Biological microbeads for flow‐cytometric immunoassays, enzyme titrations, and quantitative PCR

Pataki, Judit; Szabó, Miklós; Lantos, Erika; Székvölgyi, Lóránt; Molnár, Mónika; Hegedüs, Éva; Bacsó, Zsolt; Kappelmayer, János; Lustyik, György; Szabó, Gábor

doi:10.1002/cyto.a.20180

Cited by 8 publications

(9 citation statements)

References 21 publications

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“…approach has been demonstrated in the case of various assays of molecular diagnostic value: immunoassays, sensitive measurement of protease or nuclease activity, detection of deletion/insertion of sequences by heteroduplex analysis, etc., that could all be adapted to a 'lab-on-beads' platform, i.e., the flow-cytometric analysis of microbead-captured macromolecules (1,18,19). Many samples can be simultaneously analyzed in a FACSarray instrument using fluorescent dyes matching its optical channels.…”

Section: Flow-and Laser Scanning Cytometry In Epigenetics Researchmentioning

confidence: 99%

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Flow Cytometric and Laser Scanning Microscopic Approaches in Epigenetics Research

Székvölgyi

Imre

Minh

et al. 2009

Chromatin Immunoprecipitation Assays

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Our understanding of epigenetics has been transformed in recent years by the advance of technological possibilities based primarily on a powerful tool, chromatin immunoprecipitation (ChIP). However, in many cases, the detection of epigenetic changes requires methods providing a high-throughput (HTP) platform. Cytometry has opened a novel approach for the quantitative measurement of molecules, including PCR products, anchored to appropriately addressed microbeads (Pataki et al. 2005. Cytometry 68, 45-52). Here we show selected examples for the utility of two different cytometry-based platforms of epigenetic analysis: ChIP-on-beads, a flow-cytometric test of local histone modifications (Balint et al. 2005. Mol. Cell Biol. 25, 5648-5663), and the laser scanning cytometry-based measurement of global epigenetic modifications that might help predict clinical behavior in different pathological conditions. We anticipate that such alternative tools may shortly become indispensable in clinical practice, translating the systematic screening of epigenetic tags from basic research into routine diagnostics of HTP demand.

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Section: Flow-and Laser Scanning Cytometry In Epigenetics Researchmentioning

confidence: 99%

“…However, in many cases, the detection of epigenetic changes requires methods providing a high-throughput (HTP) platform. Cytometry has opened a novel approach for the quantitative measurement of molecules, including PCR products, anchored to appropriately addressed microbeads (Pataki et al 2005. Cytometry 68, 45-52).…”

mentioning

confidence: 99%

Flow Cytometric and Laser Scanning Microscopic Approaches in Epigenetics Research

Székvölgyi

Imre

Minh

et al. 2009

Chromatin Immunoprecipitation Assays

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“…Fluorescently functionalized microspheres and nanospheres are available commercially from several sources, spanning the UV-to-IR, in a variety of sizes ranging from 20 nm to 5 µm (3). Fluorescent microspheres are also commonly labeled with primary or secondary antibodies and are used as solid supports in many sandwich immunoassays, where they take full advantage of solution-based kinetics (51)(52)(53). Alternatively, microspheres can be obtained with carboxyl, amine or other surface-displayed functional groups for chemical conjugation to biologic molecules (3).…”

Section: Fluorescent Polymeric Microspheres and Nanospheresmentioning

confidence: 99%

Fluorescence Spectroscopy: Applications in Chemical Biology

Sapsford

Berti²,

Medintz

2008

Wiley Encyclopedia of Chemical Biology

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Fluorescence spectroscopy in all of its variations can be considered among the most powerful types of analysis available to chemical biology. However, to be useful almost all applications are dependent on optimal labeling of biomolecules with a fluorophore and on the appropriate choice of analytical technique. In this article, we examine the applications and contributions of fluorescent spectroscopy to chemical biology in three inter‐related sections. We first examine the properties of the common fluorophores available from many disparate structural and functional classes, which includes a discussion of their individual benefits and liabilities in the context of their application. The available conjugation chemistries used to attach fluorophores to myriad biomolecules are next reviewed. As each class of biomolecule differs in both structure and function, the focus here is on strategies for the specific labeling of different functional groups. Last, some major types of fluorescent spectroscopy and the associated biologic questions and analysis that can be addressed with them are covered briefly.

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“…This approach has been used to simultaneously measure activated cells and released cytokines in whole blood (86) and more examples are likely to follow. Further blurring the distinction between cell‐based assays and bead‐based assays is the notion of using cells as microparticles for multiplexed analysis (87). In this configuration, fixed bacteria or yeast cells may encode information and display receptors or other molecules, but are not themselves the object of study.…”

Section: Conclusion and Prospectsmentioning

confidence: 99%

Multiplexed and microparticle‐based analyses: Quantitative tools for the large‐scale analysis of biological systems

2006

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While the term flow cytometry refers to the measurement of cells, the approach of making sensitive multiparameter optical measurements in a flowing sample stream is a very general analytical approach. The past few years have seen an explosion in the application of flow cytometry technology for molecular analysis and measurements using microparticles as solid supports. While microsphere-based molecular analyses using flow cytometry date back three decades, the need for highly parallel quantitative molecular measurements that has arisen from various genomic and proteomic advances has driven the development in particle encoding technology to enable highly multiplexed assays. Multiplexed particle-based immunoassays are now common place, and new assays to study genes, protein function, and molecular assembly. Numerous efforts are underway to extend the multiplexing capabilities of microparticle-based assays through new approaches to particle encoding and analyte reporting. The impact of these developments will be seen in the basic research and clinical laboratories, as well as in drug development. q 2006 International Society for Analytical CytologyKey terms: microarray; systems biology; proteomics; protein array; high throughput screening; drug discovery; diagnostics A major goal for biomedical research in the 21st century will be to collect and integrate molecular information about genes, proteins, and numerous other biomolecules into the working models of cell and organism function from which predictions can be made. The rationale for pursuing such an ambitious goal stems from the very significant advances in molecular analysis that enable the sequencing of whole genomes, the highly parallel analysis of gene expression levels, and large scale identification of proteins in complex samples. These advances resulted from new molecular reagents and assay chemistries, new instrumentation with improved sensitivity and throughput, new computational tools, and a significant change in focus for experimental biology from one that focuses on individual molecules to one that considers the abundance and interactions of many different molecules as they function in networks of biochemical pathways in living systems.However, just as these new technologies have enabled the rapid acceleration of data collection and interpretation, continued progress toward transforming this information into biological understanding is dependent on continued improvement in analytical technologies. In particular, it is critical to augment qualitative analysis methods that allow the identification of important molecules with quantitative measurements of their abundance and function. The ability to make quantitative measurements of the concentrations of many individual proteins, their interactions and the formation of macromolecular assemblies, and the measurement of these assemblies in live cells and organisms represent major challenges in understanding the systems of molecular networks and pathways that underlie physiology and disease. These challenge...

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Biological microbeads for flow‐cytometric immunoassays, enzyme titrations, and quantitative PCR

Cited by 8 publications

References 21 publications

Flow Cytometric and Laser Scanning Microscopic Approaches in Epigenetics Research

Flow Cytometric and Laser Scanning Microscopic Approaches in Epigenetics Research

Fluorescence Spectroscopy: Applications in Chemical Biology

Multiplexed and microparticle‐based analyses: Quantitative tools for the large‐scale analysis of biological systems

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