method of contacting a fluid sample. In embodiments configured as a dipstick, the matrix and support will generally be located on one end of the dipstick. The configuration of such devices will allow the device to be dipped or contacted with a fluid sample with one end of a matrix that is analogous with the sample receiving zone in lateral assays and devices also described herein. After contacting the fluid sample, the sample preferably migrates in an axial flow path through the matrix from the sample receiving zone to the label zones and observation areas. Alternatively, the devices of the present invention may be shaped so that samples may be applied to the device by means other than dipping, e.g., application of controlled amounts of sample by pipettes or the like.

[0120] In a preferred embodiment, the result displayed by the test device incorporates a symbol provided by the mark on the bottom support. Due to the transparent nature of the observation area, the mark on the support is detectable through the moistened observation area. Thus, the shape of the mark will be displayed regardless of whether the analyte of interest is or is not present in the fluid sample. Typically, the shape of the mark provides a first symbol to represent a negative result. In a related embodiment, the symbol provided by the mark on the support is a minus (−) symbol. In a particularly preferred embodiment, the mark will be visible to the unaided eye, although those of skill in the art will appreciate that a variety of detection approaches may be employed. In another preferred embodiment, the mark will be blue or red, or any color which provides contrast with the surrounding area, which is typically a lighter color, such as white.

[0121] In a preferred embodiment, the mark on the support will operate in concert with a symbol provided by the capture zone. When the desired analyte is present in the fluid sample, label is collected at the capture zone. The shape of the labeled capture zone is such that, in combination with the mark, a second symbol is provided representing a positive result. In a related embodiment, the symbol presented by this combination is a plus (+) symbol.

[0122] In yet another preferred embodiment, the capture zone has a shape such that, independent of any symbol provided by that mark on the substrate, labeled reagent at the capture zone will form a second symbol to represent a positive test result.

[0123] In a preferred embodiment, the mark on the support is oriented so that the longitudinal axis of the mark is aligned with the direction of the sample flow, while the longitudinal axis of the capture zone is perpendicular to the direction of the sample flow. In a related embodiment, these axes may be at oblique angles to the sample flow. In yet another related embodiment, these axes may be oriented at any angle to the sample flow, so long as the axis of the mark and the axis of the capture zone are substantially perpendicular to each other.

[0124] In another preferred embodiment, the mark on the support includes a shape such that, in the presence or absence of the analyte of interest in the fluid sample, a logo is displayed in the observation area. In a related embodiment, the marked support provides one or more predefined symbols to be displayed when the observation area is moistened. These symbols may be read in connection with, or independent from, any signal that may be provided by the capture zone.

[0125] In yet another embodiment, the mark may be displayed below the capture zone, but not necessarily on the bottom support. For example, the mark may be contained on the Mylar strip underlying the nitrocellulose matrix membrane. Alternatively, the mark may be contained on an intermediate member disposed between the test strip and the bottom support. In a preferred embodiment, the intermediate member is a plastic strip displaying the mark. The member may or may not be affixed to either the test strip or the bottom support. In a preferred embodiment, the intermediate member is configured to remain in place once the test apparatus is constructed. In a related embodiment, the mark is applied, for example, by an embossing, printing, or stamping technique.

[0126] In still another preferred embodiment, the observation area includes a negative control area. The purpose of this control area is to alert the user that the test device is not working properly. In a preferred embodiment, the negative control is that part of the observation area outside of the capture zone, and does not include any part of the observation area located directly above the mark on the support. When working properly, no signal or mark should be visible in the negative control area.

[0127] In a preferred embodiment, the test device includes a hollow casing or housing having an application aperture and an observation port. In this embodiment, the flow matrix is contained within the hollow casing, and the fluid sample is added to the matrix through the aperture, which is an opening located in an upstream location on the housing.

[0128] Typically, the aperture is located above the sample application pad. In a related embodiment, an aperture may be disposed in any location above the matrix that would provide for facile addition of fluid sample or reagent to the matrix.

[0129] To detect the result, the observation area may be examined through the port. The artisan will appreciate that an observation port may be disposed in any location above the matrix that would provide for the detection of a signal event, whether the signal comes from the observation area, the absorbent zone, or elsewhere. In a preferred embodiment, the port is located above the observation area. Generally, the observation port is open, or the port may be covered by a transparent covering such as glass or plastic.

[0130] From the foregoing, it is appreciated that the outer casing or housing of the device may take various forms. Typically, it will include an elongate casing and may have a plurality of interfitting parts. In a particularly preferred embodiment, the housing includes a top cover and a bottom support. In a preferred embodiment, the bottom support displays a mark thereon, and in a related embodiment, the top cover contains an application aperture and an observation port. In another embodiment, the housing may also contain dividers between the matrix strips to inhibit flow of fluid sample between strips.

[0131] In a preferred embodiment, the housing is made of moisture impervious solid material, for example, a plastic material. It is contemplated that a variety of commercially available plastics, including, but not limited to, vinyl, nylon, polyvinyl chloride, polypropylene, polystyrene, polyethylene, polycarbonates, polysulfanes, polyesters, urethanes, and epoxies maybe used to construct a housing. The housing may be prepared by conventional methodologies, such as standard molding technologies that are well known and used in the art. The housing may be produced by molding technologies which include, but are not limited to, injection molding, compression molding, transfer molding, blow molding, extrusion molding, foam molding, and thermoform molding. The aforementioned molding technologies are well known in the art and so are not discussed in detail herein. See for example, Processes And Materials Of Manufacture, Third Edition, R. A. Lindsberg (1983) Allyn and Baron pp. 393-431.

[0132] It will be appreciated by one skilled in the art that a test strip device can be made of more than one material (e.g., different zones or sites can be made of different materials) and a flow-through device can have more than one layer, wherein different layers can be made of different materials, so long as the multiple materials or layers are in fluid-flow contact with one another thereby enabling the passage of test sample between the materials or layers. Fluid-flow contact permits the passage of at least some components of the test sample between the zones or layers of the device. Fluid-flow is preferably uniform along the contact interface between the different zones or layers. The present invention further provides for different reagents disposed on different materials, and different reagents disposed on different zones. For example, the specific binding member contained on a certain material in the label zone may or may not be the same binding member that is contained on a different material in the capture zone.

[0133] In further preferred embodiments, the test device of the present invention can have many configurations, several of which are dependent upon the material chosen for the solid phase. For example, the test device can include a solid phase material configured for use in a layered flow-through assay device, a chromatographic column, a dipstick or a test strip.

[0134] In a second aspect, the present invention provides a method for determining the presence or absence of one or more analytes in a fluid sample. The assay method includes providing a test device as described above, and administering a fluid sample to the test device. By inspecting the observation area of the test device, the user is able to determine whether the fluid sample contains the one or more analytes of interest. Typically, this is accomplished by observing either a plus (+) or minus (−) signal in the observation area for each analyte of interest.

[0135] In a third aspect, the present invention provides a kit for determining the presence or absence of an analyte in a fluid sample. The assay kit of the present invention will include containers for holding any necessary reagent, test membrane, sample applicator, filter, and the like, as well as instructions which set forth a protocol for practicing the method of use as described above. Typically, the components of the kit will be present in a suitable package containing sufficient components for performing one or more assays.

[0136] The present invention is particularly suitable for a test device as shown in the accompanying drawings, and described in detail as follows. It is understood that the drawings are provided for purposes of illustration and not meant limit the scope of the present invention.

[0137] FIG. 1 shows a first embodiment of a test device 10 constructed in accordance with the teachings of the present invention.

[0138] Test device 10 has a bottom support 14, a flow matrix 18, a top cover 22, and a desiccant 26. In its longitudinal direction, matrix 18 can be subdivided into a sample application zone 30, a label zone 34, an observation area 38, and an absorbent zone 42.

[0139] The bottom support further includes a mark 46 thereon. The mark is disposed beneath observation area 38. The sample application zone is located at an upstream location on matrix 18, and is configured to receive the fluid sample. Label zone 34 is located downstream of application zone 30, and contains label reagent. The observation area is located downstream of the label zone, and includes a capture zone 40 that contains capture reagent. Absorbent pad 42 is located downstream of observation area 38.

[0140] Top cover 22 has an application aperture 48 disposed above the sample application pad, and an observation port 52 disposed above the observation area. In cooperation, the top cover and the bottom support are configured to provide a housing for matrix 18 and desiccant 26. As shown, the desiccant is typically positioned separately from the matrix.

[0141] Prior to use, when in the dry state, the observation area is opaque, and thus no signal is manifested through the observation port.

[0142] FIG. 2 illustrates the test device of the present invention showing a negative test result, in the instance where the fluid sample does not contain the analyte of interest.

[0143] In one operative embodiment, the sample fluid is added through aperture 48, and on to application pad 30. The fluid sample is transported from application pad 30 to label zone 34, where the fluid is allowed to react with labeled reagent. Labeled reagent then binds with any analyte of interest contained in the fluid sample.

[0144] Next, the fluid sample is advanced to observation area 38, and then on to the absorbent zone. Observation area 38, now moistened by the sample fluid, becomes transparent. Consequently, mark 46 becomes visible through observation port 52. Through the observation port, the user can then view the mark displayed on the bottom support.

[0145] As shown here, there is no analyte present, and consequently no label is bound at capture zone 40. The resulting signal as manifested through observation port 52 is therefore in the shape of a minus (−) sign.

[0146] FIG. 3 illustrates the test device of the present invention showing a positive test result, in the instance where the fluid sample contains the analyte of interest.

[0147] In operation, the sample fluid is added through aperture 48, and on to application pad 30. The fluid sample is transported from application pad 30 to label zone 34, where the fluid is allowed to react with labeled reagent. Labeled reagent then binds with the analyte of interest contained in the fluid sample. Next, the fluid sample is advanced to observation area 38, and labeled analyte is restrained by capture reagent immobilized in capture zone 40. Unbound material in the fluid sample continues to flow into absorbent zone 42.

[0148] Observation area 38, now moistened by the sample fluid, becomes transparent. Consequently, mark 46 becomes visible through observation port 52. Through the observation port, the user can then view the mark displayed on the bottom support, in concert with the signal provided by the label contained in the capture zone. The resulting signal as manifested through observation port 52 is in the shape of a plus (+) sign.

[0149] FIG. 4 shows the test device of the present invention, where observation area 38 further includes a procedural control line 56 that develops with any fluid sample flow, whether or not analyte is present in the sample.

[0150] Vertical Flow Devices

[0151] In a further embodiment, the device of the invention may alternatively comprise a vertical flow device. In such devices, as a first member, a porous member may be provided, such as a membrane or filter, to which a capture reagent may be immobilized thereon. The first member preferably further comprises an observation area comprising a defined capture zone and is preferably comprised of a material that is opaque in a dry state and transparent in a moist state. The first member provides for fluid flow therethrough, from the top to the bottom surfaces. Similar to the capture reagents described above, preferred reagents are capable of restraining an analyte of interest on the porous first member. These capture reagents are useful in that they are capable of separating analyte from the fluid sample being analyzed.

[0152] In another aspect, the device may further comprise, as a second member, an absorbent member having fluid pathways therethrough from its upper to lower surfaces. The second member is generally disposed below, and in fluid flow contact with, the first member in the present devices and is selected to allow fluid flow through the first member when a fluid sample is introduced to the upper surface of the first member. In one aspect, the second member comprises a porous positive control membrane support. In a related aspect, the second member may act to support the first member and also contains a positive control zone. The upper surface of the first member is merely the surface lying away from the surface contacting or otherwise in communication with the second member.

[0153] In another aspect, vertical flow type devices of the present disclosure include an optional absorbent medium. Generally, the absorbent medium is useful for absorbing liquid sample, labeled reagent and/or washing solution after flow through the first and second members. The absorption capacity of contemplated absorbent mediums of the present invention are useful for promoting fluid flow through both the first and second members and thus avoiding stagnant fluid remaining on these members. To accomplish this function, the absorbent medium is preferably in close or intimate contact with the second member or positive control element. In one aspect, the absorbent medium may be compressed in a device, below the second member.

[0154] The above device may be utilized through the contact or introduction of a fluid sample suspected of containing one or more analytes and then allowing the sample to migrate through the first and second members, whereby the one or more analytes bind to one or more capture reagents bound to the first member. After the sample has migrated through both members one or more labeled reagents (described above) may be introduced to the upper surface of the first member and allowed to migrate through the first and second members. The labeled reagent is selected to bind to one or more of the analytes suspected of being present in the sample. Thereafter, a washing step may be performed to wash unbound labeled reagent from the first and second members. The presence or absence of a particular analyte may then be detected by visually inspecting the first member to locate marks, logos, symbols, colors, etc., which indicate a positive or negative result corresponding to the presence or absence of particular analytes in a given sample.

[0155] Generally, marks indicating a negative result may be disposed on the second member which may become visible through the first member when the first member is in a moist state (i.e., any time after introduction of the sample to the device). Positive results indicating the presence of one or more analytes in a sample are evident through an indication that the labeled reagent has bound to a particular analyte, i.e., the generation of a positive signal. The first member is generally comprised of a material described above that is opaque in a dry state and transparent in a moist state.

[0156] Suitable washing reagents may be, for example, buffers, solutions containing detergents, defined ionic strength chelators, proteins or other components useful for optimizing separation of bound and free label. Suitable washing reagents may have varying characteristics, however they should not interfere with or otherwise degrade: (1) the analytes or reagents themselves, (2) the interaction of the analyte with the binding or label reagents, or (3) the signal generated indicating the presence or absence of an analyte as a result of utilizing the claimed devices or methods.

[0157] FIG. 5 shows a top view of a vertical flow device. The device sidewall (61), orientation indicia (63), guide rails (62) and center chamber (64) are shown. In one aspect, liquid samples may be poured or otherwise introduced into the center chamber (64) that is surrounded by the device sidewall (61). The device guide rails (62) are useful for providing orientation, registration or indexing capability for additional components, for example, for positioning the porous positive control membrane support (see FIG. 6 (70)) (the “second member”) and filter/membrane (see FIG. 7 (71)) containing a capture/test zone (68) (together, the “first member”) within the device. In one embodiment, the device contains one guide rail. In a related embodiment, the device may contain one or more guide rails, for example between about 1 to about 50 or about 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, about 15, about 20, about 25 about 30, about 35, about 40, about 45, about 50; or a series of means for positioning the porous positive control membrane support and filter/membrane containing a capture/test zone within the device such, as a series of ridges or notches. In another aspect, the present vertical flow device may optionally contain an orientation indicia (63) useful for positioning the positive control (66) and capture/test zones (68) in a fashion such that when a positive test result is formed the positive control line or lines (66) and the capture/test zone or zones (68) are visible in a predetermined orientation. Such predetermined orientations may comprise a reference to the orientation indicia to determine the orientation of a positive control line and/or a test/capture zone. For example, the positive control line may be oriented horizontally and the test zone may be oriented vertically; without limitation, both lines may be in perpendicular relation to one another. In one embodiment a negative test result comprises the formation of a minus symbol (−) as provided in FIG. 8 (66), in a related embodiment a positive test result comprises the formation of a plus symbol (+) FIG. 9 (66 & 69).

[0158] In one aspect, a porous, positive control-support for the porous filter or membrane (FIG. 2 (70)) is positioned in a device below the porous filter or membrane (FIG. 3 (71)). Generally, the porous, positive control-support for the porous filter or membrane is positioned below the porous filter or membrane with respect to the direction of sample introduction (FIG. 10 (70 & 71)). In one aspect, these elements may be “notched” (67) in accordance with the above description to complement the guide rails (62), or means for positioning, provided in the device. In another aspect, the control line (66) is printed onto a positive-control support (65) and guide rails (62) orient this line or element in a predetermined orientation in the device (e.g., horizontally). In a related aspect, this line may become the horizontal component of the “plus” sign formed in a positive test result (FIG. 9) or the horizontal “minus” sign provided in a negative test result (FIG. 8). Such lines or elements may be made by standard printing or other methods described above.

[0159] In one aspect, prior to use, the positive control line (66) is invisible to the naked eye, due to coverage by an opaque dry membrane (69). In one embodiment, after a test is performed through the introduction of a liquid sample, the opaque membrane becomes semi-or fully-transparent, permitting visualization of a positive control line (66). Generally, the positive control line is preferably visible after sample is added, regardless of whether the test result is positive or negative.

[0160] In another aspect, the porous semi-transparent when-wet, porous filter or membrane is notched (67) to fit guide rail or rails (62) or positioning means built into the device sidewall (see FIG. 5, FIG. 7). In a further aspect, a vertical incipient, test zone (68) in the form of, e.g., a line containing capture antibody is present on the new membrane. Prior to introduction of a “positive” sample this line (68) should not be visible to the naked eye. This line becomes the second component (69) of the “plus” sign seen in a positive test result (FIG. 9). The test zone (68) can be made by standard methods used to create immunoassay devices. Such materials and methods are described herein and may be generally known in the art. After a test is performed, if analyte is present that corresponds to the capture reagent located in the zone, a signal is generated in the test zone or line creating a positive test result (69). If the sample does not contain such analyte, a visible test zone is not visible (68). In a particular aspect, the formation of a visible test zone (69), after introduction of a sample containing an analyte of interest, may be taken together with the visibility of a control line (66) as indicia of a positive test result.

[0161] A cross-section of an example vertical flow device is provided in FIG. 10. The device sidewalls (61) in the illustrated device are vertical, however, they may optionally be positioned at an angle sloping inward. For example, the device sidewalls may slope in from the top portion of the well (73) pictured in FIG. 10 down to the top portion of the filter/membrane element (70). The example vertical flow device pictured in FIG. 10 describes the device well (73) where sample is introduced, the filter/membrane elements (70), the positive control elements (71), stop elements (75), absorbent medium (72) and bottom plug (74). In one aspect, this device may feature a new constriction (75) or other means to vertically position the test membrane (70) and its support (71) in the device. Such constriction or stop element (75) may be useful to ensure uniform contact and level placement of the filter/membrane elements (70) and positive control elements (71). Stop elements may be conveniently molded into the outer wall (61), in the form of a shelf or other integrated leveling means, of the presently described vertical flow devices. Alternatively, the device may be assembled by first placing the absorbent (72) in the device (for example, from the bottom or from the top of the device) and by placing the membrane (70) and its positive control support (71) directly on the absorbent (72). Regardless of the method used, in this example it is frequently necessary to maintain direct fluid flow contact between all pictured layers to assure constant flow of liquid from the top chamber into the absorbent medium.

[0162] The invention can be better understood by way of the following examples which are representative of the preferred embodiments, but are not to be construed as limiting the scope of the invention.

EXAMPLES

[0163] Example 1

[0164] A lateral flow test device was constructed according to principles of the present invention. The test device included a G-III plastic bottom (#Z0846500), a G-III plastic scanner top (#Z0440900), a sample pad containing stock assay reagent, a label pad containing stock assay reagent, an observation zone as described below, and an absorbent pad (#0841000).

[0165] A nitrocellulose web assembly membrane from Millipore, trade name Highflow Plus Membrane, was combined with a clear Mylar backing.

[0166] A dark line was made on the inside of the plastic bottom, positioned parallel to sample flow in approximately the same area as would be underneath the fixed minus line from a current assay strip.

[0167] This bottom was then assembled with an experimental G-IV assay strip as described above, and a plastic scanner top. When a liquid sample was added to the test unit, the dark line, which was barely visible through the dry strip, became clearly visible. The results are shown generally in FIG. 2.

[0168] Example 2

[0169] Goat anti-alpha hCG antibodies were immobilized on Hi-flow plus nitrocellulose membrane (nitrocellulose membrane cast on a transparent nylon sheet), manufactured by Millipore Inc. A second, unrelated protein was immobilized on the membrane for the procedural control line. The membrane was then blocked with a protein solution and dried prior to assembly.

[0170] A sample pad (non-woven rayon fiber backed with mylar) was impregnated with a buffered protein solution and dried.

[0171] The label pad (non-woven rayon fiber backed with mylar) was impregnated with a solution containing red colored polystyrene microspheres coated with anti-beta hCG monoclonal antibodies, blue colored polystyrene microspheres coated with a binding pair member to the control line protein, and stabilizing agents followed by a drying process.

[0172] The sample and label pad, the capture membrane and an absorbent pad were then assembled into a test strip similar to FIG. 4.

[0173] A visible line was printed onto the bottom half of the plastic housing of a test cassette. The line was placed directly beneath and perpendicular to the immobilized goat anti-alpha hCG test line on the capture membrane. The preprinted line was approximately 1 mm thick and 5-9 mm long. The assembled test strip was then placed on top of the preprinted line into the bottom of the plastic housing as indicated in FIGS. 1-4, and the cassette was closed with the top portion of the plastic housing. Upon assembly, the preprinted line on the plastic housing was nearly invisible.

[0174] Upon addition of a liquid sample, the sample pad and label pad were re-hydrated and the sample wet the nitrocellulose capture membrane thus making it transparent. The pre-printed line which was barely visible in the dry state was now clearly visible. The results are shown generally in FIG. 4.

[0175] Numerous modifications may be made to the foregoing systems without departing from the basic teachings thereof. Although the present invention has been described in substantial detail with reference to one or more specific embodiments, those of skill in the art will recognize that changes may be made to the embodiments specifically disclosed in this application, yet these modifications and improvements are within the scope and spirit of the invention, as set forth in the claims which follow. All publications or patent documents cited in this specification are incorporated herein by reference as if each such publication or document was specifically and individually indicated to be incorporated herein by reference.

[0176] Citation of the above publications or documents is not intended as an admission that any of the foregoing is pertinent prior art, nor does it constitute any admission as to the contents or date of these publications or documents.

Claims

1. A test device for determining the presence or absence of an analyte in a fluid sample, the test device comprising: a) a support bearing a mark thereon; b) a matrix defining an axial flow path affixed to the support, the matrix comprising: i) a sample receiving zone, at an upstream end of the flow path, that receives the fluid sample, ii) a label zone, on the flow path downstream from the sample receiving zone, comprising a label reagent that binds with the analyte in the fluid sample flowing through the label zone, and iii) an observation area, on the flow path downstream from the label zone, the observation area comprising a defined capture zone having an immobilized capture reagent that restrains the labeled analyte, wherein the observation area comprises a material that is opaque in a dry state and transparent in a moist state; wherein the mark on the support is detectable through the observation area when the observation area is in a moist state, wherein upon restraint of labeled analyte, if present, in the capture zone, the capture zone becomes detectable through the observation area, and wherein both the detectable mark and the detectable capture zone are separately distinguishable.

2. The test device of claim 1, wherein: a) the mark has a shape such that, in the presence or absence of the analyte in the sample, a first symbol is displayed to represent a negative result, and b) the capture zone has a shape such that, taken together with the first symbol in the presence of the analyte in the sample, a second symbol is formed to represent a positive result.

3. The test device of claim 1, wherein: a) the mark has a shape such that, in the presence or absence of the analyte in the sample, a minus symbol (−) is displayed to represent a negative result, and b) the capture zone has a shape such that, taken together with the minus symbol in the presence of the analyte in the sample, a plus symbol (+) is formed to represent a positive result.

4. The test device of claim 3, wherein the longitudinal axis of the mark is in the direction of the sample flow, and the longitudinal axis of the capture zone is perpendicular to the direction of the sample flow.

5. The test device of claim 1, wherein the mark has a shape such that, in the presence or absence of the analyte in the sample, a logo is displayed.

6. The test device of claim 1, wherein the mark has a shape such that, in the presence or absence of the analyte in the sample, one or more predefined symbols are displayed.

7. The test device of claim 1, wherein: a) the mark has a shape such that, in the presence or absence of the analyte in the sample, a first symbol is displayed, and b) the capture zone has a shape such that, independent of the first symbol in the presence of the analyte in the sample, a second symbol is formed to represent a positive result.

8. The test device of claim 1, wherein the observation area further comprises a negative control area.

9. The test device of claim 1, wherein the observation area further comprises a positive control area.

10. The test device of claim 1, further comprising a hollow casing having a sample application aperture and an observation port, wherein the matrix and support are contained within the hollow casing, the sample is applied to the matrix through the aperture, and the observation area can be observed through the port.

11. The test device of claim 1, wherein the device comprises a dipstick.

12. A test device for determining the presence or absence of an analyte in a fluid sample, the test device comprising: a) an intermediate piece bearing a mark thereon; b) a matrix defining an axial flow path, the matrix comprising: i) a sample receiving zone, at an upstream end of the flow path, that receives the fluid sample, ii) a label zone, on the flow path downstream from the sample receiving zone, comprising a label reagent that binds with the analyte in the fluid sample flowing through the label zone, and iii) an observation area, on the flow path downstream from the label zone, the observation area comprising a defined capture zone having an immobilized capture reagent that restrains the labeled analyte, wherein the observation area comprises a material that is opaque in a dry state and transparent in a moist state; wherein the mark on the support is detectable through the observation area when the observation area is in a moist state, wherein upon restraint of labeled analyte, if present, in the capture zone, the capture zone becomes detectable through the observation area, and wherein both the detectable mark and the detectable capture zone are separately distinguishable, and wherein the intermediate piece is disposed between the matrix and a support.

13. The test device of claim 12, wherein the device comprises a dipstick.

14. A method of determining the presence or absence of an analyte in a fluid sample, comprising the steps of: a) providing a support bearing a mark thereon; b) providing a matrix defining an axial flow path, wherein the matrix comprises: i) a sample receiving zone, at an upstream end of the flow path, that receives the fluid sample, ii) a label zone, on the flow path downstream from the sample receiving zone, comprising a label reagent that binds with the analyte in the fluid sample flowing through the label zone, and iii) an observation area, on the flow path downstream from the label zone, the observation area comprising a defined capture zone having an immobilized capture reagent that restrains the labeled analyte, wherein the observation area comprises a material that is opaque in a dry state and transparent in a moist state; c) contacting the sample receiving zone with the fluid sample and allowing the sample to migrate into the test device, thereby subjecting any analyte present in the test sample to react with the label reagent, followed by further migration of the sample into the observation area, thereby subjecting any labeled analyte present in the sample to react with the immobilized capture reagent; and d) detecting analyte restrained in the capture zone by inspecting the observation area, wherein the mark on the support is detectable through the observation area when the observation area is in a moist state, wherein upon restraint of labeled analyte, if present, in the capture zone, the capture zone becomes detectable through the observation area, and wherein both the detectable mark and the detectable capture zone are separately distinguishable.

15. The method of claim 14 wherein the restrained analyte is detected by producing an observable signal that is related to the presence or absence of analyte contained in the sample.

16. A test device for determining the presence or absence of one or more analytes in a sample comprising the test device of claim 1 further comprising a) said support bearing one or more marks thereon, b) said matrix further comprising i) said label zone comprising one or more label reagents that bind with the analytes in the fluid sample, ii) said observation area comprising multiple capture zones having multiple immobilized capture reagents that restrain one or more labeled analytes, wherein said observation is comprised of a material that is opaque in a dry state and transparent in a moist state; wherein said marks are visible through the observation area when the observation area is in a moist state, wherein upon restraint of labeled analyte, if present, in the capture zones, the capture zones become detectable through the observation area, and wherein the detectable marks and the detectable capture zones are separately distinguishable.

17. The test device of claim 16, wherein: a) each of the one or more marks have a shape such that, in the presence or absence of one or more analytes in the sample, first symbols are displayed to represent negative results, wherein each of the one or more marks corresponds with a particular capture zone, and b) each of the capture zones have a shape such that, taken together with the first symbols in the presence of one or more analytes in the sample, second symbols are formed to represent a positive result for each of the analytes.

18. The test device of claim 17 wherein multiple results comprise positive results, negative results, or a combination thereof.

19. The test device of claim 16, wherein: a) each of the one or more marks have a shape such that, in the presence or absence of one or more analytes in the sample, minus symbols are displayed to represent negative results, wherein each of the one or more marks corresponds with a particular capture zone, and b) each of the capture zones have a shape such that, taken together with the minus symbols in the presence of the one or more analytes in the sample, plus symbols are formed to represent a positive results for each of the analytes.

20. The test device of claim 19 wherein multiple results comprise plus symbols, negative symbols, or a combination thereof.

21. The test device of claim 19, wherein the longitudinal axis of the one or more marks are situated in the direction of the sample flow, and the longitudinal axis of the capture zones are perpendicular to the direction of the sample flow.

22. The test device of claim 16, wherein the one or more marks have a shape such that, in the presence or absence of analytes in the sample, identical, or discrete logos are displayed for each discrete analyte.

23. The test device of claim 16, wherein the one or more marks have a shape such that, in the presence or absence of the analytes in the sample, one or more predefined symbols are displayed.

24. The test device of claim 16, wherein: a) each of the one or more marks have a shape such that, in the presence or absence of the one or more analytes in the sample, one or more first symbols are displayed, and b) each of the capture zones are shaped such that, independent of the one or more first symbols, in the presence of the one or more analytes in the sample, one or more second symbols are formed to represent a positive result for each analyte.

25. The test device of claim 24 wherein multiple results comprise positive results, negative results, or a combination thereof.

26. The test device of claim 16, wherein the observation area further comprises one or more negative control areas.

27. The test device of claim 16, wherein the observation area further comprises one or more positive control areas.

28. The test device of claim 16, wherein the label reagents are colored label reagents and the matrix further comprises one or more quantitative control areas defining the color intensity of a given amount of analyte, wherein a higher concentration of analyte corresponds to a higher color intensity.

29. The test device of claim 16, wherein the device comprises a dipstick.

30. The test device of claim 16, further comprising a hollow casing having a sample application aperture and an observation port, wherein the matrix and support are contained within the hollow casing, the sample is applied to the matrix through the aperture, and the observation area can be observed through the port.

31. A method of manufacturing a test device for determining the presence or absence of an analyte in a fluid sample, the method comprising: a) providing a support bearing a mark thereon; b) providing a matrix defining an axial flow path, wherein the matrix comprises: i) a sample receiving zone, at an upstream end of the flow path, that receives the fluid sample, ii) a label zone, on the flow path downstream from the sample receiving zone, comprising a label reagent that binds with the analyte in the fluid sample flowing through the label zone, and iii) an observation area, on the flow path downstream from the label zone, the observation area comprising a capture zone having an immobilized capture reagent that restrains the analyte; wherein the observation area is comprised of a material that is opaque in a dry state and transparent in a moist state, wherein the mark on the support is visible through the observation area when the observation area is in the moist state, wherein upon restraint of labeled analyte, if present, in the capture zones, the capture zones become detectable through the observation area, and wherein the detectable marks and the detectable capture zones are separately distinguishable; and c) disposing said matrix on said support.

32. A method of manufacturing a test device for determining the presence or absence of an analyte in a fluid sample, the method comprising: a) providing an intermediate piece bearing a mark thereon; b) providing a matrix defining an axial flow path, wherein the matrix comprises: i) a sample receiving zone, at an upstream end of the flow path, that receives the fluid sample, ii) a label zone, on the flow path downstream from the sample receiving zone, comprising a label reagent that binds with the analyte in the fluid sample flowing through the label zone, and iii) an observation area, on the flow path downstream from the label zone, the observation area comprising a capture zone having an immobilized capture reagent that restrains the analyte; wherein the observation area is comprised of a material that is opaque in a dry state and transparent in a moist state, wherein the mark on the intermediate piece is visible through the observation area when the observation area is in the moist state, wherein upon restraint of labeled analyte, if present, in the capture zones, the capture zones become detectable through the observation area, and wherein the detectable marks and the detectable capture zones are separately distinguishable; c) wherein the intermediate piece is disposed between the matrix and a support.

33. A test device for determining the presence or absence of an analyte in a fluid sample, the test device comprising: a) a matrix, the matrix comprising: i) a porous first member comprising a capture zone and an observation area, the capture zone having an immobilized capture reagent that restrains the analyte, wherein the first member comprises a material that is opaque in a dry state and transparent in a moist state; and ii) a porous second member bearing a mark thereon, disposed below and contacting said first member, wherein said second member allows flow through the first member into and through the second member when a fluid sample is introduced; and b) wherein the mark on the second member is detectable through the observation area in the first member when the first member is in the moist state; and c) wherein upon introduction of a separate detectable label reagent that binds with the analyte in the fluid sample, the capture zone becomes detectable through the observation area, and wherein the detectable mark and the detectable capture zone are separately distinguishable.

34. The test device of claim 33, wherein: a) the mark has a shape such that, in the presence or absence of the analyte in the sample, a first symbol is displayed to represent a negative result, and b) the capture zone having a shape such that, taken together with the first symbol in the presence of the analyte in the sample, a second symbol is formed to represent a positive result.

35. The test device of claim 33, wherein: a) the mark has a shape such that, in the presence or absence of the analyte in the sample, a minus symbol is displayed to represent a negative result, and b) the capture zone having a shape such that, taken together with the minus symbol in the presence of the analyte in the sample, a plus symbol is formed to represent a positive result.

36. The test device of claim 33, wherein the mark has a shape such that, in the presence or absence of the analyte in the sample, a logo is displayed.

37. The test device of claim 33, wherein the mark has a shape such that, in the presence or absence of the analyte in the sample, one or more predefined symbols are displayed.

38. The test device of claim 33, wherein the first member further comprises a negative control area.

39. The test device of claim 33, wherein the wherein the label reagents are colored label reagents and the first member further comprises a quantitative control area defining the color intensity of a given amount of analyte, wherein a higher concentration of analyte corresponds to a higher color intensity.

40. A test device for determining the presence or absence of one or more analytes in a fluid sample comprising the test device of claim 33 further comprising a) said first member further comprising one or more capture zones having one or more immobilized capture reagents that bind with analytes in the sample, b) said second member further comprising one or more marks that are visible through the observation area of the first member when the first member is in the moist state; and c) wherein upon introduction of separate detectable label reagent that binds with analyte in the fluid sample, the capture zones become detectable through the observation area, and wherein the detectable marks and the corresponding detectable capture zones are separately distinguishable.

41. The test device of claim 40, wherein: a) each of the marks have a shape such that, in the presence or absence of one or more analytes in the sample, first symbols are displayed to represent negative results, and b) each of the capture zones have a shape such that, taken together with the first symbols, in the presence of one or more analytes in the sample, second symbols are formed to represent a positive result for each of the analytes.

42. The test device of claim 40, wherein: a) each of the marks have a shape such that, in the presence or absence of one or more analytes in the sample, minus symbol are displayed to represent negative results, and b) each of the capture zones have a shape such that, taken together with the minus symbols in the presence of one or more analytes in the sample, plus symbols are formed to represent positive results.

43. The test device of claim 40, wherein the marks have a shape such that, in the presence or absence of one or more analytes in the sample, one or more logos are displayed.

44. The test device of claim 40, wherein the marks are shaped such that, in the presence or absence of one or more, analytes in the sample, one or more predefined symbols are displayed.

45. The test device of claim 40, wherein the first member further comprises a negative control area.

46. The test device of claim 40, wherein the label reagents are colored label reagents and the first member further comprises a quantitative control area defining the color intensity of a given amount of analyte, wherein a higher concentration of analyte corresponds to a higher color intensity.

47. The test device of claim 33, wherein the device further comprises an absorbent medium disposed below but in contact with the second member.

48. The test device of claim 33, wherein the device further comprises a registration or indexing means in physical interaction with the first and second members in the device to orient the capture zone in relation to the mark such that, in the presence of analyte, both the capture zone, including labeled reagent bound to the analyte, and the mark are separately distinguishable.

49. The test device of claim 48, wherein, in the presence of analyte, the mark and the capture zone together form an interactive symbol indicating a positive test result.

50. A method of determining the presence or absence of an analyte in a fluid sample, comprising the steps of: a) providing the test device of claim 33;b) contacting the fluid sample with the upper surface of the first member and allowing the sample to migrate through the first and second members, whereby the sample moistens the first member rendering the mark detectable, and analyte, if present, binds to the capture reagent in the first member; c) introducing a detectable label reagent to the upper surface of the first member, wherein said label reagent binds with the analyte within the capture zone rendering the capture zone detectable; d) washing unbound labeled reagent; and e) detecting analyte bound on the first member by inspecting the observation area of the first member, wherein the detectable mark and the corresponding detectable capture zone are separately distinguishable.

51. The method of claim 50 wherein the presence or absence of multiple analytes are determined.