WO2004050919A2 - Surface treatment - Google Patents

Surface treatment Download PDF

Info

Publication number
WO2004050919A2
WO2004050919A2 PCT/US2003/038752 US0338752W WO2004050919A2 WO 2004050919 A2 WO2004050919 A2 WO 2004050919A2 US 0338752 W US0338752 W US 0338752W WO 2004050919 A2 WO2004050919 A2 WO 2004050919A2
Authority
WO
WIPO (PCT)
Prior art keywords
functional group
monolayer
covalent bond
biomolecules
homobifunctional
Prior art date
Application number
PCT/US2003/038752
Other languages
French (fr)
Other versions
WO2004050919A3 (en
Inventor
Sergey Amontov
Bruno Michel
Sally Swanson
Heiko Wolf
Original Assignee
International Business Machines Corporation
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by International Business Machines Corporation filed Critical International Business Machines Corporation
Priority to JP2004557616A priority Critical patent/JP2006509201A/en
Priority to EP03812520A priority patent/EP1572352A2/en
Publication of WO2004050919A2 publication Critical patent/WO2004050919A2/en
Publication of WO2004050919A3 publication Critical patent/WO2004050919A3/en

Links

Classifications

    • BPERFORMING OPERATIONS; TRANSPORTING
    • B82NANOTECHNOLOGY
    • B82YSPECIFIC USES OR APPLICATIONS OF NANOSTRUCTURES; MEASUREMENT OR ANALYSIS OF NANOSTRUCTURES; MANUFACTURE OR TREATMENT OF NANOSTRUCTURES
    • B82Y30/00Nanotechnology for materials or surface science, e.g. nanocomposites
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/543Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals
    • G01N33/54353Immunoassay; Biospecific binding assay; Materials therefor with an insoluble carrier for immobilising immunochemicals with ligand attached to the carrier via a chemical coupling agent
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N2610/00Assays involving self-assembled monolayers [SAMs]

Definitions

  • the present invention generally relates to surface treatment and particularly relates to methods and apparatus for treating surfaces such as biosensor surfaces by molecular chemisorption.
  • Biosensor arrays typically involves patterned deposition of biomolecules onto a surface. Sensitivity, reproducibility, and selectivity are significant aspects of biosensor quality. Sensitivity is typically achieved via a dense layer of chemisorbed capture molecules to efficiently capture target molecules.
  • Reproducibility typically depends on highly reproducible anchoring chemistry and good quality patterning of capture molecules.
  • Selectivity typically depends on high selectivity of target molecules and low non-selective adsorption of other molecules.
  • the latter can limit utility of biosensors by accounting for 30% of the signal to be detected.
  • Bioconjugation involves linking molecules to form a complex having the combined properties of the individual components. Natural and synthetic compounds, and their activities, can be chemically combined to engineer substances having desired characteristics. For example, a protein bound to a target molecule in a complex mixture may be cross-linked with another molecule capable of being detected to form a traceable conjugate. The detection component provides visibility of the target component to produce a complex that can be localized, followed through various processes, or used for measurement.
  • Bioconjugation has affected many areas in the life sciences. Application of cross- linking reactions to creation of novel conjugates with particular activities has enabled the assay of minute quantities of substances for detection of cellular components and treatment of disease. The ability to chemically attach one molecule to another has produced a growing industry serving research, diagnostics, and therapeutic markets. A significant portion of biological assays is now performed using conjugates for interaction with specific analytes in solutions, cells, or tissues. An overview of conjugate molecules, reagent systems, and applications of bioconjugate techniques is given in G.T. Hermanson, "Bioconjugate Techniques", Academic Press, San Diego, 1996.
  • direct chemisorption or physisorption binds capture molecules 10 to the surface 20.
  • the surface 20 is functionalized with relatively short linker molecules 30.
  • the surface 20 may be amine-functionalized.
  • the linkers 30 immobilize the capture molecules 10 on the surface 20.
  • Unwanted molecules also present on the surface 20 can be typically removed by stringent washing to optimize selectivity of the biosensor. However, washing can remove physisorbed molecules. Chemisorbed molecules are more resistant to washing. Referring to Figure IB, this scheme leaves many linkers 30 exposed. This leads to much nonspecific chemisorption or physisorption of other molecules 40. This reduces the selectivity of the biosensor.
  • the ratio of molecules bound by specific interaction to molecules bound by nonspecific interaction is reduced.
  • the selectivity of the capture molecules 10 may be high in solution, many detection methods are convoluted by presence of other molecules 40. Additionally, direct physisorption or chemisorption of the capture molecules 10 limits molecular mobility. Few capture molecules 10 have full functionality. The sensitivity of the capture molecules 10 is thus reduced. Binding efficiency is usually reduced where the capture molecules 10 are for binding assays. The affinity constant and binding kinetics vary in dependence on the orientation of chemisorption. This results in less target molecules 70 such as antigens being bound to the surface 20. Also, there is higher binding variability between different surfaces. If the detection scheme employed cannot distinguish between the target molecules 70 and the other molecules 40, the effective specificity of the biosensor is significantly reduced.
  • the capture molecules 10 are chemisorbed to the surface 20 through spacer molecules 50. As indicated earlier, chemisorption of capture molecules 10 allows more stringent washing procedures, thus reducing nonspecifically physisorbed molecules.
  • the spacers 50 are longer than the linkers 30 herein before described with reference to Figure 1 A. The spacers 50 tether the capture molecules 10 to the surface 20. However, the spacers 50 also allow limited movement of the capture molecules 10 relative to the surface 20. This allows the capture molecules 10 increased activity. The mobility and thus functionality of capture molecules 10 is improved.
  • Binding efficiency of the capture molecules 10 chemisorbed through spacers 50 is thus increased.
  • the exposed surface 20 and the spacers 50 allow nonspecific binding of other molecules 40. Nonspecific binding can occur in roughly the same amount as in the Figure IB arrangement.
  • the capture molecules 20 anchored to the surface 20 through spacers 50 in a sea of biocompatible molecules 60.
  • the biocompatible molecules 60 are resistant to nonspecific adsorption of the other molecules 40. This improves the effective specificity of the surface 20.
  • nonspecific binding is reduced because the surface 20 is less exposed. Only the spacers 50 and the capture molecules 10 offer sites for nonspecific binding of other molecules 40. Stringent washing can improve specificity further by removing more nonspecifically bound molecules 40 than specifically bound molecules 10.
  • the susceptibility of biosensors to nonspecific adsorption also depends on labeling and detection schemes employed. For example, sandwich ELISA assays are less susceptible because the signal measured depends only on the number of target antigen molecules 10 and the specificity with which labeling antibodies bind to the surface 20. This approach is inert because it involves a dual selective detection. However, label- free detection schemes are more susceptible to other molecules 40 adsorbing nonspecifically to the surface 20. These schemes measure the protein/DNA present on the surface 20 by mass or refractive index. More control over nonspecific adsorption is needed than in sandwich ELISA biosensors. Control over nonspecific adsorption and nonspecific signal generation is also important where bound molecules are detected by chemical labeling techniques.
  • Such control is particularly desirable when chemical labeling exhibits cross-reactivity with chemical groups involved in the chemisorption.
  • a barrier can be added to prevent access to the groups.
  • BSA blocking of nonspecific adsorption is not usually possible because BSA produces a signal and reduces the "effective" selectivity of the biosensor.
  • Nucleic acid aptamers are useful for biosensor production because they can form three dimensional structures. Aptamers can also bind a range of target molecules with acceptable affinity and specificity. Also, aptamers can function in a similar manner to protein molecules. For example, aptamers can change in structure due to ligand- binding. There are many different receptors that are useful in biosensor arrays. However, aptamers are especially useful for several reasons. One reason is that aptamers can be more easily engineered than antibodies. Following selection, aptamers can be reduced to 30-60 nucleotide residue core sequences without reducing binding function. Another reason is that modifications such as fluorescent reporters can be easily introduced by chemical synthesis. Yet another reason is that aptamer structure is mainly a function of Watson-Crick base pairing. Secondary structural interactions allow aptamers to be more easily converted to receptors than antibodies.
  • capture molecules in the form of amine- functionalized aptamers 120 are crosslinked onto a glass surface 20.
  • the surface is first functionalized with APTS (3-aminopropyl triethoxysilane) 100.
  • APTS 3-aminopropyl triethoxysilane
  • the cross- linking is then performed by spacers in the form of bifunctional succinimide crosslinkers (BS3) 110.
  • BS3 bifunctional succinimide crosslinkers
  • the remaining crosslinking spacers 50 and amine surface 20 are blocked with a single functionalized succinimide to cover the amines, and ethanolamine to saturate unreacted succinimide groups. Any remaining surface areas may be treated with PEG.
  • These post-chemisorption steps reduce nonspecific protein absorption.
  • spaces between the capture molecules 10 and the spacers 50 can still react. These spaces accept nonspecific protein adsorption.
  • BS3 spacers are too short for many proteins and pose problems as herein before described with reference to Figure 1 A.
  • the functionalizing, cross-linking, and blocking steps each involve exposure of the surface 20 to a different environment in a different bath. This process is laborious, time consuming, and wasteful of raw materials.
  • biosensor fabrication that: irreversibly attaches capture molecules to the biosensor surface; provides sufficient mobility and accessibility for capture molecules to remain functional; and, minimizes nonspecific adsorption of target antigens or other molecules. It would also be desirable to provide a method for fabricating biosensors which is less laborious, less time consuming, and less wasteful of materials.
  • a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
  • biomolecules refers to molecules having biological functionality.
  • the biomolecules may be amine-functionalised.
  • the biomolecules may comprise a nucleic acid aptamer derivative.
  • an excess of the homobifunctional polymer is involved.
  • the heterobifunctional reagent is preferably mixed with the homobifunctional polymer prior to exposure to the surface.
  • the surface may be glass, metal, or the like.
  • the heterobifunctional reagent is preferably an aminoalkyl trialkoxysilane.
  • the heterobifunctional reagent is 3-aminopropyl triethoxysilane.
  • the heterobifunctional reagent may be an alkylthiol.
  • the second functional group of the heterobifunctional reagent preferably reacts with one functional group of the homobifunctional polymer to form a covalent bond therebetween.
  • the functional groups of the homobifunctionl polymer are N-hydroxy succinimide groups.
  • the homobifunctional polymer may be a homobifunctional polyethylene glycol.
  • the biomolecules may react with one functional group of the homobifunctional polymer to form a covalent bond therebetween.
  • the covalent bonds formed between the biomolecules and the homobifunctional polymer is preferably an amide bond.
  • a biosensor having a surface layer formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules.
  • a biosensor array comprising a patterned deposit of biomolecules on a substrate wherein the patterned deposit is formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules.
  • a biochip having a surface layer formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
  • a biochip array comprising a patterned deposit of biomolecules on a substrate wherein the patterned deposit is formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
  • a simple two step chemical process for attaching capture molecules to a biosensor surface employs a homobifunctional PEG crosslinker with succinimide groups at each end to chemisorb the capture molecules onto the surface with higher density and reproducibility than hitherto possible.
  • the process improves the sensitivity and selectivity of bioassays. Also provided are protocols and devices for treating biosensor surfaces economically with high yield.
  • a method for attaching a spacer molecule to a clean glass surface involves a non-symmetrical reaction of a heterobifunctional reagent such as 3-aminopropyl triethoxysilane (APTS) with a homobifunctional polymer such as homobifunctional succinimide end functionalized PEG polymer.
  • APTS 3-aminopropyl triethoxysilane
  • the reaction is carried out in a water free solvent.
  • a high concentration is employed to favor bimolecular reactions.
  • the present invention also extends a device for applying a small amount of prereacted reagent to glass surfaces in the interests of saving expensive reagents.
  • Figure 1 A is a cross sectional view of a biosensor surface showing direct adsorption of capture molecules on a surface
  • Figure IB is a cross sectional view of the surface showing nonspecific chemisorption of other molecules to the arrangement shown in Figure 1 A;
  • Figure IC is a cross sectional view of the surface showing chemisorption of capture molecules via spacer molecules
  • Figure ID is a cross sectional view of the surface showing nonspecific chemisorption of other molecules to the arrangement shown in Figure 1 C;
  • Figure IE is a cross sectional view of the surface showing capture molecules anchored to a surface via spacer molecules in a sea of biocompatible molecules;
  • Figure IF is a cross sectional view of the surface showing nonspecific chemisorption of other molecules to the arrangement shown in Figure IE;
  • Figure 1G is a cross sectional view of a preferred embodiment of the present invention in which capture molecules are anchored to a surface through combined anchor/spacers;
  • Figure 1H is a cross sectional view showing nonspecific chemisorption of other molecules to the arrangement shown in Figure 1G;
  • Figure 2A is a flow diagram showing attachment of an amine-functionalized aptamer to an APTS (3-aminopropyl triethoxysilane) functionalized glass surface via a bifunctional succinimide crosslinker (BS3);
  • APTS 3-aminopropyl triethoxysilane
  • Figure 2B is a flow diagram showing attachment of an amine-functionalized aptamer to a glass surface where the surface is treated with a preprocessed solution of APTS (aminpropyltrimethoxysilane) and a homobifunctional PEG N-hydroxy succinimide crosslinker (NHS) in DMSO;
  • APTS aminopropyltrimethoxysilane
  • NHS homobifunctional PEG N-hydroxy succinimide crosslinker
  • Figure 2C shows a reaction of APTS (aminopropyl trimethoxysilane) to one end of a homobifunctional PEG N-hydroxy succinimide crosslinker (NHS) in DMSO;
  • APTS aminopropyl trimethoxysilane
  • Figure 3 is an NMR spectrum showing reaction of aminopropyl triethoxysilane with NHS PEG
  • Figure 4A is a plan view of a fluid cell for treating biosensor surfaces
  • Figure 4B is a side view of the fluid cell
  • Figure 4C is another plan view of the cell
  • Figure 5 A is a photographic image of a treated surface
  • Figure 5B is a plot of fluorescence versus data point corresponding to the surface of Figure 5A;
  • Figure 5C is a photographic image of another treated surface.
  • Figure 5D is a plot of fluorescence versus data point corresponding to the surface of Figure 5B; DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT
  • a biosensor in which capture molecules 10 are anchored to a glass biosensor surface 20 via combined anchor/spacers acting as biocompatibility molecules 80.
  • the biocompatiblity molecules 80 are resistant to the nonspecific adsorption of other molecules 40 and also act as crosslinkers. This further reduces potential nonspecific adsorption sites.
  • surplus biocompatibility molecules 80 provide lateral spacing of capture molecules 40 without leaving the underlying surface 20 exposed.
  • the concentration of capture molecules 10 applied determines the density of surface activation.
  • target molecules 70 are bound to the surface 20 via the capture molecules 80.
  • the glass surface 20 is treated with a preprocessed solution of APTS (aminopropyl trimethoxysilane) 200 and a homobifunctional PEG N-hydroxy succinimide crosslinker (NHS) 210 in dimethyl sulphoxide (DMSO).
  • APTS aminopropyl trimethoxysilane
  • NHS homobifunctional PEG N-hydroxy succinimide crosslinker
  • DMSO dimethyl sulphoxide
  • the NHS crosslinker 210 has two NHS functions; one at each end. At one end, the first NHS function binds to the APTS 200. At the other end, the second NHS function binds to an amine-functionalized aptamer 220. In both case, the binding is via covalent bonds.
  • Figure 3 shows an NMR spectrum illustrating the reaction of the APTS 200 with the NHS PEG 210. The molecule shown is the result of that reaction.
  • the reaction referred to in connection with Figure 3 starts with preparation of a heterobifunctional reagent in the form of NHS-PEG-triethoxysilane from APTS and a homobifunctional PEG in the form of (a,w)NHS-PEG 2000, Rapp Polymere in a solution of DMSO at 42-48 degrees C.
  • 300 microliters of 80 mM homobifunctional NHS-PEG in DMSO is mixed with 200 microliters of 120 M APTS in DMSO, 6 microliters APTS in 300 microliters DMSO. This produces an equimolar mixture with both substances having a concentration of 48 mM.
  • the mixture is heated to between 46 and 50 degrees C and allowed to react for between 30 and 60 minutes.
  • the result is then transferred to a narrow gap between two pretreated glass surfaces for between 60 and 120 minutes.
  • Capillary action is employed to promote ingress of the mixture into the gap until the gap is filled. Filling the gap at elevated temperature is desirable. Otherwise, the viscosity of the mixture is too high.
  • the surfaces were pretreated by a mixture of 1 part concentrated sulfuric (Fluka) acid and 2 parts hydrogen peroxide (Fluka puriss) for several hours and then washed in deionized water.
  • the mixture of sulfuric acid and hydrogen peroxide sometimes called 'piranha solution', heats to boiling point during mixing.
  • NMR performed after 30 minutes shows that over 90% amine groups react with the NHS groups on the PEG and that no free APTS can be detected with a detection threshold of 10%.
  • Homobifunctional side products of unreacted NHS-PEG and homobifunctional triethoxysilane PEG form statistically. However, these do not disturb chemisorption. This is because NHS-PEG cannot chemisorb to glass.
  • Homobifunctional triethoxysilane PEG may only dilute the density of the NHS-PEG and will decay to Si-(OH)3 in the subsequent protein adsorption step.
  • Figures 4A to C show a fluid cell for treating glass surfaces 20 with a high concentration of a relatively expensive linker/spacer biocompatibility molecule such as that herein before described.
  • the surfaces 20 are separated and sealed by a 100-300 micrometers thick peripheral gasket 300.
  • the gasket 300 may be formed from Teflon.
  • the fluid cell is then filled with the reactive mixture by capillary force from one side with a volume of 150 microliters. Specifically, the mixture is drawn into the gap intervening between the surfaces 20 and defined by the gasket 300 via capillary action. The surfaces 20 are thus treated.
  • the technique herein before described is superior to conventional techniques because the heterobifunctional reagent is prepared in situ.
  • Non-aqueous conditions prevent polymerization of APTS and facilitate regular treatment of the surfaces 20.
  • In-situ preparation of the reagent provides a fresh reactive intermediate which is not degraded or polymerized due to storage.
  • the high concentration in the mixture of 50 mM PEG and APTS improves bimolecular reaction speed. This allows preparation of the reagent without unwanted decay.
  • a higher concentration of NHS over APTS helps to drive the reaction of APTS with NHS groups to completion.
  • the capillary gap increases the speed of surface reaction by eliminating diffusion limitation. Because there are substantially no gradients in the mixture, treatment of the surfaces 20 is more homogeneous.
  • Reaction of the reagent between the surfaces 20 is stopped by removal of the solution by filter paper followed by three wash cycles with DMSO. Washing removes unreacted heterobifunctional molecules together with polymerization products and homobifuctional byproducts.
  • the surfaces 20 are then disassembled and blow dried with nitrogen to remove traces of DMSO. Capture molecules 10 are then attached to the freshly NHS-activated surfaces 20. Alternatively, the surfaces 20 may be stored for a few days in dry argon.
  • Treated glass surfaces 20 as herein before described can anchor oligonucleotides with terminal aminogroups (5' or 3' end), proteins, and other NH2-functionalized molecules.
  • chemisorption is performed by filling a PDMS microfluidic network applied to the NHS-activated surface 20 with aqueous solutions of amino-functionalized compounds.
  • a concentration of 20 M oligonucleotide provides particularly homogeneous coverage of the surface 20 by oligonucleotides during chemical reaction and remains substantially unaffected by drying.
  • Figures 5 A to 5D exemplify improved homogeneity achievable using surface functionalization embodying the present invention.
  • Figure 5 A shows a fluorescence image of patterned TAMRA labelled 18-mer DNA oligomer molecules chemisorbed to the surface by an NHS-PEG- APTS conjugate spacer. The lighter stripes show the chemisorbed oligomer molecules.
  • Figure 5B is a plot of fluorescence counts from the Figure 5A surface showing an intraspot standard deviation ⁇ 2% and an interspot standard deviation ⁇ 4%. The fluorescence intensity averaged over 45 separate areas distributed over the image in this case is 9748+- 350 counts. The variability is less than 4%. For one area, 600 pixels were averaged. The accuracy of patterning remains stable even during washing and hybridization cycles.

Abstract

Described is a process for producing a biomolecular monolayer on a biosensor surface comprising the steps of: reacting a biosensor surface with a solution of heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to the biosensor surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules.

Description

SURFACE TREATMENT
BACKGROUND OF THE INVENTION Field of the Invention
The present invention generally relates to surface treatment and particularly relates to methods and apparatus for treating surfaces such as biosensor surfaces by molecular chemisorption.
Discussion of Related Art
Production of biosensor arrays typically involves patterned deposition of biomolecules onto a surface. Sensitivity, reproducibility, and selectivity are significant aspects of biosensor quality. Sensitivity is typically achieved via a dense layer of chemisorbed capture molecules to efficiently capture target molecules.
Reproducibility typically depends on highly reproducible anchoring chemistry and good quality patterning of capture molecules. Selectivity typically depends on high selectivity of target molecules and low non-selective adsorption of other molecules.
The latter can limit utility of biosensors by accounting for 30% of the signal to be detected.
Bioconjugation involves linking molecules to form a complex having the combined properties of the individual components. Natural and synthetic compounds, and their activities, can be chemically combined to engineer substances having desired characteristics. For example, a protein bound to a target molecule in a complex mixture may be cross-linked with another molecule capable of being detected to form a traceable conjugate. The detection component provides visibility of the target component to produce a complex that can be localized, followed through various processes, or used for measurement.
Bioconjugation has affected many areas in the life sciences. Application of cross- linking reactions to creation of novel conjugates with particular activities has enabled the assay of minute quantities of substances for detection of cellular components and treatment of disease. The ability to chemically attach one molecule to another has produced a growing industry serving research, diagnostics, and therapeutic markets. A significant portion of biological assays is now performed using conjugates for interaction with specific analytes in solutions, cells, or tissues. An overview of conjugate molecules, reagent systems, and applications of bioconjugate techniques is given in G.T. Hermanson, "Bioconjugate Techniques", Academic Press, San Diego, 1996.
Surfaces for use in biological environments are found in tools for molecular and cell biology such as substrates for Enzyme Linked Inmmunosorbent Assay (ELISA) in cell cultures, contact lenses, implanted prostheses, catheters, and containers for storage of proteins. Many such surfaces are quickly coated with a layer of proteins via spontaneous adsorption. Some have a beneficial effect. Others are detrimental. There is much interest in identifying biologically "inert" materials for resisting adsorption of proteins. A conventional surface treatment method for introducing such resistance involves coating the surface with poly(ethylene glycol) (PEG). See, for example J.M. Harris ed. Poly(ethylene glycol) Chemistry: Biotechnical and Biomedical Applications, Plenum, New York, 1992. Further details of PEG are provided in Gombotz, W.R. et al., J. Biomed. Matter. Res. 15, 1547-1562 (1991). An alternative approach involves the pre-adsorption of bovine serum albumin. This approach however suffers from denaturation of the protein over time or exchange of the protein with other molecules. Therefore, this approach is unsuitable for application to biosensors for detecting presence of proteins by mass or primary amines. Self- assembled monolayers of short chain PEG oligomers (n=2-7) have also been shown to resist adsorption of proteins. See, for example Mrksich, M. and Whitesides, G.M., Annu. Rev. Biophys. Biomol. Struct. 25, 55-78 (1996). However, a protein attempting to adsorb may compress and desolvate PEG. These effects are both energetically disadvantageous. See, for example Jeon, S.I. and Andrade, J.D. "Protein surface interactions in the presence of polyethylene oxide: effect of protein size", J. Coll. Interface Sci. 142, 159-166 (1991); and, Jeon, S.I., Lee, J.H., Adrade, J.D. and de Gennes, P.G., "Protein surface interactions in the presence of polyethyleneoxide: simplified theory", J. Coll. Interface Sci. 142, 149-158 (1991)). Biosensor surfaces are typically formed from borosilicate glass. Various conventional schemes for attaching capture molecules, such as antibodies or DNA oligomers, to a biosensor surface will now be described.
Referring to Figure 1 A, in one conventional scheme, direct chemisorption or physisorption binds capture molecules 10 to the surface 20. The surface 20 is functionalized with relatively short linker molecules 30. For example, the surface 20 may be amine-functionalized. The linkers 30 immobilize the capture molecules 10 on the surface 20. Unwanted molecules also present on the surface 20 can be typically removed by stringent washing to optimize selectivity of the biosensor. However, washing can remove physisorbed molecules. Chemisorbed molecules are more resistant to washing. Referring to Figure IB, this scheme leaves many linkers 30 exposed. This leads to much nonspecific chemisorption or physisorption of other molecules 40. This reduces the selectivity of the biosensor. The ratio of molecules bound by specific interaction to molecules bound by nonspecific interaction is reduced. Although the selectivity of the capture molecules 10 may be high in solution, many detection methods are convoluted by presence of other molecules 40. Additionally, direct physisorption or chemisorption of the capture molecules 10 limits molecular mobility. Few capture molecules 10 have full functionality. The sensitivity of the capture molecules 10 is thus reduced. Binding efficiency is usually reduced where the capture molecules 10 are for binding assays. The affinity constant and binding kinetics vary in dependence on the orientation of chemisorption. This results in less target molecules 70 such as antigens being bound to the surface 20. Also, there is higher binding variability between different surfaces. If the detection scheme employed cannot distinguish between the target molecules 70 and the other molecules 40, the effective specificity of the biosensor is significantly reduced. This is common in both label free and labelled detection schemes. Stringent washing does not usually correct this problem because cooperative effects during nonspecific binding are virtually irreversible. Referring to Figure IC, in another conventional scheme, the capture molecules 10 are chemisorbed to the surface 20 through spacer molecules 50. As indicated earlier, chemisorption of capture molecules 10 allows more stringent washing procedures, thus reducing nonspecifically physisorbed molecules. The spacers 50 are longer than the linkers 30 herein before described with reference to Figure 1 A. The spacers 50 tether the capture molecules 10 to the surface 20. However, the spacers 50 also allow limited movement of the capture molecules 10 relative to the surface 20. This allows the capture molecules 10 increased activity. The mobility and thus functionality of capture molecules 10 is improved. Binding efficiency of the capture molecules 10 chemisorbed through spacers 50 is thus increased. However, referring to Figure ID, the exposed surface 20 and the spacers 50 allow nonspecific binding of other molecules 40. Nonspecific binding can occur in roughly the same amount as in the Figure IB arrangement.
Referring to Figure IE, in a modification of the Figure IC scheme, the capture molecules 20 anchored to the surface 20 through spacers 50 in a sea of biocompatible molecules 60. The biocompatible molecules 60 are resistant to nonspecific adsorption of the other molecules 40. This improves the effective specificity of the surface 20. Referring to Figure IF, nonspecific binding is reduced because the surface 20 is less exposed. Only the spacers 50 and the capture molecules 10 offer sites for nonspecific binding of other molecules 40. Stringent washing can improve specificity further by removing more nonspecifically bound molecules 40 than specifically bound molecules 10.
The susceptibility of biosensors to nonspecific adsorption also depends on labeling and detection schemes employed. For example, sandwich ELISA assays are less susceptible because the signal measured depends only on the number of target antigen molecules 10 and the specificity with which labeling antibodies bind to the surface 20. This approach is inert because it involves a dual selective detection. However, label- free detection schemes are more susceptible to other molecules 40 adsorbing nonspecifically to the surface 20. These schemes measure the protein/DNA present on the surface 20 by mass or refractive index. More control over nonspecific adsorption is needed than in sandwich ELISA biosensors. Control over nonspecific adsorption and nonspecific signal generation is also important where bound molecules are detected by chemical labeling techniques. Such control is particularly desirable when chemical labeling exhibits cross-reactivity with chemical groups involved in the chemisorption. A barrier can be added to prevent access to the groups. However, BSA blocking of nonspecific adsorption is not usually possible because BSA produces a signal and reduces the "effective" selectivity of the biosensor.
Nucleic acid aptamers are useful for biosensor production because they can form three dimensional structures. Aptamers can also bind a range of target molecules with acceptable affinity and specificity. Also, aptamers can function in a similar manner to protein molecules. For example, aptamers can change in structure due to ligand- binding. There are many different receptors that are useful in biosensor arrays. However, aptamers are especially useful for several reasons. One reason is that aptamers can be more easily engineered than antibodies. Following selection, aptamers can be reduced to 30-60 nucleotide residue core sequences without reducing binding function. Another reason is that modifications such as fluorescent reporters can be easily introduced by chemical synthesis. Yet another reason is that aptamer structure is mainly a function of Watson-Crick base pairing. Secondary structural interactions allow aptamers to be more easily converted to receptors than antibodies.
Referring to Figure 2A, in a conventional process for producing a biosensor as herein before described with reference to Figure IF, capture molecules in the form of amine- functionalized aptamers 120 are crosslinked onto a glass surface 20. The surface is first functionalized with APTS (3-aminopropyl triethoxysilane) 100. The cross- linking is then performed by spacers in the form of bifunctional succinimide crosslinkers (BS3) 110.
Following such chemisorption of capture molecules 10, the remaining crosslinking spacers 50 and amine surface 20 are blocked with a single functionalized succinimide to cover the amines, and ethanolamine to saturate unreacted succinimide groups. Any remaining surface areas may be treated with PEG. These post-chemisorption steps reduce nonspecific protein absorption. However, as herein before indicated, spaces between the capture molecules 10 and the spacers 50 can still react. These spaces accept nonspecific protein adsorption. BS3 spacers are too short for many proteins and pose problems as herein before described with reference to Figure 1 A. In addition, the functionalizing, cross-linking, and blocking steps each involve exposure of the surface 20 to a different environment in a different bath. This process is laborious, time consuming, and wasteful of raw materials.
It would be desirable to provide a method for effecting chemisorption of capture molecules with improved activity, accessibility, capacity, and specificity of the capture molecules. In particular, it would be desirable to provide a method for biosensor fabrication that: irreversibly attaches capture molecules to the biosensor surface; provides sufficient mobility and accessibility for capture molecules to remain functional; and, minimizes nonspecific adsorption of target antigens or other molecules. It would also be desirable to provide a method for fabricating biosensors which is less laborious, less time consuming, and less wasteful of materials.
SUMMARY OF THE INVENTION In accordance with the present invention, there is now provided a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
The term biomolecules, as used herein, refers to molecules having biological functionality. For example, the biomolecules may be amine-functionalised. Equally, the biomolecules may comprise a nucleic acid aptamer derivative. Preferably, an excess of the homobifunctional polymer is involved. The heterobifunctional reagent is preferably mixed with the homobifunctional polymer prior to exposure to the surface. The surface may be glass, metal, or the like. The heterobifunctional reagent is preferably an aminoalkyl trialkoxysilane. In a preferred embodiment of the present invention, the heterobifunctional reagent is 3-aminopropyl triethoxysilane. However, the heterobifunctional reagent may be an alkylthiol. The second functional group of the heterobifunctional reagent preferably reacts with one functional group of the homobifunctional polymer to form a covalent bond therebetween. In a preferred embodiment of the present invention, the functional groups of the homobifunctionl polymer are N-hydroxy succinimide groups. The homobifunctional polymer may be a homobifunctional polyethylene glycol. The biomolecules may react with one functional group of the homobifunctional polymer to form a covalent bond therebetween. The covalent bonds formed between the biomolecules and the homobifunctional polymer is preferably an amide bond.
Viewing the present invention from another aspect, there is now provided a biosensor having a surface layer formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules.
Viewing the present invention from yet another aspect, there is now provided a biosensor array comprising a patterned deposit of biomolecules on a substrate wherein the patterned deposit is formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules. Viewing the present invention from a further aspect, there is now provided a biochip having a surface layer formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
Viewing the present invention from still a further aspect, there is now provided a biochip array comprising a patterned deposit of biomolecules on a substrate wherein the patterned deposit is formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
In a preferred embodiment of the present invention, there is provided a simple two step chemical process for attaching capture molecules to a biosensor surface. The process employs a homobifunctional PEG crosslinker with succinimide groups at each end to chemisorb the capture molecules onto the surface with higher density and reproducibility than hitherto possible. The process improves the sensitivity and selectivity of bioassays. Also provided are protocols and devices for treating biosensor surfaces economically with high yield.
In a particularly preferred embodiment of the present invention, there is provided a method for attaching a spacer molecule to a clean glass surface. The method involves a non-symmetrical reaction of a heterobifunctional reagent such as 3-aminopropyl triethoxysilane (APTS) with a homobifunctional polymer such as homobifunctional succinimide end functionalized PEG polymer. The reaction is carried out in a water free solvent. A high concentration is employed to favor bimolecular reactions. The present invention also extends a device for applying a small amount of prereacted reagent to glass surfaces in the interests of saving expensive reagents.
BRIEF DESCRIPTION OF THE DRAWINGS
Preferred embodiments of the present invention will now be described, by way of example only, with reference to the accompanying drawings, in which:
Figure 1 A is a cross sectional view of a biosensor surface showing direct adsorption of capture molecules on a surface;
Figure IB is a cross sectional view of the surface showing nonspecific chemisorption of other molecules to the arrangement shown in Figure 1 A;
Figure IC is a cross sectional view of the surface showing chemisorption of capture molecules via spacer molecules;
Figure ID is a cross sectional view of the surface showing nonspecific chemisorption of other molecules to the arrangement shown in Figure 1 C;
Figure IE is a cross sectional view of the surface showing capture molecules anchored to a surface via spacer molecules in a sea of biocompatible molecules;
Figure IF is a cross sectional view of the surface showing nonspecific chemisorption of other molecules to the arrangement shown in Figure IE;
Figure 1G is a cross sectional view of a preferred embodiment of the present invention in which capture molecules are anchored to a surface through combined anchor/spacers;
Figure 1H is a cross sectional view showing nonspecific chemisorption of other molecules to the arrangement shown in Figure 1G; Figure 2A is a flow diagram showing attachment of an amine-functionalized aptamer to an APTS (3-aminopropyl triethoxysilane) functionalized glass surface via a bifunctional succinimide crosslinker (BS3);
Figure 2B is a flow diagram showing attachment of an amine-functionalized aptamer to a glass surface where the surface is treated with a preprocessed solution of APTS (aminpropyltrimethoxysilane) and a homobifunctional PEG N-hydroxy succinimide crosslinker (NHS) in DMSO;
Figure 2C shows a reaction of APTS (aminopropyl trimethoxysilane) to one end of a homobifunctional PEG N-hydroxy succinimide crosslinker (NHS) in DMSO;
Figure 3 is an NMR spectrum showing reaction of aminopropyl triethoxysilane with NHS PEG;
Figure 4A is a plan view of a fluid cell for treating biosensor surfaces;
Figure 4B is a side view of the fluid cell;
Figure 4C is another plan view of the cell;
Figure 5 A is a photographic image of a treated surface;
Figure 5B is a plot of fluorescence versus data point corresponding to the surface of Figure 5A;
Figure 5C is a photographic image of another treated surface; and,
Figure 5D is a plot of fluorescence versus data point corresponding to the surface of Figure 5B; DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENT
With reference to Figure 1G, in a preferred embodiment of the present invention, there is provided a biosensor in which capture molecules 10 are anchored to a glass biosensor surface 20 via combined anchor/spacers acting as biocompatibility molecules 80.
Referring now to Figure 1H, the biocompatiblity molecules 80 are resistant to the nonspecific adsorption of other molecules 40 and also act as crosslinkers. This further reduces potential nonspecific adsorption sites. Advantageously, surplus biocompatibility molecules 80 provide lateral spacing of capture molecules 40 without leaving the underlying surface 20 exposed. The concentration of capture molecules 10 applied determines the density of surface activation. In operation, target molecules 70 are bound to the surface 20 via the capture molecules 80.
Referring to Figure 2B and 2C in combination, in a particularly preferred embodiment of the present invention, the glass surface 20 is treated with a preprocessed solution of APTS (aminopropyl trimethoxysilane) 200 and a homobifunctional PEG N-hydroxy succinimide crosslinker (NHS) 210 in dimethyl sulphoxide (DMSO). The NHS crosslinker 210 has two NHS functions; one at each end. At one end, the first NHS function binds to the APTS 200. At the other end, the second NHS function binds to an amine-functionalized aptamer 220. In both case, the binding is via covalent bonds.
Figure 3 shows an NMR spectrum illustrating the reaction of the APTS 200 with the NHS PEG 210. The molecule shown is the result of that reaction.
In a particularly preferred process embodying the present invention, the reaction referred to in connection with Figure 3 starts with preparation of a heterobifunctional reagent in the form of NHS-PEG-triethoxysilane from APTS and a homobifunctional PEG in the form of (a,w)NHS-PEG 2000, Rapp Polymere in a solution of DMSO at 42-48 degrees C. 300 microliters of 80 mM homobifunctional NHS-PEG in DMSO is mixed with 200 microliters of 120 M APTS in DMSO, 6 microliters APTS in 300 microliters DMSO. This produces an equimolar mixture with both substances having a concentration of 48 mM. The mixture is heated to between 46 and 50 degrees C and allowed to react for between 30 and 60 minutes. The result is then transferred to a narrow gap between two pretreated glass surfaces for between 60 and 120 minutes. Capillary action is employed to promote ingress of the mixture into the gap until the gap is filled. Filling the gap at elevated temperature is desirable. Otherwise, the viscosity of the mixture is too high. The surfaces were pretreated by a mixture of 1 part concentrated sulfuric (Fluka) acid and 2 parts hydrogen peroxide (Fluka puriss) for several hours and then washed in deionized water. The mixture of sulfuric acid and hydrogen peroxide, sometimes called 'piranha solution', heats to boiling point during mixing.
Remaining with Figure 3, NMR performed after 30 minutes shows that over 90% amine groups react with the NHS groups on the PEG and that no free APTS can be detected with a detection threshold of 10%. Homobifunctional side products of unreacted NHS-PEG and homobifunctional triethoxysilane PEG form statistically. However, these do not disturb chemisorption. This is because NHS-PEG cannot chemisorb to glass. Homobifunctional triethoxysilane PEG may only dilute the density of the NHS-PEG and will decay to Si-(OH)3 in the subsequent protein adsorption step.
Figures 4A to C show a fluid cell for treating glass surfaces 20 with a high concentration of a relatively expensive linker/spacer biocompatibility molecule such as that herein before described. Referring to Figures 4A and 4B, the surfaces 20 are separated and sealed by a 100-300 micrometers thick peripheral gasket 300. The gasket 300 may be formed from Teflon. Referring to Figure 4C, the fluid cell is then filled with the reactive mixture by capillary force from one side with a volume of 150 microliters. Specifically, the mixture is drawn into the gap intervening between the surfaces 20 and defined by the gasket 300 via capillary action. The surfaces 20 are thus treated. The technique herein before described is superior to conventional techniques because the heterobifunctional reagent is prepared in situ. No further purification is needed. This is especially advantageous because purification of silanized PEG by conventional techniques such as chromatography is very difficult if not impossible. Non-aqueous conditions prevent polymerization of APTS and facilitate regular treatment of the surfaces 20. In-situ preparation of the reagent provides a fresh reactive intermediate which is not degraded or polymerized due to storage. The high concentration in the mixture of 50 mM PEG and APTS improves bimolecular reaction speed. This allows preparation of the reagent without unwanted decay. A higher concentration of NHS over APTS helps to drive the reaction of APTS with NHS groups to completion. The capillary gap increases the speed of surface reaction by eliminating diffusion limitation. Because there are substantially no gradients in the mixture, treatment of the surfaces 20 is more homogeneous. The larger the surface to volume ratio between the surfaces 20, the more polymerization reactions are reduced and reaction of triethoxysilane with the surfaces 20 is favored. These may otherwise reduce the specificity of detection schemes such as detection of primary amines through CBQCA or NHS-rhodamine. A low level of APTS present in the mixture significantly reduces the background level against which primary amines are detected.
Reaction of the reagent between the surfaces 20 is stopped by removal of the solution by filter paper followed by three wash cycles with DMSO. Washing removes unreacted heterobifunctional molecules together with polymerization products and homobifuctional byproducts. The surfaces 20 are then disassembled and blow dried with nitrogen to remove traces of DMSO. Capture molecules 10 are then attached to the freshly NHS-activated surfaces 20. Alternatively, the surfaces 20 may be stored for a few days in dry argon.
Treated glass surfaces 20 as herein before described can anchor oligonucleotides with terminal aminogroups (5' or 3' end), proteins, and other NH2-functionalized molecules. In a particularly preferred embodiment of the present invention, chemisorption is performed by filling a PDMS microfluidic network applied to the NHS-activated surface 20 with aqueous solutions of amino-functionalized compounds. Oligonucleotides are chemisorbed to the surface 20 in an aqueous solution containing 10% DMSO and 15-20% PEG (MW=1000). A concentration of 20 M oligonucleotide provides particularly homogeneous coverage of the surface 20 by oligonucleotides during chemical reaction and remains substantially unaffected by drying.
Figures 5 A to 5D exemplify improved homogeneity achievable using surface functionalization embodying the present invention. Figure 5 A shows a fluorescence image of patterned TAMRA labelled 18-mer DNA oligomer molecules chemisorbed to the surface by an NHS-PEG- APTS conjugate spacer. The lighter stripes show the chemisorbed oligomer molecules. Figure 5B is a plot of fluorescence counts from the Figure 5A surface showing an intraspot standard deviation <2% and an interspot standard deviation <4%. The fluorescence intensity averaged over 45 separate areas distributed over the image in this case is 9748+- 350 counts. The variability is less than 4%. For one area, 600 pixels were averaged. The accuracy of patterning remains stable even during washing and hybridization cycles.
Referring to Figures 5C and 5D, this is demonstrated by the image and graph therein. The lighter square areas are created by patterned chemisorption of aptamers along vertical tracks and by patterned hybridization of labelled 16-mer oligomer primers along spaced horizontal tracks. The fluorescence image averaged over 9 areas is 21539+- 1085 counts. The variability is 5%. For one area, 784 pixels were averaged.
Preferred embodiments of the present invention have been described herein by way of example only. It will be appreciated by those skilled in the art that there are many more embodiments of the present invention possible.

Claims

1. A process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of foπning a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
2. A process as claimed in claim 1, wherein the biomolecules are amine functionalised.
3. A process as claimed in claim 1, wherein the biomolecules comprise a nucleic acid aptamer derivative.
4. A process as claimed in claim 1, further comprising an excess of the homobifunctional polymer.
5. A process as claimed in claim 1, wherein the heterobifunctional reagent is mixed with the homobifunctional polymer prior to exposure to the surface.
6. A process as claimed in claim 1, wherein the surface is a glass surface.
7. A process as claimed in claim 1 wherein the surface is a metal surface.
8. A process as claimed in claim 1, wherein the heterobifunctional reagent is an aminoalkyl trialkoxysilane.
9. A process as claimed in claim 8, wherein the wherein the heterobifunctional reagent is 3-aminopropyl triethoxysilane.
10. A process as claimed in claim 1, wherein the heterobifunctional reagent is an alkylthiol.
11. A process as claimed in claim 1 wherein the second functional group of the heterobifunctional reagent reacts with one functional group of the homobifunctional polymer to form the covalent bond therebetween.
12. A process as claimed in claim 11 wherein the functional groups of the homobifunctional polymer are N-hydroxy succinimide groups.
13. A process as claimed in claim 1, wherein the homobifunctional polymer is a homobifunctional polyethylene glycol.
14. A process as claimed in claim 1, wherein the biomolecules react with one functional group of the homobifunctional polymer to form a covalent bond therebetween.
15. A process as claimed in claim 14, wherein the covalent bond formed between the biomolecules and the homobifunctional polymer is an amide bond.
16. A biosensor having a surface layer formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules.
17. A biosensor array comprising a patterned deposit of biomolecules on a substrate wherein the patterned deposit is formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with capture molecules.
18. A biochip having a surface layer formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
19. A biochip array comprising a patterned deposit of biomolecules on a substrate wherein the patterned deposit is formed by a process for producing a biomolecular monolayer on a surface comprising the steps of: reacting the surface with a solution of a heterobifunctional reagent having a first functional group and a second functional group, the first functional group being capable of forming a covalent bond to surface groups, the second functional group forming a covalent bond with a homobifunctional polymer to obtain a self-assembled monolayer, and thereafter reacting the monolayer with biomolecules.
PCT/US2003/038752 2002-12-04 2003-12-04 Surface treatment WO2004050919A2 (en)

Priority Applications (2)

Application Number Priority Date Filing Date Title
JP2004557616A JP2006509201A (en) 2002-12-04 2003-12-04 Surface treatment method
EP03812520A EP1572352A2 (en) 2002-12-04 2003-12-04 Surface treatment

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
US10/309,674 2002-12-04
US10/309,674 US7070922B2 (en) 2002-12-04 2002-12-04 Surface treatment

Publications (2)

Publication Number Publication Date
WO2004050919A2 true WO2004050919A2 (en) 2004-06-17
WO2004050919A3 WO2004050919A3 (en) 2004-08-26

Family

ID=32467904

Family Applications (1)

Application Number Title Priority Date Filing Date
PCT/US2003/038752 WO2004050919A2 (en) 2002-12-04 2003-12-04 Surface treatment

Country Status (7)

Country Link
US (2) US7070922B2 (en)
EP (1) EP1572352A2 (en)
JP (1) JP2006509201A (en)
KR (1) KR100694930B1 (en)
CN (1) CN1720096A (en)
TW (1) TWI277653B (en)
WO (1) WO2004050919A2 (en)

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
DE112010001382B4 (en) * 2009-03-27 2013-11-21 Hitachi High-Technologies Corporation Automatic analyzer pipetting nozzle, process for its manufacture and auto-analyzer using it

Families Citing this family (24)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
KR100682919B1 (en) * 2005-01-20 2007-02-15 삼성전자주식회사 Pattern forming method of fine metal thin layer, biomolecular fixing substrate and biochip using the same
WO2007089464A2 (en) * 2006-01-20 2007-08-09 The Regents Of The University Of California Self assembled monolayer surface patterning using a molding technique
TW200837349A (en) * 2007-03-07 2008-09-16 Nat Univ Tsing Hua Biochip and manufacturing method thereof
WO2009039466A1 (en) 2007-09-20 2009-03-26 Vanderbilt University Free solution measurement of molecular interactions by backscattering interferometry
US8120777B2 (en) 2007-12-10 2012-02-21 Molecular Sensing, Inc. Temperature-stable interferometer
US8535805B2 (en) * 2008-04-28 2013-09-17 The United States Of America, As Represented By The Secretary Of The Navy Hydrophobic nanostructured thin films
CN102215757A (en) * 2008-10-01 2011-10-12 罗切斯特大学 Use of non-nucleophilic additives for reduction of surface morphological anomalies in probe arrays
US20100099203A1 (en) * 2008-10-03 2010-04-22 Molecular Sensing, Inc. Substrates with surfaces modified with PEG
WO2010080708A2 (en) * 2009-01-12 2010-07-15 Molecular Sensing, Inc. Methods and systems for interferometric analysis
WO2010080710A2 (en) * 2009-01-12 2010-07-15 Molecular Sensing, Inc. Sample collection and measurement in a single container by back scattering interferometry
JP5255553B2 (en) 2009-12-11 2013-08-07 株式会社日立ハイテクノロジーズ Dispensing nozzle for automatic analyzer and automatic analyzer equipped with the same
US9310363B2 (en) * 2010-01-07 2016-04-12 Sensor-Kinesis Corporation Method and apparatus for forming of an automated sampling device for the detection of salmonella enterica utilizing an electrochemical aptamer biosensor
US9638632B2 (en) 2010-06-11 2017-05-02 Vanderbilt University Multiplexed interferometric detection system and method
WO2012079030A2 (en) * 2010-12-10 2012-06-14 The Regents Of The University Of California Bioconjugation using bifunctional linkers
US8647535B2 (en) 2011-01-07 2014-02-11 International Business Machines Corporation Conductive metal and diffusion barrier seed compositions, and methods of use in semiconductor and interlevel dielectric substrates
US9562853B2 (en) 2011-02-22 2017-02-07 Vanderbilt University Nonaqueous backscattering interferometric methods
JP5252036B2 (en) 2011-06-28 2013-07-31 大日本印刷株式会社 Substrate having a hydrophilic layer
CN104379724B (en) * 2012-01-31 2018-01-02 托莱多大学 Method and apparatus for detection and the measurement of analyte
US9273949B2 (en) 2012-05-11 2016-03-01 Vanderbilt University Backscattering interferometric methods
WO2016029139A1 (en) * 2014-08-21 2016-02-25 University Of Central Florida Research Foundation, Inc. Functionalized eyewear device for detecting biomarker in tears
WO2016118812A1 (en) 2015-01-23 2016-07-28 Vanderbilt University A robust interferometer and methods of using same
US10627396B2 (en) 2016-01-29 2020-04-21 Vanderbilt University Free-solution response function interferometry
CN108795732B (en) * 2017-04-27 2021-01-22 京东方科技集团股份有限公司 Gene detection chip, detection method thereof and micro-fluidic chip system
WO2021033789A1 (en) * 2019-08-19 2021-02-25 Nexmos Co., Ltd. An aptamer-functionalized contact lens and an early diagnosis method of disease using the same

Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
GB2324866A (en) * 1997-04-21 1998-11-04 Randox Lab Ltd Device for multianalyte assays.
WO1999017120A1 (en) * 1997-09-26 1999-04-08 Becton, Dickinson And Company Preparing conjugates using polyethylene glycol linkers
EP1132739A1 (en) * 2000-05-16 2001-09-12 BioChip Technologies GmbH Linker system for activating surfaces for bioconjugation and methods for their use
US20020045277A1 (en) * 2000-10-12 2002-04-18 Beate Schmid Process for detecting biological molecules

Family Cites Families (13)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
FR2584090B1 (en) * 1985-06-27 1987-08-28 Roussel Uclaf NEW SUPPORTS, THEIR PREPARATION AND THE INTERMEDIATES OBTAINED, THEIR APPLICATION TO THE SYNTHESIS OF OLIGONUCLEOTIDES AND THE NEW NUCLEOSIDES AND OLIGONUCLEOTIDES RELATED TO THE SUPPORTS OBTAINED
US5510481A (en) * 1990-11-26 1996-04-23 The Regents, University Of California Self-assembled molecular films incorporating a ligand
WO1994019694A1 (en) * 1993-02-19 1994-09-01 Arris Pharmaceutical Corporation Thin film hpmp matrix systems and methods for constructing and displaying ligands
JP2002523041A (en) * 1998-08-25 2002-07-30 ユニバーシティ オブ ワシントン Streptavidin variants having a second functional domain
US6506594B1 (en) * 1999-03-19 2003-01-14 Cornell Res Foundation Inc Detection of nucleic acid sequence differences using the ligase detection reaction with addressable arrays
AU769571B2 (en) * 1999-04-28 2004-01-29 Universitat Zurich Polyionic coatings in analytic and sensor devices
US20020028455A1 (en) * 2000-05-03 2002-03-07 Laibinis Paul E. Methods and reagents for assembling molecules on solid supports
US7153682B2 (en) * 2000-06-05 2006-12-26 Chiron Corporation Microarrays on mirrored substrates for performing proteomic analyses
WO2002004951A1 (en) * 2000-07-10 2002-01-17 Wakunaga Pharmaceutical Co., Ltd. Micro-array
US6905816B2 (en) * 2000-11-27 2005-06-14 Intelligent Medical Devices, Inc. Clinically intelligent diagnostic devices and methods
EP2202520A1 (en) * 2000-11-27 2010-06-30 Intelligent Medical Devices LLC Clinically intelligent diagnostic devices and methods
US6844028B2 (en) * 2001-06-26 2005-01-18 Accelr8 Technology Corporation Functional surface coating
US7067322B2 (en) * 2001-07-10 2006-06-27 Wisconsin Alumni Research Foundation Fusion protein arrays on metal substrates for surface plasmon resonance imaging

Patent Citations (4)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
GB2324866A (en) * 1997-04-21 1998-11-04 Randox Lab Ltd Device for multianalyte assays.
WO1999017120A1 (en) * 1997-09-26 1999-04-08 Becton, Dickinson And Company Preparing conjugates using polyethylene glycol linkers
EP1132739A1 (en) * 2000-05-16 2001-09-12 BioChip Technologies GmbH Linker system for activating surfaces for bioconjugation and methods for their use
US20020045277A1 (en) * 2000-10-12 2002-04-18 Beate Schmid Process for detecting biological molecules

Non-Patent Citations (3)

* Cited by examiner, † Cited by third party
Title
BEIER M ET AL: "Versatile derivatisation of solid support media for covalent bonding on DNA-microchips" NUCLEIC ACIDS RESEARCH, OXFORD UNIVERSITY PRESS, SURREY, GB, vol. 27, no. 9, 1999, pages 1970-1977, XP002145887 ISSN: 0305-1048 *
CHRISEY L A ET AL: "Covalent attachment of synthetic DNA to self-assembled monolayer films" NUCLEIC ACIDS RESEARCH, OXFORD UNIVERSITY PRESS, SURREY, GB, vol. 24, no. 15, 1996, pages 3031-3039, XP002149193 ISSN: 0305-1048 *
ZALIPSKY S: "FUNCTIONALIZED POLY(ETHYLENE GLYCOL) FOR PREPARATION OF BIOLOGICALLY RELEVANT CONJUGATES" BIOCONJUGATE CHEMISTRY, AMERICAN CHEMICAL SOCIETY, WASHINGTON, US, vol. 6, no. 2, 1995, pages 150-165, XP002068523 ISSN: 1043-1802 *

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
DE112010001382B4 (en) * 2009-03-27 2013-11-21 Hitachi High-Technologies Corporation Automatic analyzer pipetting nozzle, process for its manufacture and auto-analyzer using it

Also Published As

Publication number Publication date
EP1572352A2 (en) 2005-09-14
KR100694930B1 (en) 2007-03-14
JP2006509201A (en) 2006-03-16
US7070922B2 (en) 2006-07-04
US20060286682A1 (en) 2006-12-21
WO2004050919A3 (en) 2004-08-26
CN1720096A (en) 2006-01-11
US20040110276A1 (en) 2004-06-10
TWI277653B (en) 2007-04-01
KR20050084969A (en) 2005-08-29
TW200424315A (en) 2004-11-16

Similar Documents

Publication Publication Date Title
US20060286682A1 (en) Surface treatment
US10655166B2 (en) Electrically active combinatorial chemical (EACC) chip for biochemical analyte detection
EP0874242B2 (en) Device and apparatus for the simultaneous detection of multiple analytes
JP5588430B2 (en) Surface and method for label independent detection
US20060223113A1 (en) Immobilization of binding agents
Sung et al. Toward immunoassay chips: Facile immobilization of antibodies on cyclic olefin copolymer substrates through pre-activated polymer adlayers
UA54400C2 (en) System for simultaneously analyzing contents of several substances
JP2005525554A (en) Polyelectrolyte complexes (eg zwitterionic polythiophene) with receptors (eg polynucleotides, antibodies, etc.) for biosensor applications
US20080293592A1 (en) Method For Covalently Immobilising Biomolecules on Organic Surfaces
JP2002532699A (en) Biochip manufacturing method and biochip
EP1726661A1 (en) Method for manufacturing a biosensor element
KR101029154B1 (en) Zinc Oxide Nanostructured Micropattern and Method for Preparing the Same
Kant et al. Relevance of adhesion in fabrication of microarrays in clinical diagnostics
JP4197279B2 (en) Biologically-derived substance detection substrate and manufacturing method thereof
JP2004505170A (en) Surface-bound polyfunctional polymer networks for sensor chips
US20090171052A1 (en) Polyelectrolyte Monolayers and Multilayers for Optical Signal Transducers
AU2003261568B2 (en) Fixation carrier and solid phase
CA2708637A1 (en) Capillary driven assay device and its manufacture
Marquette et al. Biochips: non-conventional strategies for biosensing elements immobilization
Desmet et al. Surface functionalization for immobilization of probes on microarrays
Jiménez Meneses Study of substrate modulation and bioreceptor anchoring for the development of high performance microarrays
Huang 5.1 Biosensors and biointerfaces
Prilutsky et al. Bioreceptor functionalization of gold-coated sensor surfaces
Wu Microarrays: Bioassay performance on waveguide sensors and commercial capture surfaces

Legal Events

Date Code Title Description
AK Designated states

Kind code of ref document: A2

Designated state(s): CN JP KR PH SG

AL Designated countries for regional patents

Kind code of ref document: A2

Designated state(s): AT BE BG CH CY CZ DE DK EE ES FI FR GB GR HU IE IT LU MC NL PT RO SE SI SK TR

121 Ep: the epo has been informed by wipo that ep was designated in this application
DFPE Request for preliminary examination filed prior to expiration of 19th month from priority date (pct application filed before 20040101)
WWE Wipo information: entry into national phase

Ref document number: 1-2005-501059

Country of ref document: PH

WWE Wipo information: entry into national phase

Ref document number: 1020057008085

Country of ref document: KR

WWE Wipo information: entry into national phase

Ref document number: 168976

Country of ref document: IL

Ref document number: 1098/CHENP/2005

Country of ref document: IN

WWE Wipo information: entry into national phase

Ref document number: 2004557616

Country of ref document: JP

WWE Wipo information: entry into national phase

Ref document number: 20038A51975

Country of ref document: CN

WWE Wipo information: entry into national phase

Ref document number: 2003812520

Country of ref document: EP

WWP Wipo information: published in national office

Ref document number: 1020057008085

Country of ref document: KR

WWP Wipo information: published in national office

Ref document number: 2003812520

Country of ref document: EP