The invention relates to a test strip for paper-based assays. The invention further relates to a method of detecting an analyte in a sample using said test strip.
Paper-based assays such as the dipstick and lateral flow tests are available as low-cost screening devices for many physiological-relevant compounds in bodily fluids. Paper-based assays utilize test strips that rely on the use of enzymes or bio/chemistry principles to enable detections of analytes or nucleotides or antibodies conjugated to detector molecules for analyte detection.
An important limitation of test strips used in lateral flow tests is the sensitivity of the test strip due to the poor limit-of-detection of the detector molecules used to visualize the results. Poor limit-of-detection translates to a larger sample requirement. While this limitation can be overcome via using the enzyme-substrate or horseradish peroxidase (HRP) with tetramethylbenzidine (TMB) amplification approach, a minimum waiting time is required prior to activation of the substrate addition step. As such, this introduces the possibility of human error. If the user activates the addition step too early, false negatives can arise. Another limitation of the enzyme-substrate amplification approach is the rate at which the enzymatic substrate contacts the test zone, which directly affects the rate of transport of the substrate to the enzymes and therefore assay sensitivity.
There is therefore a need to provide a test strip that overcomes, or at least ameliorates, one or more of the disadvantages described above.
In one aspect, there is provided a test strip for a paper-based assay comprising, a substrate addition zone for receiving a substrate and a test zone, said test zone comprising a capture agent, wherein the substrate addition zone is located upstream of said test zone.
In one aspect, there is provided a paper-based enzyme assay comprising a test strip as described herein.
In one aspect, there is provided a method of detecting the presence of an analyte in a sample, said method comprising the steps of: a) contacting said sample onto said test zone of a test strip as described herein; b) dispensing a substrate onto the substrate addition zone; and c) detecting an emitted signal from said test zone to confirm the presence or absence of said analyte in said sample.
In one aspect, there is provided a method of detecting the presence of an analyte in a sample, said method comprising the steps of: a) contacting said sample onto said detector zone of a test strip as described herein; b) dispensing a substrate onto the substrate addition zone; and c) detecting an emitted signal from said test zone to confirm the presence or absence of said analyte in said sample.
The term “antigen binding protein” as used herein refers to antibodies, antibody fragments and other protein constructs, such as domains, which are capable of binding to an antigen.
The term “antibody” is used herein in the broadest sense to refer to molecules with an immunoglobulin-like domain and includes monoclonal, recombinant, polyclonal, chimeric, humanised, bispecific and heteroconjugate antibodies; a single variable domain, a domain antibody, antigen binding fragments, immunologically effective fragments, single chain Fv, diabodies, Tandabs™, etc (for a summary of alternative “antibody” formats see Holliger and Hudson, Nature Biotechnology, 2005, Vol 23, No. 9, 1126-1136).
The phrase “single variable domain” refers to an antigen binding protein variable domain (for example, VH, VHH, VL) that specifically binds an antigen or epitope independently of a different variable region or domain.
A “domain antibody” or “dAb” may be considered the same as a “single variable domain” which is capable of binding to an antigen. A single variable domain may be a human antibody variable domain, but also includes single antibody variable domains from other species such as rodent, nurse shark and Camelid VHH dAbs. Camelid VHH are immunoglobulin single variable domain polypeptides that are derived from species including camel, llama, alpaca, dromedary, and guanaco, which produce heavy chain antibodies naturally devoid of light chains. Such VHH domains may be humanised according to standard techniques available in the art, and such domains are considered to be “domain antibodies”. As used herein VH includes camelid VHH domains.
As used herein the term “domain” refers to a folded protein structure which has tertiary structure independent of the rest of the protein. Generally, domains are responsible for discrete functional properties of proteins, and in many cases may be added, removed or transferred to other proteins without loss of function of the remainder of the protein and/or of the domain. A “single variable domain” is a folded polypeptide domain comprising sequences characteristic of antibody variable domains. It therefore includes complete antibody variable domains and modified variable domains, for example, in which one or more loops have been replaced by sequences which are not characteristic of antibody variable domains, or antibody variable domains which have been truncated or comprise N- or C-terminal extensions, as well as folded fragments of variable domains which retain at least the binding activity and specificity of the full-length domain. A domain can bind an antigen or epitope independently of a different variable region or domain.
An antigen binding fragment may be provided by means of arrangement of one or more CDRs on non-antibody protein scaffolds such as a domain. The domain may be a domain antibody or may be a domain which is a derivative of a scaffold selected from the group consisting of CTLA-4, lipocalin, SpA, an Affibody, an avimer, GroEI, transferrin, GroES and fibronectin/adnectin, which has been subjected to protein engineering in order to obtain binding to an antigen, other than the natural ligand.
An antigen binding fragment or an immunologically effective fragment may comprise partial heavy or light chain variable sequences. Fragments are at least 5, 6, 8 or 10 amino acids in length. Alternatively the fragments are at least 15, at least 20, at least 50, at least 75, or at least 100 amino acids in length.
The term “specifically binds” as used throughout the present specification in relation to antigen binding proteins means that the antigen binding protein binds to a specific antigen of interest with no or insignificant binding to other proteins. However, the term does not exclude the fact that the antigen binding proteins may also be cross-reactive with closely related molecules. The antigen binding proteins described herein may bind to an antigen with at least 2, 5, 10, 50, 100, or 1000 fold greater affinity than they bind to closely related molecules.
As used herein, the term “analyte” refers to a compound of interest. It will be generally understood that an analyte includes but is not limited to an antigen, antibody, hormone, drug, therapeutic, cell protein, nucleic acid, cardiac marker, tumor or cancer marker, autoimmune disease marker, or any macromolecule. For example, an antigen analyte can be an antigen associated with an infectious agent such as a virus, a bacterium, a fungus, or a prion. An example of a hormone analyte includes but is not limited to hCG, thyroxine, TSH, glucagons, insulin, relaxin, prolactin, luteinizing hormone, melanotropin, somatotropin, follicle-stimulating hormone, gastrin, bradykinin, vasopressin, and other releasing factors; other hormones of physiological or pathological interest can be the analyte. An example of an analyte that is a cancer or tumor marker includes but is not limited to prostate specific antigen (PSA), carcinoembryonic antigen (CEA), and α-fetoprotein. However, other cancer or tumor markers can be the analyte. An example of a drug analyte includes but is not limited to an opiate. Examples of an antibody analyte include but are not limited to immunoglobulins such as IgG, IgM, IgA, IgE and IgD. An example of a therapeutic analyte includes but is not limited to doxorubicin.
As used herein, the term “sample” refers to a biological sample or non-biological sample. Biological sample refers to a sample obtained from a biological subject, including a sample of biological tissue or fluid origin obtained in vivo or in vitro. Such samples can be, but are not limited to blood, blood plasma, serum, buccal smear, amniotic fluid, prenatal tissue, sweat, nasal swab or urine, organs, tissues, fractions, and cells isolated from mammals including humans. Biological samples also may include sections of the biological sample including tissues (e.g., sectional portions of an organ or tissue). Biological samples may also include extracts from a biological sample, for example, an antigen from a biological fluid (e.g., blood or urine). A non-biological sample includes but is not limited to water from some ecological niche, e.g., a river or a lake; or a solution used in a laboratory.
As used herein, the term “applicator” refers to a device to apply a compound onto a test strip. An applicator may be a membrane, including but not limited to porous membranes, such as a filter membrane. Examples of filter membranes include but are not limited to Fusion5 from Whatman™, glass fibers, symmetric and asymmetric polyethersulfone membranes, CytoSep™ and cellulose filter membranes.
As used herein, the term “porous membrane” refers to a membrane with pores. Examples of porous membrane include but are not limited to porous membranes may be selected from the group consisting of cellulose acetate, cellulosic paper, filter paper, tissue paper, writing paper, paper towel, cloth, or porous polymer film nitrocellulose membrane, polyvinylidene fluoride (PVDF) membrane and filter paper. In one embodiment, the porous membrane is a nitrocellulose membrane such as nitrocellulose acetate.
As used herein the terms “applied” or “contacted” may be used interchangeably with respect to the applicator.
As used herein, the term “nucleic acid” refers to any single or double-stranded RNA or DNA molecule, such as mRNA, cDNA, and genomic DNA.
As used herein, the term “oligonucleotide” refers to a single-stranded nucleotide polymer made of more than 2 nucleotide subunits covalently joined together. Preferably between 10 and 100 nucleotide units are present, most preferably between 12 and 50 nucleotides units are joined together. The sugar groups of the nucleotide subunits may be ribose, deoxyribose or modified derivatives thereof such as 2′-O-methyl ribose. The nucleotide subunits of an oligonucleotide may be joined by phosphodiester linkages, phosphorothioate linkages, methyl phosphonate linkages or by other rare or non-naturally-occurring linkages that do not prevent hybridization of the oligonucleotide. Furthermore, an oligonucleotide may have uncommon nucleotides or nonnucleotide moieties. An oligonucleotide as defined herein is a nucleic acid, preferably DNA, but may be RNA or have a combination of ribo- and deoxyribonucleotides covalently linked. Oligonucleotide probes and amplification oligonucleotides of a defined sequence may be produced by techniques known to those of ordinary skill in the art, such as by chemical or biochemical synthesis, and by in vitro or in vivo expression from recombinant nucleic acid molecules, e.g., bacterial or retroviral vectors. As intended by this disclosure, an oligonucleotide does not consist of wild-type chromosomal DNA or the in vivo transcription products thereof. One use of a probe is as a hybridization assay probe; probes may also be used as in vivo or in vitro therapeutic amplification oligomers or antisense agents to block or inhibit gene transcription, or translation in diseased, infected, or pathogenic cells.
As used herein, the term “peptide” refers to two or more amino acid molecules linked by amide bonds. Peptides may be naturally occurring or synthetic.
The invention will be better understood with reference to the detailed description when considered in conjunction with the non-limiting examples and the accompanying drawings, in which:
In one aspect, there is provided a test strip for a paper-based assay comprising, a substrate addition zone for receiving a substrate and a test zone, said test zone comprising a capture agent, wherein the substrate addition zone is located upstream of said test zone.
It will be generally understood that the substrate addition zone is located upstream of the test zone with respect to the direction of flow of liquid through and/or along said test strip.
In some embodiments, the substrate addition zone and the test zone are in a spaced part configuration. Spaced apart would be generally understood to mean that the substrate addition zone and test zone may be arranged anywhere on the test strip apart from each other, whilst maintaining the upstream location of the substrate addition zone with respect to the test zone. In other words, the test zone and substrate addition zone may be located on the test strip in any spaced apart relationship with respect to one another. For example, the substrate addition zone may be situated at one end or end region of the test strip and the test zone may be situated at the opposite end or end region of the test strip. The substrate addition zone and the test zone may also be situated in the middle region of the test strip.
In some embodiments, the substrate addition zone and the test zone are in an adjacent configuration.
In some embodiments, the substrate addition zone and the test zone are in an immediately adjacent configuration.
In some embodiments, the substrate addition zone and the test zone are situated on the test strip such that fluid flow may be direct from the substrate addition zone to the test zone. In other words, fluid flow from the substrate addition zone to the test zone is not interposed by any other zone or chemical addition, as is exemplified in
In other embodiments, the substrate addition zone and the test zone may be interposed by a detector zone.
In some embodiments, the sample may be premixed with a detector agent. It will be appreciated that the sample premixed with a detector agent may be contacted with the test strip at the test zone.
In some embodiments, the detector agent may be pre-dried onto the detector zone or test zone.
In some embodiments, the detector agent may be pre-dried onto an applicator. It will generally be understood that pre-drying refers to drying the detector agent onto the detector zone or test zone on the test strip or applicator prior to using the test strip. Drying the detector agent may take place in a vacuum or at atmospheric pressure. Drying the detector agent may also take place at ambient temperature or at temperatures above or below ambient temperature. It will also be appreciated that the detector agent may be dried at various levels of relative humidity. For example, 100%, 95%, 90%, 85%, 80%, 75%, 70%, 65%, 60%, 55%, 50%, 45%, 40%, 35%, 30%, 25%, 20%, 15%, 10%, 5%, 0%. It will generally be understood that the length of time of drying the detector agent will vary according to the conditions employed. The detector may also be dried with one or more additional compounds including but not limited to preservatives, proteins and/or surfactants. Examples of preservatives include but are not limited to sucrose and trehalose. An example of a protein that may be dried with the detector is bovine serum albumin (BSA). An example of a surfactant that may be dried with the detector is polysorbate 20. It will generally be appreciated that drying the detector with one or more additional compounds may confer stability during long-term storage.
In some embodiments, the detector agent may be pre-dried onto an applicator. It will be generally understood that an applicator may be any absorbent or porous material. For example, an applicator may be a membrane such as a filter membrane. It will also be generally understood that a membrane may be a single layer membrane or a plurality of layers. Examples of an applicator include but are not limited to Fusion5 from Whatman™, glass fibers, CytoSep™, symmetric and asymmetric polyethersulfone membranes, and cellulose filter membranes.
In one embodiment, an applicator may be a conjugate pad comprising a detector-agent conjugated to an enzyme.
It will be generally understood that the applicator may be untreated or treated prior to the addition of a detector agent. Pre-treatment of the applicator includes but is not limited to washing the applicator with compounds such as preservative, proteins and/or surfactants. Examples of preservative include but are not limited to sucrose and trehalose. Examples of proteins include but are not limited to bovine serum albumin (BSA). Examples of surfactants include but are not limited to polysorbate 20.
It will also be appreciated that the applicator may be cut to an appropriate size prior to use. The material, thickness, number of layers and size of the applicator used will be generally understood to vary based on the assay in question. The applicator will be applied onto the test zone or detector zone prior to the start of the assay.
In some embodiments, the sample may be contacted with the test strip at the test zone. In other embodiments, the sample is contacted with the test strip at the interposed detector zone.
In some embodiments, the sample may be applied onto the applicator.
In some embodiments, the applicator may be applied onto the test strip and the sample may be applied onto the applicator.
In some embodiments, the applicator may be removed from the test strip prior to addition of the substrate but after addition of the sample. The applicator may be removed after 1 s, 5 s, 10 s, 20 s, 30 s, 45 s, 1 min, 2 min, 3 min, 4 min, 5 min, 6 min, 7 min, 8 min, 9 min 10 min.
In other embodiments, the applicator may not be removed prior to addition of the substrate.
The detector agent may be selected from the group consisting of antibodies, antigens, oligonucleotides and peptides. It will be appreciated that the detector agent may be conjugated to a detectable material such as a coloured agent, a fluorescent agent, an enzyme or a chemiluminescent agent. For example, the detector agent may be conjugated to an enzyme selected from the group consisting of alkaline phosphatase, beta-galactosidase, glucose oxidase, glucose dehydrogenase and horseradish peroxidase. It will be appreciated that the detector agent will bind to an analyte of interest. It will also be appreciated that the enzyme conjugated on the detector agent will react with the substrate to emit a signal.
In one embodiment, the test strip is a porous membrane. Suitable porous membranes may be selected from the group consisting of cellulose acetate, cellulosic paper, filter paper, tissue paper, writing paper, paper towel, cloth, or porous polymer film nitrocellulose membrane, polyvinylidene fluoride (PVDF) membrane and filter paper. In one embodiment, the porous membrane is a nitrocellulose membrane such as nitrocellulose acetate.
In one embodiment, the test zone is subdivided into two or more areas, each area comprising the same or different capture agent. In some embodiments, each area may comprise one or more than one capture agent. In some embodiments, the test zone may occupy a footprint from a single test spot to an array of test spots 2×1, 2×2, 3×1, up to but not limited to 4×4, covering an area of up to 4×4 cm. The at least two or more areas may comprise the same or different capture agent. In some embodiments, the test strip may comprise more than one test zone. In other embodiments, the test strip may comprise an array of test zones, each test zone may occupy a footprint from a single test spot to an array of test spots 2×1, 2×2, 3×1, up to but not limited to 4×4, covering an area of up to 4 cm×4 cm. In some embodiments, the capture agent may be selected from the group consisting of antibodies, antigens, oligonucleotides and peptides. It will be appreciated that the capture agent specifically binds to an analyte of interest and retains the analyte of interest on the test zone. In one embodiment, the or each capture agent may be mixed with a coloured marker to assist in the localization of the or each capture agent on said test strip. Examples of colour markers include but are not limited to dyes and coloured beads. It will be appreciated that dyes such as water dye, food dye, poster colour and colours that generically absorbs on porous membranes may be used. It will also be appreciated that coloured beads include but are not limited to dyed polystyrene beads, nanoparticles such as gold or silver nanoparticles and cerium nanoparticles.
In another embodiment, coloured beads may be mixed with the captured antibody and dispensed onto the test zone during the membrane preparation phase. An advantage of using coloured beads is that these produce a light, but observable colour to enable users to identify the test zone. A further advantage is that since coloured beads are used, the colour will persist throughout the experiment.
In one embodiment, the test strip further comprises one or more control areas located within or without of the test zone. The control area may be downstream or upstream of the test zone relative to the flow of the liquid through and/or along said test strip. The control area may be one or more spots in an array of test spots within the test zone.
In one embodiment, the test zone is marked on the test strip. Marking the test zone may assist the user to accurately dispense the mix onto the test zone. The test zone is marked on the test strip with a dye or an outline. It will generally be understood that the test zone may be marked by an indication line or circle. The dye may be a washable dye. For example, water dye, food dye, poster colour and colours that generically absorbs on porous membranes.
In some embodiments, the substrate may be an enzymatic substrate. The enzymatic substrate may be converted into a product that emits a signal. Suitable examples of such substrate include 5-Bromo-4-chloro-3-indolyl phosphate (BCIP), nitroblue tetrazolium (NBT) or combined BCIP/NBT, tetramethylbenzidine (TMB), diaminobenzidine (DAB), glucose/electron acceptor, glucose/potassium ferricyanide/Fe3+ and 5-bromo-4-chloro-3-indolyl-β-D-galactopyranoside (X-gal). It will be understood to a skilled person that other enzymatic substrates known in the art would be possible.
In one embodiment, the substrate may be contacted with the test strip as an aqueous solution. In another embodiment, the substrate may be contacted with the test strip as a polymer solution. It will generally be understood that a polymer solution refers to a polymeric solution prior to the polymeric solution setting into a gel. In yet another embodiment, the substrate may be contacted with the test strip in a polymer gel. It will generally be understood that the substrate may be added upstream at the substrate addition zone. It will also be appreciated that the substrate may be added via a cavity under the test strip. It will also be appreciated that the substrate may be added onto the test strip.
In some embodiments, the substrate is polymerized in polyacrylamide. In some embodiments, the substrate may be mixed with precast polymeric gels before flowing. The choice of polymeric gel includes, but not limited to, polyacrylamide gels. The advantage of applying gels to substrate is to improve the contact between the substrate and test zone. In addition, the curing of gels may consume the excess, unreacted substrate to improve the signal stability.
In some embodiments, the substrate may be dispensed onto the test strip. In other embodiments, the substrate may be dispensed onto the underside of the test strip. For example, the aqueous solution, polymeric solution or polymeric gel comprising the substrate may be dispensed onto the test strip. In another example, the aqueous solution, polymeric solution or polymeric gel comprising the substrate may be dispensed onto the underside of the test strip. In some embodiments, when the substrate is dispensed onto the underside of the test strip, this dispensing step is via a cavity underneath the test strip.
In some embodiments a sample is contacted with the test strip directly at the test zone. In one embodiment, a sample is dispensed onto said test zone. The sample may be one of blood, urine, saliva, sweat, nasal swab with or without a suitable buffer, and with or without a detector, or a mix of at least two of blood, urine, saliva, sweat, nasal swab with or without a suitable buffer, and with or without a detector. The sample may be added in the range of 0.1 to 100 μl. For example, 0.1 μl to 100 μl, 0.5 μl to 95 μl, 1 μl to 90 μl, 1.5 μl to 85 μl, 2 μl to 80 μl, 2.5 μl to 75 μl, 3 μl to 70 μl, 3.5 μl to 65 μl, 4 μl to 60 μl, 4.5 μl to 55 μl, 5 μl to 50 μl, 5.5 μl to 45 μl, 6 μl to 40 μl, 6.5 μl to 35 μl, 7 μl to 30 μl, 7.5 μl to 30 μl, 8 μl to 25 μl, 8.5 μl to 20 μl, 9 μl to 15 μl, 9.5 μl to 10 μl.
In one aspect, there is provided a paper-based enzyme assay comprising a test strip as described herein.
In one aspect, there is provided a method of detecting the presence of an analyte in a sample, said method comprising the steps of: a) contacting said sample onto said test zone of a test strip as described herein, wherein said sample comprises a detector antibody specific for said analyte; b) dispensing a substrate onto the substrate addition zone; and c) detecting an emitted signal from said test zone to confirm the presence or absence of said analyte in said sample.
In one aspect, there is provided a method of detecting the presence of an analyte in a sample, said method comprising the steps of: a) contacting said sample onto said detector zone of a test strip as described herein,; b) dispensing a substrate onto the substrate addition zone; and c) detecting an emitted signal from said test zone to confirm the presence or absence of said analyte in said sample.
In some embodiments, the sample may be contacted onto the test zone or the detector zone directly.
In some embodiments, the sample may be contacted onto the test zone or detector zone via the applicator located at the test zone or detector zone.
In some embodiments, the applicator may be applied onto or contacted with the test zone. In other embodiments, the applicator may be applied onto or contacted with the detector zone. It will be appreciated that the sample may be added onto the applicator either in situ on the test strip or prior to contacting the test strip with the applicator.
It will be appreciated that the applicator may be removed prior to substrate addition. It will also be appreciated that the applicator may be removed at any time prior to the substrate front reaching a zone where the applicator was applied. For example, the test zone or the detector zone. For example, the applicator may be applied onto the test zone or detector zone and the sample may then be added onto the applicator. The applicator may then be removed prior to substrate addition, or after substrate is added but prior to the substrate front reaching the applicator. In another example, the applicator may be applied onto the test zone or detector zone. The applicator may then be removed and the sample may be added onto the zone from which the applicator was removed. Subsequently, substrate may be added.
The emitted signal may be detected by means of a colour change, a chemiluminescent detector such as a charge-coupled device (CCD) imager or X-ray or a plate reader. It will be appreciated that other methods of detection known in the art may be used. These include but are not limited to fluorescence, radioactive, electrochemiluminescence and electrochemical detection methods.
In one embodiment, step (b) may immediately follow step (a) with no waiting time in between steps (a) and (b). In another embodiment, step (a) may be followed by an incubation period prior to step (b). Incubation period may be from between 1 second to 10 minutes. For example, between 10 seconds to 10 minutes, between 20 seconds to 9 minutes, between 30 seconds to 8 minutes, between 30 seconds to 7 minutes, between 40 seconds to 6 minutes, between 50 seconds to 5 minutes, between 1 minute to 4 minutes, between 2 minutes to 3 minutes. In some embodiments, incubation of the test strip after step (a) permits the sample to interact with the capture agent at the test zone and increase the signal. In other embodiments, incubation of the test strip after step (a) permits the sample to interact with the detector agent at the detector zone and increase the signal. It will be generally understood that the incubation period may be varied depending on the sample and capture agent used.
In one embodiment, the signal is a colourimetric signal. In another embodiment, the signal is a fluorescent signal. In yet another embodiment, the signal is a chemiluminescent signal. It another embodiment, the signal is an electrochemiluminescent signal. In another embodiment, the signal is an electrochemical signal.
In some embodiments, the test strip may be washed after step (a). In other embodiments, the test strip may be washed after step (b). In yet other embodiments, the test strip may be washed after step (a) and after step (b).
The wash step can be introduced by a droplet of wash buffer onto the test membrane thus ensuring that excess unbound sample or substrate is washed downstream before the test zone contacts the substrate. The mentioned droplet may range from 10 μl to 500 μl. For example, 15 μl to 450 μl, 20 μl to 400 μl, 25 μl to 350 μl, 30 μl to 350 μl, 35 μl to 300 μl, 40 μl to 250 μl, 45 μl to 200 μl, 50 μl to 150 μl, 55 μl to 100 μl, 60 μl to 100 μl, 70 μl to 90 μl or 80 μl to 90 μl.
Advantageously, the invention described herein provides improved paper-based assay results, including cleaner signal readout, reduction in false positives and/or false negatives and improved efficiency in obtaining results.
The invention illustratively described herein may suitably be practiced in the absence of any element or elements, limitation or limitations, not specifically disclosed herein. Thus, for example, the terms “comprising”, “including”, “containing”, etc. shall be read expansively and without limitation. Additionally, the terms and expressions employed herein have been used as terms of description and not of limitation, and there is no intention in the use of such terms and expressions of excluding any equivalents of the features shown and described or portions thereof, but it is recognized that various modifications are possible within the scope of the invention claimed. Thus, it should be understood that although the present invention has been specifically disclosed by preferred embodiments and optional features, modification and variation of the inventions embodied therein herein disclosed may be resorted to by those skilled in the art, and that such modifications and variations are considered to be within the scope of this invention.
The invention has been described broadly and generically herein. Each of the narrower species and subgeneric groupings falling within the generic disclosure also form part of the invention. This includes the generic description of the invention with a proviso or negative limitation removing any subject matter from the genus, regardless of whether or not the excised material is specifically recited herein.
Other embodiments are within the following claims and non-limiting examples. In addition, where features or aspects of the invention are described in terms of Markush groups, those skilled in the art will recognize that the invention is also thereby described in terms of any individual member or subgroup of members of the Markush group.
Non-limiting examples of the invention, including the best mode, and a comparative example will be further described in greater detail by reference to specific Examples, which should not be construed as in any way limiting the scope of the invention.
Materials and Methods
Paper-Based Wash-Free ELISA Procedure and Colourimetric Results Using Nitrocellulose Membranes.
Prior to performing the paper-based wash-free ELISA, the nitrocellulose membrane strip 101 was prepared with a test spot/line 201 and control spot/line 202 (
To start the ELISA (
Results and Discussion
Distinct colorimetric results can be obtained, on the test spots, for the AP with BCIP/NBT system (
Materials and Methods
Paper-based Wash-free ELISA Array Procedure and Colourimetric Results using Nitrocellulose Membranes.
Prior to performing the array of paper-based wash-free ELISA, the nitrocellulose membrane strip 101 was prepared with an array of test spots 201a and control spot/line 202 (
To start the ELISA (
Results and Discussion
Distinct colourimetric results can be obtained, on the test spots, for the AP with BCIP/NBT system (
Visualization of the test spots can be achieved using either water-soluble dyes or water-insoluble dyes (
Water-insoluble dyes can also be spotted onto the test spots to indicate where the sample-detector mixture should be introduced and where results should be expected (
Example 4
In another embodiment, the enzyme conjugate is dried at region 207, or anywhere between the test zone 201/201a and region 203. This allows for direct dispensing of biological samples 301 onto the test zone 201/201a with minimum sample preparation. The colourimetric substrate then is introduced upstream before it flows underneath the porous test membrane and within cavity 205 after wash-buffer is introduced through the test strip 101 at region 204.
Yet in another embodiment, the sample 301 or sample-detector mixture 301a may be dispensed at Region 203 instead of the test zone 201/201a. This technique is useful when the test requires a large amount of mix flows through the test zone. The amount of mix may range from 5 μl to 400 μl. The colourimetric substrate then is introduced upstream before it flows underneath the porous test membrane and within cavity 205 after wash-buffer is introduced through the test strip 101 at region 204.
As depicted in
To prepare the platform, 1% ammonium persulfate (dissolved in water) was coated and dried on the base 206 of the device (
To prepare the substrate mix, acrylamide and bis-acrylamide solution were first mixed at a ratio of 19:1, followed by dissolution in water to obtain a 30% solution (
Significance of Sample Location Spotting on Colourimetric Results.
Use of Impregnated Detector Enzyme Conjugate System
Prior to performing the paper-based ELISA, the nitrocellulose membrane was prepared with a test spot/line 201 and a control spot/line 202, and an upstream region 207 was impregnated with dried detector antibody-AP conjugate (
To start the ELISA (
Results and Discussion
Colourimetric results were obtained from using this set of hCG concentrations (
Preparation of Conjugate Pad
RBC filter membranes (e.g. Fusion5 from Whatman) are first cut into desired diameters to handle the appropriate volume of whole blood samples. Although it is not necessary for the assay to work, pre-treatment of the filter membranes (e.g. with surfactants such as polysorbate 20) can be performed to reduce protein adsorption. Next, the desired detector agent-enzyme conjugate is dispensed onto these RBC filter membrane discs and dried. The desired detector agent-enzyme conjugate can be dried in the presence of sucrose and/or trehalose to preserve its stability during long-term storage. The filter membrane containing dried detector agent-enzyme is herein defined as conjugate pad 104.
Performing of Paper-Based ELISA
A representative method for assembly of the conjugate pad 104 with the test strip is illustrated in
In a preferred embodiment, performing the paper-based ELISA is initiated via direct introduction of sample 301 onto conjugate pad 104 and where sample 301 will dissolve the dried detector agent-enzyme conjugate. Any analyte of interest present in sample 301 will react with this conjugate to form an analyte-detector antibody complex. As conjugate pad 104 is in direct contact with test spot/line 201, the non-particulate components in solution (e.g. detector agent-enzyme conjugate and any analyte-detector agent complex) from sample 301 will be filtered through conjugate pad 104, and gets transferred directly onto test spot/line 201. Any analyte-detector antibody complex present will bind with capture agents within test spot/line 201. Enzymatic substrate 302 is introduced directly onto substrate pad 102, after removal of conjugate pad 104, and will migrate along substrate pad 102 and reaction matrix 101 before reaching absorbent pad 103. (NB: Removal of contact between conjugate pad 104 and reaction matrix 101 is crucial to prevent non-specific colorimetric smearing of reaction matrix 101.) Due to differential migration of components in enzymatic substrate 302, any detector agent-enzyme conjugate not binding to test spot/line 201 will get washed downstream and binds to capture agents in control spot/line 202 before reacting with the enzymatic substrate components present in enzymatic substrate 302. If the analyte is present in sample 301, both test spot/line 201 and control spot/line 202 will eventually show colorimetric results; whereas if the analyte is not present in sample 301, only the control spot/line 202 will eventually show colorimetric results.
Hepatitis B Surface Antigen (HbsAg) Paper-Based ELISA Using RBCs Filter Membranes as Conjugate Pads and Assembled on Top of the Test Spots
Briefly, the paper platform (nitrocellulose membrane) strip was prepared with a test spot by dispensing anti-hepatitis B surface antigen (HbsAg) antibody (capture antibody) upstream of the strip. The strips were vacuum dried, blocked using 1×PBS with 2% BSA and 0.02% Tween®20, and then washed with 5 mM of phosphate buffer in double distilled H2O, pH ˜7.6. Finally, the strips were vacuum dried again to allow complete removal of water. “Whole blood samples” were obtained by mixing packed red blood cells with serum in the volume ratio of 1:1. Hepatitis B negative “whole blood sample” were obtained by using the mixed sample as it was. Hepatitis B positive “whole blood sample” were obtained by spiking recombinant HBsAg into the “whole blood sample” at a concentration of 4300 ng/mL. The detector component, anti-HBsAg antibody-AP conjugate, was dried on a red blood cell filter membrane (e.g. Fusion5) disc. The desired concentration was preferably ˜1 μg/mL, and dried in 1 mM Tris buffer pH ˜7.4 with 2% sucrose and 0.2% BSA. The red blood cell filter membrane containing the dried anti-HBsAg antibody-AP conjugate was termed the conjugate pad. This conjugate pad was directly assembled on top of the test spot before starting the HBsAg paper-based ELISA. To start the HBsAg paper-based ELISA, ˜5 □L of “whole blood sample” was first aspirated into the droppers before dispensing onto the conjugate pad. The conjugate pad was next removed (when sufficient serum samples have been transferred onto the paper platform strip) and excess BCIP/NBT substrate was immediately added upstream of the test spot. After 15 min of substrate addition, the strips were washed with 1× Tris-buffered saline, 0.1% Tween®20. Finally, the strips were scanned using a scanner to obtain digital images for image analysis using ImageJ.
Results for the HBsAg paper-based ELISA (using RBCs filter membranes as conjugate pads and assembled on top of the test spots) are shown in
Preparation of Conjugate Pad
RBC filter membranes (e.g. Fusion5 from Whatman) are first cut into desired diameters to handle the appropriate volume of whole blood samples. Although it is not necessary for the assay to work, pre-treatment of the filter membranes (e.g. with surfactants such as polysorbate 20) can be performed to reduce protein adsorption. Next, the desired detector agent-enzyme conjugate is dispensed onto these RBC filter membrane discs and dried. The desired detector agent-enzyme conjugate can be dried in the presence of sucrose and/or trehalose to preserve its stability during long-term storage. The filter membrane containing dried detector agent-enzyme is herein defined as conjugate pad 104.
An alternative representative method for assembling the conjugate pad 104 with the test strip is illustrated in
In a preferred embodiment, performing the paper-based ELISA is initiated via direct introduction of sample 301 onto conjugate pad 104, and where sample 301 will dissolve the dried detector agent-enzyme conjugate. Any analyte of interest present in sample 301 will react with this conjugate to form an analyte-detector antibody conjugate. As conjugate pad 104 is in direct contact with reaction matrix 101, the non-particulate components in solution (e.g. detector agent-enzyme conjugate and any analyte-detector agent complex) from sample 301 will filter through conjugate pad 104, and gets transferred directly onto reaction matrix 101. Enzymatic substrate 302 is introduced directly onto substrate pad 102 after removal of conjugate pad 104, and will migrate along substrate pad 102 and reaction matrix 101 before reaching absorbent pad 103. (NB: Removal of contact between conjugate pad 104 and reaction matrix 101 is crucial to prevent non-specific colorimetric smearing of reaction matrix 101.) Due to differential migration of components in enzymatic substrate 302, the detector agent enzyme complex or analyte-detector antibody conjugate will get washed downstream before reacting with the enzymatic substrate components present in enzymatic substrate 302. During the downstream washing process, the analyte-detector antibody complex (if any) will bind with capture agents within test spot/line 201, whereas the detector agent-enzyme conjugate will bind to capture agents in control spot/line 202. If the analyte is present in sample 301, both test spot/line 201 and control spot/line 202 will eventually show colorimetric results; whereas if the analyte is not present in sample 301, only the control spot/line 202 will eventually show colorimetric results.
Hepatitis B Surface Antigen (HBsAg) Paper-Based ELISA Using RBCs Filter Membranes as Conjugate Pads and Assembled Upstream of the Test Spots
Briefly, the paper platform (nitrocellulose membrane) strip was prepared with a test spot by dispensing anti-hepatitis B surface antigen (HbsAg) antibody (capture antibody) upstream of the strip. The strips were dried, blocked using 1×PBS with 2% BSA with 0.02% Tween®20, and then washed with 5 mM of phosphate buffer in double distilled H2O, pH ˜7.6. Finally, the strips were dried again to allow complete removal of water.
“Whole blood sample” was obtained by mixing packed red blood cells with serum in the volume ratio of 1:1. Hepatitis B negative “whole blood sample” was obtained by using the mixed sample as it is. Hepatitis B positive “whole blood sample” were obtained by spiking recombinant HBsAg into the “whole blood sample” at a concentration of 4300 ng/mL. The detector component, anti-HBsAg antibody-AP conjugate, was dried on a red blood cell filter membrane (e.g. Fusion5) disc. The desired concentration was preferably ˜1 μg/mL, and dried in 1 mM Tris buffer pH ˜7.4 with 2% sucrose and 0.2% BSA. The red blood cell filter membrane containing the dried anti-HBsAg antibody-AP conjugate was termed the conjugate pad. This conjugate pad was assembled upstream of the test spot (but downstream of the enzymatic substrate addition region) before starting the HBsAg paper-based ELISA. To start the HBsAg paper-based ELISA, ˜5 □L of “whole blood sample” was first aspirated into the droppers before dispensing onto the conjugate pad. The conjugate pad was next removed (when sufficient serum samples have been transferred onto the paper platform strip), and excess BCIP/NBT substrate was immediately added upstream of the test spot. After 15 min of substrate addition, the strips were washed with 1× Tris-buffered saline, 0.1% Tween® 20. Finally, the strips were scanned using a scanner to obtain digital images for image analysis using ImageJ.
Results for the HBsAg paper-based ELISA (using RBCs filter membranes as conjugate pads and assembled upstream of the test spots) are shown in
Number | Date | Country | Kind |
---|---|---|---|
10201405360P | Aug 2014 | SG | national |
This application is a divisional of U.S. application Ser. No. 15/506,964, which is the U.S. National Phase of International Application No. PCT/SG2015/050291 filed Aug. 31, 2015, which in turn claims the priority benefit of priority of Singapore application number 10201405360P filed 30 Aug. 2014, the contents of all such applications being hereby incorporated by reference in their entirety for all purposes.
Number | Date | Country | |
---|---|---|---|
Parent | 15506964 | Feb 2017 | US |
Child | 17574169 | US |