56 research outputs found
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Deposition of functionalized polymer layers in surface plasmon resonance immunosensors by in-situ polymerization in the evanescent wave field
Traditionally, the integration of sensing gel layers in surface plasmon
resonance (SPR) is achieved via âbulkâ methods, such as precipitation, spin-
coating or in-situ polymerization onto the total surface of the sensor chip,
combined with covalent attachment of the antibody or receptor to the gel
surface. This is wasteful in terms of materials as the sensing only occurs at
the point of resonance interrogated by the laser. By isolating the sensing
materials (antibodies, enzymes, aptamers, polymers, MIPs, etc.) to this exact
spot a more efficient use of these recognition elements will be achieved. Here
we present a method for the in-situ formation of polymers, using the energy of
the evanescent wave field on the surface of an SPR device, specifically
localized at the point of interrogation. Using the photo-initiator couple of
methylene blue (sensitizing dye) and sodium p-toluenesulfinate (reducing agent)
we polymerized a mixture of N,N-methylene-bis-acrylamide and methacrylic acid in
water at the focal point of SPR. No polymerization was seen in solution or at
any other sites on the sensor surface. Varying parameters such as monomer
concentration and exposure time allowed precise control over the polymer
thickness (from 20â200 nm). Standard coupling with 1-ethyl-3-(3-
dimethylaminopropyl)carbodiimide and N-hydroxysuccinimide was used for the
immobilization of protein G which was used to bind IgG in a typical biosensor
format. This model system demonstrated the characteristic performance for this
type of immunosensor, validating our deposition
The rational development of molecularly imprinted polymer-based sensors for protein detection.
The detection of specific proteins as biomarkers of disease, health status,
environmental monitoring, food quality, control of fermenters and civil defence
purposes means that biosensors for these targets will become increasingly more
important. Among the technologies used for building specific recognition
properties, molecularly imprinted polymers (MIPs) are attracting much attention.
In this critical review we describe many methods used for imprinting recognition
for protein targets in polymers and their incorporation with a number of
transducer platforms with the aim of identifying the most promising approaches
for the preparation of MIP-based protein sensors (277 references)
Direct replacement of antibodies with molecularly imprinted polymer (MIP) nanoparticles in ELISAÂ - development of a novel assay for vancomycin
A simple and straightforward technique for coating microplate wells with molecularly imprinted polymer nanoparticles (nanoMIPs) to develop ELISA type assays is presented here for the first time. NanoMIPs were synthesized by a solid phase approach with immobilized vancomycin (template) and characterized using Biacore 3000, dynamic light scattering and electron microscopy. Immobilization, blocking and washing conditions were optimized in microplate format. The detection of vancomycin was achieved in competitive binding experiments with a HRP-vancomycin conjugate. The assay was capable of measuring vancomycin in buffer and in blood plasma within the range 0.001-70 nM with a detection limit of 0.0025 nM (2.5 pM). The sensitivity of the assay was three orders of magnitude better than a previously described ELISA based on antibodies. In these experiments nanoMIPs have shown high affinity and minimal interference from blood plasma components. Immobilized nanoMIPs were stored for 1 month at room temperature without any detrimental effects to their binding properties. The high affinity of nanoMIPs and the lack of a requirement for cold chain logistics make them an attractive alternative to traditional antibodies used in ELIS
Introducing MINA-The Molecularly Imprinted Nanoparticles Assay
A new ELISAâ (enzymeâlinked immunosorbent assay)âlike assay is demonstrated in which no elements of biological origin are used for molecular recognition or signaling. Composite imprinted nanoparticles that contain a catalytic core and which are synthesized by using a solidâphase approach can simultaneously act as recognition/signaling elements, and be used with minimal modifications to standard assay protocols. This assay provides a new route towards replacement of unstable biomolecules in immunoassays
Does size matter? Study of performance of pseudo-ELISAs based on molecularly imprinted polymer nanoparticles prepared for analytes of different sizes
The aim of this work is to evaluate whether the size of the analyte used as template for the synthesis of molecularly imprinted polymer nanoparticles (nanoMIPs) can affect their performance in pseudo-enzyme linked immunosorbent assays (pseudo-ELISAs). Successful demonstration of a nanoMIPs-based pseudo-ELISA for vancomycin (1449.3 g mol) was demonstrated earlier. In the present investigation, the following analytes were selected: horseradish peroxidase (HRP, 44 kDa), cytochrome C (Cyt C, 12 kDa) biotin (244.31 g mol) and melamine (126.12 g mol). NanoMIPs with a similar composition for all analytes were synthesised by persulfate-initiated polymerisation in water. In addition, core-shell nanoMIPs coated with polyethylene glycol (PEG) and imprinted for melamine were produced in organics and tested. The polymerisation of the nanoparticles was done using a solid-phase approach with the correspondent template immobilised on glass beads. The performance of the nanoMIPs used as replacement for antibodies in direct pseudo-ELISA (for the enzymes) and competitive pseudo-ELISA for the smaller analytes was investigated. For the competitive mode we rely on competition for the binding to the nanoparticles between free analyte and corresponding analyte-HRP conjugate. The results revealed that the best performances were obtained for nanoMIPs synthesised in aqueous media for the larger analytes. In addition, this approach was successful for biotin but completely failed for the smallest template melamine. This problem was solved using nanoMIP prepared by UV polymerisation in an organic media with a PEG shell. This study demonstrates that the preparation of nanoMIP by solid-phase approach can produce material with high affinity and potential to replace antibodies in ELISA tests for both large and small analytes. This makes this technology versatile and applicable to practically any target analyte and diagnostic field
Deposition of functionalized polymer layers in surface plasmon resonance immunosensors by in-situ polymerization in the evanescent wave field
Traditionally, the integration of sensing gel layers in surface plasmon
resonance (SPR) is achieved via âbulkâ methods, such as precipitation, spin-
coating or in-situ polymerization onto the total surface of the sensor chip,
combined with covalent attachment of the antibody or receptor to the gel
surface. This is wasteful in terms of materials as the sensing only occurs at
the point of resonance interrogated by the laser. By isolating the sensing
materials (antibodies, enzymes, aptamers, polymers, MIPs, etc.) to this exact
spot a more efficient use of these recognition elements will be achieved. Here
we present a method for the in-situ formation of polymers, using the energy of
the evanescent wave field on the surface of an SPR device, specifically
localized at the point of interrogation. Using the photo-initiator couple of
methylene blue (sensitizing dye) and sodium p-toluenesulfinate (reducing agent)
we polymerized a mixture of N,N-methylene-bis-acrylamide and methacrylic acid in
water at the focal point of SPR. No polymerization was seen in solution or at
any other sites on the sensor surface. Varying parameters such as monomer
concentration and exposure time allowed precise control over the polymer
thickness (from 20â200 nm). Standard coupling with 1-ethyl-3-(3-
dimethylaminopropyl)carbodiimide and N-hydroxysuccinimide was used for the
immobilization of protein G which was used to bind IgG in a typical biosensor
format. This model system demonstrated the characteristic performance for this
type of immunosensor, validating our deposition
Effect of the cross-linker on the general performance and temperature dependent behaviour of a molecularly imprinted polymer catalyst of a Diels-Alder reaction
Here we present a series of molecularly imprinted polymers capable of catalysing
the Diels-Alder reaction between benzyl 1,3-butadienylcarbamate (1) and N,N-
dimethyl acrylamide (2). The polymer systems studied here demonstrated an
unusual cross-linker and temperature dependent behaviour, namely that polymer
catalysis of the Diels-Alder reaction was lower at elevated temperature, in
contrast to the solution reaction. Furthermore, not only was the catalytic
activity significantly influenced by the choice of cross-linker, but in a
similar fashion also the extent of the temperature effect, indicating a close
relationship between catalysis and the observed inhibition. Molecular dynamics
simulations of both the polymer systems studied were used to provide insight
into the molecular background of transition state stabilisation, and differences
in properties of the systems based on different cross-linkers
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