Your search keyword '"Landegren U"' showing total 24 results

1. Protein Diagnostics by Proximity Ligation

Author

Cane, G., primary, Leuchowius, K.-J., additional, Söderberg, O., additional, Kamali-Moghaddam, M., additional, Jarvius, M., additional, Helbing, I., additional, Pardali, K., additional, Koos, B., additional, Ebai, T., additional, and Landegren, U., additional

Published

2017

2. List of Contributors

Author

Ali, B.R., primary, Ansorge, W.J., additional, Atherton, D.S., additional, Barnett, M.P.G., additional, Bell, W.C., additional, Brand, S.R., additional, Cane, G., additional, Chantratita, W., additional, Conze, T., additional, Corach, D., additional, Coun, F., additional, Danielson, P.B., additional, den Dunnen, J.T., additional, Dequeker, E., additional, De Rycke, M., additional, Deshpande, A., additional, Drmanac, S., additional, Drmanac, R., additional, Ebai, T., additional, Farrar, J.S., additional, Ferguson, L.R., additional, Forero, D.A., additional, Fredenburgh, J., additional, Gale, B.K., additional, Göransson, J., additional, Grizzle, W.E., additional, Grundberg, I., additional, Gut, I.G., additional, Heideman, D., additional, Helbing, I., additional, Henriksson, S., additional, Hernández-Neuta, I., additional, Innocenti, F., additional, Isaksson, M., additional, Jarvius, M., additional, Jayamohan, H., additional, Kamali-Moghaddam, M., additional, Kampourakis, K., additional, Katsila, T., additional, Koos, B., additional, Koumakis, L., additional, Laissue, P., additional, Landegren, U., additional, Larsson, C., additional, Legg, K.M., additional, Leuchowius, K.-J., additional, Li, H., additional, Liu, J.S., additional, Llerena, A., additional, Lopez-Correa, C., additional, Mathieu, C., additional, McKiernan, H.E., additional, Mendrinou, E., additional, Mezger, A., additional, Mitropoulos, K., additional, Mizzi, C., additional, Moens, L., additional, Mohamed, Z., additional, Nelson, J., additional, Nilsson, M., additional, Overbergh, L., additional, Papachatzopoulou, A., additional, Pardali, K., additional, Patenaude, A.F., additional, Patrinos, G.P., additional, Patsalis, P.C., additional, Peters, B.A., additional, Potamias, G., additional, Reisdorph, N., additional, Romanov, V., additional, Samuel, R., additional, Sexton, K.C., additional, Sgourou, A., additional, Sie, D., additional, Sistermans, E., additional, Söderberg, O., additional, Son, J., additional, Squassina, A., additional, Staessen, C., additional, Stenberg, J., additional, Taschner, P.E.M., additional, Tönnies, H., additional, Tost, J., additional, Tzimas, G., additional, Velissariou, V., additional, Viennas, E., additional, Vig, S., additional, White, P.S., additional, Wittwer, C.T., additional, Wonkam, A., additional, Xun, X., additional, and Ylstra, B., additional

Published

2017

3. Detection of SARS-CoV-2 antibodies in serum and dried blood spot samples of vaccinated individuals using a sensitive homogeneous proximity extension assay.

Author

Zhao H, Wang M, Muthelo P, Löf L, Sterky F, Gallini R, Kumar NV, Monsen T, Nilsson K, Åberg M, Kamali-Moghaddam M, Mei YF, and Landegren U

Subjects

Humans, Biological Assay, Antibodies, Kinetics, Oligonucleotides, Antibodies, Viral, SARS-CoV-2, COVID-19 diagnosis

Abstract

A homogeneous PCR-based assay for sensitive and specific detection of antibodies in serum or dried blood spots (DBS) is presented and the method is used to monitor individuals infected with or vaccinated against SARS-CoV-2. Detection probes were prepared by conjugating the recombinant spike protein subunit 1 (S1), containing the receptor binding domain (RBD) of SARS-CoV-2, to each of a pair of specific oligonucleotides. The same was done for the nucleocapsid protein (NP). Upon incubation with serum or DBS samples, the bi- or multivalency of the antibodies (IgG, IgA or IgM) brings pairs of viral proteins with their conjugated oligonucleotides in proximity, allowing the antibodies to be detected by a modified proximity extension assay (PEA). Anti-S1 and anti-NP antibodies could be detected simultaneously from one incubation reaction. This Antibody PEA (AbPEA) test uses only 1 µl of neat or up to 100,000-fold diluted serum or one ø1.2 mm disc cut from a DBS. All 100 investigated sera and 21 DBS collected prior to the COVID-19 outbreak were negative, demonstrating a 100% specificity. The area under the curve, as evaluated by Receiver Operating Characteristic (ROC) analysis reached 0.998 (95%CI: 0.993-1) for samples taken from 11 days after symptoms onset. The kinetics of antibody responses were monitored after a first and second vaccination using serially collected DBS from 14 individuals. AbPEA offers highly specific and sensitive solution-phase antibody detection without requirement for secondary antibodies, no elution step when using DBS sample in a simple procedure that lends itself to multiplex survey of antibody responses., Competing Interests: Declaration of Competing Interest UL is a founder and shareholder of Olink Proteomics, having rights to the PEA technology. All other authors declare that they have no competing financial interests or personal relationships that could influence the work reported in this paper., (Copyright © 2022. Published by Elsevier B.V.)

Published

2022

4. Human proteins incorporated into tick-borne encephalitis virus revealed by in situ proximity ligation.

Author

Ikebuchi R, Isaac AW, Yoshii K, Doulabi EM, Löf L, Azimi A, Chen L, Fredolini C, Gallini R, Landegren U, and Kamali-Moghaddam M

Subjects

Cell Line, Humans, Proteins ultrastructure, Virion metabolism, Virion ultrastructure, Encephalitis Viruses, Tick-Borne metabolism, Nucleic Acid Amplification Techniques methods, Proteins metabolism

Abstract

Host proteins incorporated into virus particles have been reported to contribute to infectivity and tissue-tropism. This incorporation of host proteins is expected to be variable among viral particles, however, protein analysis at single-virus levels has been challenging. We have developed a method to detect host proteins incorporated on the surface of virions using the in situ proximity ligation assay (isPLA) with rolling circle amplification (RCA), employing oligonucleotide-conjugated antibody pairs. The technique allows highly selective and sensitive antibody-based detection of viral and host proteins on the surface of individual virions. We detected recombinant noninfectious sub-viral particles (SVPs) of tick-borne encephalitis virus (TBEV) immobilized in microtiter wells as fluorescent particles detected by regular fluorescence microscopy. Counting the particles in the images enabled us to estimate individual TBEV-SVP counts in different samples. Using isPLA we detected individual calnexin-, CD9-, CD81-, CD29- and CD59-positive SVPs among the viral particles. Our data suggests that a diversity of host proteins may be incorporated into TEBV, illustrating that isPLA with digital counting enables single-virus analysis of host protein incorporation., Competing Interests: Declaration of competing interest The authors declare the following financial interests/personal relationships which may be considered as potential competing interests: Ulf Landegren is a founder, shareholder and board member of Navinci, having rights to the in situ PLA (isPLA) technology., (Copyright © 2020 The Authors. Published by Elsevier Inc. All rights reserved.)

Published

2020

5. A myopic perspective on the future of protein diagnostics.

Author

Landegren U, Al-Amin RA, and Björkesten J

Subjects

Biomarkers analysis, Humans, Immunoassay, Blood Proteins analysis, Proteome

Abstract

Plasma proteome analyses of the future promise invaluable insights into states of health, not only by measuring proteins whose role it is to ensure blood homeostasis, but increasingly also as a window into the health of practically any tissue in the body via so-called leakage protein biomarkers. Realizing more of this vast potential will require progress along many lines. Here we discuss the main ones, such as optimal selection of target proteins, affinity reagents, immunoassay formats, samples, and applications, with a view from ongoing work in our laboratory., (Copyright © 2018 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2018

6. AFFINOMICS and the prospects for large-scale protein analyses.

Author

Landegren U

Subjects

Affinity Labels economics, Biotechnology, European Union, Humans, Proteomics economics, Proteomics trends, Proteins analysis, Proteomics methods

Published

2016

7. Offshoots of the ESF functional genomics programme.

Author

Landegren U

Subjects

Biological Specimen Banks, Europe, Foundations, Humans, Indicators and Reagents, Protein Binding, Genomics, Molecular Biology

Abstract

After the conclusion of the second five-year period of the European Science Foundation (ESF) programme on functional genomics, it is time to take stock and evaluate its accomplishments. The programme networked leading scientists from a large number of European countries for strategy discussions about the promotion of functional genomics research, and to arrange scientific meetings and exchange programmes. In brief, I believe this programme has punched above its weight, and that it has successfully contributed to the overall organisation of molecular biosciences in Europe. With a modest annual budget the programme has created several interesting new opportunities, some of which may have yet to show their full impact. However, these mini-reviews are intended to provide a personal perspective on this functional genomics effort, and accordingly I focus on my personal experiences from the ESF programme., (Copyright © 2013 Elsevier B.V. All rights reserved.)

Published

2013

8. Protein tag-mediated conjugation of oligonucleotides to recombinant affinity binders for proximity ligation.

Author

Gu GJ, Friedman M, Jost C, Johnsson K, Kamali-Moghaddam M, Plückthun A, Landegren U, and Söderberg O

Subjects

Cell Extracts, Cell Line, Tumor, Female, HEK293 Cells, Humans, Indicators and Reagents, Receptor, ErbB-2 metabolism, Molecular Probes metabolism, Oligonucleotides metabolism, Protein Interaction Mapping methods, Recombinant Fusion Proteins metabolism

Abstract

While antibodies currently play a dominant role as affinity reagents in biological research and for diagnostics, a broad range of recombinant proteins are emerging as promising alternative affinity reagents in detection assays and quantification. DNA-mediated affinity-based assays, such as immuno-PCR and proximity ligation assays (PLA), use oligonucleotides attached to affinity reagents as reporter molecules. Conjugation of oligonucleotides to affinity reagents generally employs chemistries that target primary amines or cysteines. Because of the random nature of these processes neither the number of oligonucleotides conjugated per molecule nor their sites of attachment can be accurately controlled for affinity reagents with several available amines and cysteines. Here, we present a straightforward and convenient approach to functionalize recombinant affinity reagents for PLA by expressing the reagents as fusion partners with SNAP protein tags. This allowed us to conjugate oligonucleotides in a site-specific fashion, yielding precisely one oligonucleotide per affinity reagent. We demonstrate this method using designed ankyrin repeat proteins (DARPins) recognizing the tumor antigen HER2 and we apply the conjugates in different assay formats. We also show that SNAP or CLIP tags, expressed as fusion partners of transfected genes, allow oligonucleotide conjugations to be performed in fixed cells, with no need for specific affinity reagents. The approach is used to demonstrate induced interactions between the fusion proteins FKBP and FRB by allowing the in situ conjugated oligonucleotides to direct the production of templates for localized rolling circle amplification reactions., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2013

9. Workshop on laboratory protocol standards for the Molecular Methods Database.

Author

Klingström T, Soldatova L, Stevens R, Roos TE, Swertz MA, Müller KM, Kalaš M, Lambrix P, Taussig MJ, Litton JE, Landegren U, and Bongcam-Rudloff E

Subjects

Internet, Congresses as Topic, Databases as Topic, Laboratories standards, Molecular Biology methods, Molecular Biology standards

Abstract

Management of data to produce scientific knowledge is a key challenge for biological research in the 21st century. Emerging high-throughput technologies allow life science researchers to produce big data at speeds and in amounts that were unthinkable just a few years ago. This places high demands on all aspects of the workflow: from data capture (including the experimental constraints of the experiment), analysis and preservation, to peer-reviewed publication of results. Failure to recognise the issues at each level can lead to serious conflicts and mistakes; research may then be compromised as a result of the publication of non-coherent protocols, or the misinterpretation of published data. In this report, we present the results from a workshop that was organised to create an ontological data-modelling framework for Laboratory Protocol Standards for the Molecular Methods Database (MolMeth). The workshop provided a set of short- and long-term goals for the MolMeth database, the most important being the decision to use the established EXACT description of biomedical ontologies as a starting point., (Copyright © 2012. Published by Elsevier B.V. All rights reserved.)

Published

2013

10. Multiplex protein detection with DNA readout via mass spectrometry.

Author

Flanigon J, Kamali-Moghaddam M, Burbulis I, Annink C, Steffen M, Oeth P, Brent R, van den Boom D, Landegren U, and Cantor C

Subjects

Animals, Chickens, Polymerase Chain Reaction, Proteins chemistry, DNA analysis, Proteins analysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

Multiplex protein quantification has been constrained by issues of assay specificity, sensitivity and throughput. This research presents a novel approach that overcomes these limitations using antibody-oligonucleotide conjugates for immuno-polymerase chain reaction (immuno-PCR) or proximity ligation, coupled with competitive PCR and MALDI-TOF mass spectrometry. Employing these combinations of technologies, we demonstrate multiplex detection and quantification of up to eight proteins, spanning wide dynamic ranges from femtomolar concentrations, using only microliter sample volumes., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2013

11. Molecular tools for companion diagnostics.

Author

Zieba A, Grannas K, Söderberg O, Gullberg M, Nilsson M, and Landegren U

Subjects

Genotyping Techniques, Humans, Neoplasm Proteins blood, Neoplasms blood, Neoplasms genetics, Neoplastic Cells, Circulating pathology, Sequence Analysis, DNA, Molecular Diagnostic Techniques methods, Neoplasms diagnosis

Abstract

The heterogeneous nature of cancer results in highly variable therapeutic responses even among patients with identical stages and grades of a malignancy. The move towards personalised medicine in cancer therapy has therefore been motivated by a need to customise therapy according to molecular features of individual tumours. Companion diagnostics serves to support early drug development, it can provide surrogate markers in clinical trials, and also guide selection of individual therapies and monitoring of responses in routine clinical care. The era of companion diagnostics can be said to have begun with the introduction of the HercepTest - a first-of-a-kind diagnostic tool developed by DakoCytomation in 1998 to select patients for therapy with the anticancer drug Herceptin (trastuzumab). Herceptin and the paired test proved that companion diagnostics can help guide patient-tailored therapies. We will discuss herein technologies to analyse companion diagnostics markers at the level of DNA, RNA or protein, focusing on a series of methods developed in our laboratory that can facilitate drug development and help stratify patients for therapy., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

12. Visualising individual sequence-specific protein-DNA interactions in situ.

Author

Weibrecht I, Gavrilovic M, Lindbom L, Landegren U, Wählby C, and Söderberg O

Subjects

Alu Elements genetics, Animals, Base Sequence, Genome, Human genetics, Histones metabolism, Humans, Image Processing, Computer-Assisted, Mice, NIH 3T3 Cells, Nucleic Acid Hybridization, Oligonucleotides metabolism, Protein Binding, Templates, Genetic, Biological Assay methods, DNA metabolism, DNA-Binding Proteins metabolism

Abstract

Gene expression - a key feature for modulating cell fate-is regulated in part by histone modifications, which modulate accessibility of the chromatin to transcription factors. Until now, protein-DNA interactions (PDIs) have mostly been studied in bulk without retrieving spatial information from the sample or with poor sequence resolution. New tools are needed to reveal proteins interacting with specific DNA sequences in situ for further understanding of the orchestration of transcriptional control within the nucleus. We present herein an approach to visualise individual PDIs within cells, based on the in situ proximity ligation assay (PLA). This assay, previously used for the detection of protein-protein interactions in situ, was adapted for analysis of target PDIs, using padlock probes to identify unique DNA sequences in complex genomes. As a proof-of-principle we detected histone H3 interacting with a 26 bp consensus sequence of the Alu-repeat abundantly expressed in the human genome, but absent in mice. However, the mouse genome contains a highly similar sequence, providing a model system to analyse the selectivity of the developed methods. Although efficiency of detection currently is limiting, we conclude that in situ PLA can be used to achieve a highly selective analysis of PDIs in single cells., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2012

13. Ligation-based molecular tools for lab-on-a-chip devices.

Author

Melin J, Jarvius J, Larsson C, Söderberg O, Landegren U, and Nilsson M

Subjects

Humans, Ligases metabolism, Nucleic Acid Amplification Techniques, Lab-On-A-Chip Devices, Molecular Probe Techniques

Abstract

Molecular diagnostics can offer early detection of disease, improved diagnostic accuracy, and qualified follow-up. Moreover, the use of microfluidic devices can in principle render these analyses quickly and user-friendly, placing them within the reach of the general practitioner and maybe even in households. However, the progress launching such devices has been limited so far. We propose that an important limiting factor has been the difficulty of establishing molecular assays suitable for microfabricated formats. The assays should be capable of monitoring a wide range of molecules, including genomic DNA, RNA and proteins with secondary modifications and interaction partners, and they must exhibit excellent sensitivity and specificity. We discuss these problems and describe a series of molecular tools that may present new opportunities for lab-on-a-chip devices at the point-of-care.

Published

2008

14. Proximity ligation assays for sensitive and specific protein analyses.

Author

Gustafsdottir SM, Schallmeiner E, Fredriksson S, Gullberg M, Söderberg O, Jarvius M, Jarvius J, Howell M, and Landegren U

Subjects

Proteins chemistry, Sensitivity and Specificity, Antibodies chemistry, Biological Assay methods, DNA Ligases chemistry, Oligodeoxyribonucleotides chemistry, Polymerase Chain Reaction methods, Proteins antagonists & inhibitors

Published

2005

15. A sense of closeness: protein detection by proximity ligation.

Author

Gullberg M, Fredriksson S, Taussig M, Jarvius J, Gustafsdottir S, and Landegren U

Subjects

Base Sequence, Enzyme-Linked Immunosorbent Assay methods, Macromolecular Substances, Nucleic Acid Amplification Techniques methods, Oligonucleotides chemistry, Protein Binding, Proteins analysis, Proteins genetics, DNA Probes, Molecular Probe Techniques, Proteins chemistry, Sequence Analysis, Protein methods

Abstract

Highly specific and sensitive procedures will be required to evaluate proteomes. Proximity ligation is a recently introduced mechanism for protein analysis. In this technique, the convergence of sets of protein-binding reagents on individual target molecules juxtaposes attached nucleic acid sequences. Through a ligation reaction a DNA reporter sequence is created, which can be amplified. The procedure thus encodes detected proteins as specific nucleic acid sequences in what may be viewed as a reverse translation reaction.

Published

2003

16. More keys to padlock probes: mechanisms for high-throughput nucleic acid analysis.

Author

Banér J, Nilsson M, Isaksson A, Mendel-Hartvig M, Antson DO, and Landegren U

Subjects

Biotechnology methods, DNA, Circular, Nucleic Acid Conformation, RNA, RNA, Circular, Molecular Probe Techniques, Oligonucleotide Probes

Abstract

With the impending availability of total information about nucleic acid sequences in humans and other organisms, tools to investigate these sequences on a large scale assume increasing importance. Methods currently in use, however, cannot offer the required combination of high-throughput, sensitivity and specificity of detection. Padlock probes, circularizing oligonucleotides, may provide a means to detect, distinguish, quantitate and also locate very large numbers of DNA or RNA sequences. Recent developments in areas such as the biochemistry of ligation and characterization of ligases, methods to replicate circularized probes and the development of assays based on these principles augment the potential of padlock probes.

Published

2001

17. Molecular genetic applications of streptavidin-coated manifold supports.

Author

Barbany G, Hagberg A, Waldenström E, and Landegren U

Subjects

DNA, Complementary genetics, Gene Amplification, Humans, Kinetics, Metals, Rare Earth, Microscopy, Electron, Scanning, Protein Binding, Protein Engineering, RNA, Messenger isolation & purification, Sequence Analysis, DNA methods, Surface Properties, Molecular Biology methods, Streptavidin

Abstract

Practical problems of handling large numbers of samples limit the application of molecular genetic procedures in clinical settings and in research. In the present review we describe a multipronged manifold support, coated with streptavidin, that offers distinct advantages in preparative and diagnostic applications. In order to increase the surface available on the manifold, porous Sepharose particles conjugated with streptavidin were attached to the plastic support. This procedure increased the surface by almost three orders of magnitude, permitting sufficient streptavidin to be coupled to the support for most routine applications. The manifold supports have been used for sample preparation and in a number of genetic assays, including allele discrimination assays and DNA sequencing, In all these assay formats the manifold supports allow large numbers of samples to be processed in parallel.

Published

1999

18. Accessing genomic information: alternatives to PCR.

Author

Isaksson A and Landegren U

Subjects

Nucleic Acid Amplification Techniques, Polymerase Chain Reaction methods, Genetic Techniques, Oligonucleotide Array Sequence Analysis methods, Sequence Analysis, DNA methods

Abstract

The growing abundance of genomic sequence data invites increasingly large-scale genetic analyses. Studies of genetic variation in large sets of genes can illuminate important disease mechanisms and serve to identify novel drug targets or predict therapeutic responses. At present mostly a concern in extensive research projects, large-scale genetic analyses will gradually also find their way into clinical practice as an aid to the physician. It is timely, therefore, to take stock of methods that are becoming available for analyses of large sets of gene sequences. Clearly PCR remains the workhorse for molecular genetic analysis, and several modifications such as homogenous amplification assays and parallel detection on DNA microarrays further increase throughput. Recent developments, however, also offer hope that other methods will become available for genomic investigations, providing substantially increased analytical capacity.

Published

1999

19. Seven-color time-resolved fluorescence hybridization analysis of human papilloma virus types.

Author

Samiotaki M, Kwiatkowski M, Ylitalo N, and Landegren U

Subjects

Female, Fluorometry methods, Humans, Metals, Rare Earth analysis, Polymerase Chain Reaction methods, Sensitivity and Specificity, In Situ Hybridization, Fluorescence methods, Papillomaviridae genetics, Papillomaviridae isolation & purification

Abstract

Identification of human papilloma virus (HPV) types is important in order to determine the risk of cervical carcinoma in women. This requires a technique to probe individual samples for multiple virus specificities. Here we describe simultaneous multicolor analysis of amplification products for any of seven amplified HPV types 16, 18, 31, 33, 35, 39, and 45, associated with cancer of the cervix. A seminested polymerase chain reaction was performed in a single tube using a biotinylated inner primer. Sets of amplification products, immobilized on a 96-pronged manifold solid support, were rendered single stranded and probed with a mix of seven type-specific, differentially labeled oligonucleotides. These probes contained 10 or 20 lanthanide chelates at the 5' ends with seven distinct combinations of europium, terbium, and samarium ions. The seven viral strains were correctly identified by time-resolved fluorescence measurement of the specifically hybridized probes. Using this assay format, simultaneous detection of any of seven or even more target variants is possible., (Copyright 1997 Academic Press.)

Published

1997

20. The challengers to PCR: a proliferation of chain reactions.

Author

Landegren U

Subjects

Base Sequence, Cloning, Molecular, DNA analysis, DNA chemistry, Genome, Humans, Polymerase Chain Reaction methods

Published

1996

21. A high-capacity manifold support for the detection of specific IgE antibodies in allergic individuals.

Author

Kwiatkowski M, Parik J, and Landegren U

Subjects

Chelating Agents, Enzyme-Linked Immunosorbent Assay, Europium, Fluorescence, Humans, Immunoassay methods, Immunoenzyme Techniques, Immunoglobulin E blood, Allergens immunology, Antibody Specificity, Hypersensitivity diagnosis, Immunoassay instrumentation, Immunoglobulin E immunology

Abstract

A high-capacity manifold support with immobilized antigen was developed for the analysis of IgE-mediated immune reactivity in allergic subjects. Using this 96-pronged support, specific antibodies were trapped and detected from large sets of serum samples. We describe the binding of large amounts of antigen onto the expanded surface of the manifold support, permitting efficient identification of allergic individuals.

Published

1994

22. A manifold support for molecular genetic reactions.

Author

Parik J, Kwiatkowski M, Lagerkvist A, Lagerström Fermér M, Samiotaki M, Stewart J, Glad G, Mendel-Hartvig M, and Landegren U

Subjects

Avidin, Bacterial Proteins, Biotin, DNA isolation & purification, Kinetics, Polymerase Chain Reaction, Polystyrenes, Sepharose, Streptavidin, Molecular Biology instrumentation

Abstract

Large numbers of samples can be efficiently processed through sequential reaction steps using a 96-pronged support that projects into individual microtiter wells. The support was constructed by creating a porous surface on a disposable polystyrene manifold, with avidin coupled to this greatly expanded surface. The shape and high binding capacity of the device allow the parallel transfer of large sets of reaction intermediates between different binding or enzymatic processing steps. We have applied the support to increase the efficiency of preparative and analytical molecular genetic reactions. The support also reduce the risks of sample mix-up and contamination in applications such as PCR and DNA sequencing.

Published

1993

23. Detection of mutations in human DNA.

Author

Landegren U

Subjects

Alleles, DNA drug effects, Humans, Nucleic Acid Denaturation, Nucleic Acid Hybridization, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length, DNA Mutational Analysis

Abstract

Efficient methods for the detection of mutations are of fundamental importance in research and in diagnostics. By detection of a DNA sequence alteration that cosegregates with a clinical phenotype in an affected family, the gene at fault may be identified and assigned a function. Mutation detection methods are also a rate-limiting factor for the clinical application of DNA diagnostics. Currently a large number of techniques are in use to scan for new mutations and to distinguish among previously established sequence variants. Here, some of the problems connected with mutation detection are discussed together with principles on which current and future mutation detection assays can be based.

Published

1992

24. Measurement of cell numbers by means of the endogenous enzyme hexosaminidase. Applications to detection of lymphokines and cell surface antigens.

Author

Landegren U

Subjects

Animals, Binding Sites, Antibody, Cell Line, Humans, Interferons physiology, Interleukin-2 physiology, Liver metabolism, Lymphocytes enzymology, Lymphocytes immunology, Lymphocytes metabolism, Mice, Antigens, Surface immunology, Cell Count methods, Hexosaminidases metabolism, Lymphokines physiology

Abstract

By using a chromogenic substrate for an ubiquitous lysosomal enzyme, hexosaminidase to estimate cell numbers, a sensitive and simple procedure has been developed in which microtiter reaction wells are directly scanned in a spectrophotometer. This method has been adapted to several cell biological assays. Quantitation of the biological activities of T cell growth factor and interferon can be performed on large numbers of samples. Adhesion of dispersed solid tissue cells to fibronectin coated substrates may be quantitated with little expenditure of reagents. By use of a panning procedure in microtiter plates a sensitive and very simple assay for the binding of monoclonal antibodies to cell surface antigens has been developed.

Published

1984