Strategies for the detection of food pathogens and contaminants

Stephen Hearty; Paul Leonard; Alfredo Darmanin Sheehan; Sharon Stapleton; Elizabeth Tully; Lynsey Dunne; Stephen Daly; Barry McDonnell; Peter Skottrup; Richard O'Kennedy

Strategies for the detection of food pathogens and contaminants

Stephen Hearty, Paul Leonard, Alfredo Darmanin Sheehan, Sharon Stapleton, Elizabeth Tully, Lynsey Dunne, Stephen Daly, Barry McDonnell, Peter Skottrup, Richard O'Kennedy

Klinisk Biokemisk Afdeling

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Abstract

We routinely use Biacore for affinity ranking and kinetic characterisation of diverse panels of hybridoma-derived and recombinant antibodies against a wide range of different clinically relevant antigens for diagnostic applications. Generally the analytes of interest are haptens or defined protein molecules and once suitably high affinity antibodies have been isolated, it is relatively straightforward to design and optimise concentration-based assays using SPR. Recently we have investigated the potential of applying Biacore technology to routine food analysis. Our experiences have shown that molecular contaminants such as microbial toxins and drug/pesticide residues translate well onto Biacore-based assay formats. However, larger and more complex entities such as spores and whole bacterial cells represent an altogether more difficult challenge. Here, we present an overview of our experiences to date with using Biacore for analysis of food contaminants and in particular the challenges associated with large analyte detection

Originalsprog	Udefineret/Ukendt
Publikationsdato	2006
Status	Udgivet - 2006

Adgang til dokumentet

Hearty Berlin Biacore 2006 short version final for website.pdfAccepteret manuskript, 3,19 MB

Citationsformater

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abstract = "We routinely use Biacore for affinity ranking and kinetic characterisation of diverse panels of hybridoma-derived and recombinant antibodies against a wide range of different clinically relevant antigens for diagnostic applications. Generally the analytes of interest are haptens or defined protein molecules and once suitably high affinity antibodies have been isolated, it is relatively straightforward to design and optimise concentration-based assays using SPR. Recently we have investigated the potential of applying Biacore technology to routine food analysis. Our experiences have shown that molecular contaminants such as microbial toxins and drug/pesticide residues translate well onto Biacore-based assay formats. However, larger and more complex entities such as spores and whole bacterial cells represent an altogether more difficult challenge. Here, we present an overview of our experiences to date with using Biacore for analysis of food contaminants and in particular the challenges associated with large analyte detection",

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T1 - Strategies for the detection of food pathogens and contaminants

AU - Hearty, Stephen

AU - Leonard, Paul

AU - Sheehan, Alfredo Darmanin

AU - Stapleton, Sharon

AU - Tully, Elizabeth

AU - Dunne, Lynsey

AU - Daly, Stephen

AU - McDonnell, Barry

AU - Skottrup, Peter

AU - O'Kennedy, Richard

PY - 2006

Y1 - 2006

N2 - We routinely use Biacore for affinity ranking and kinetic characterisation of diverse panels of hybridoma-derived and recombinant antibodies against a wide range of different clinically relevant antigens for diagnostic applications. Generally the analytes of interest are haptens or defined protein molecules and once suitably high affinity antibodies have been isolated, it is relatively straightforward to design and optimise concentration-based assays using SPR. Recently we have investigated the potential of applying Biacore technology to routine food analysis. Our experiences have shown that molecular contaminants such as microbial toxins and drug/pesticide residues translate well onto Biacore-based assay formats. However, larger and more complex entities such as spores and whole bacterial cells represent an altogether more difficult challenge. Here, we present an overview of our experiences to date with using Biacore for analysis of food contaminants and in particular the challenges associated with large analyte detection

AB - We routinely use Biacore for affinity ranking and kinetic characterisation of diverse panels of hybridoma-derived and recombinant antibodies against a wide range of different clinically relevant antigens for diagnostic applications. Generally the analytes of interest are haptens or defined protein molecules and once suitably high affinity antibodies have been isolated, it is relatively straightforward to design and optimise concentration-based assays using SPR. Recently we have investigated the potential of applying Biacore technology to routine food analysis. Our experiences have shown that molecular contaminants such as microbial toxins and drug/pesticide residues translate well onto Biacore-based assay formats. However, larger and more complex entities such as spores and whole bacterial cells represent an altogether more difficult challenge. Here, we present an overview of our experiences to date with using Biacore for analysis of food contaminants and in particular the challenges associated with large analyte detection

M3 - Andet bidrag

ER -