Literature DB >> 21339175

Sensitive immunofluorescent staining of cells via generation of fluorescent nanoscale polymer films in response to biorecognition.

Heather J Avens1, Brad J Berron, Allison M May, Katerina R Voigt, Gregory J Seedorf, Vivek Balasubramaniam, Christopher N Bowman.   

Abstract

Immunofluorescent staining is central to nearly all cell-based research, yet only a few fluorescent signal amplification approaches for cell staining exist, each with distinct limitations. Here, the authors present a novel, fluorescent polymerization-based amplification (FPBA) method that is shown to enable similar signal intensities as the highly sensitive, enzyme-based tyramide signal amplification (TSA) approach. Being non-enzymatic, FPBA is not expected to suffer from nonspecific staining of endogenous enzymes, as occurs with enzyme-based approaches. FPBA employs probes labeled with photopolymerization initiators, which lead to the controlled formation of fluorescent polymer films only at targeted biorecognition sites. Nuclear pore complex proteins (NPCs; in membranes), vimentin (in filaments), and von Willebrand factor (in granules) were all successfully immunostained by FPBA. Also, FPBA was demonstrated to be capable of multicolor immunostaining of multiple antigens. To assess relative sensitivity, decreasing concentrations of anti-NPC antibody were used, indicating that both FPBA and TSA stained NPC down to a 1:100,000 dilution. Nonspecific, cytoplasmic signal resulting from NPC staining was found to be reduced up to 5.5-fold in FPBA as compared to TSA, demonstrating better signal localization with FPBA. FPBA's unique approach affords a combination of preferred attributes, including high sensitivity and specificity not otherwise available with current techniques.

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Year:  2011        PMID: 21339175      PMCID: PMC3201124          DOI: 10.1369/jhc.2010.955948

Source DB:  PubMed          Journal:  J Histochem Cytochem        ISSN: 0022-1554            Impact factor:   2.479


  24 in total

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Journal:  J Histochem Cytochem       Date:  1999-03       Impact factor: 2.479

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Journal:  J Microbiol Methods       Date:  2009-04-20       Impact factor: 2.363

6.  Signal amplification in the detection of single-copy DNA and RNA by enzyme-catalyzed deposition (CARD) of the novel fluorescent reporter substrate Cy3.29-tyramide.

Authors:  B F Schmidt; J Chao; Z Zhu; R L DeBiasio; G Fisher
Journal:  J Histochem Cytochem       Date:  1997-03       Impact factor: 2.479

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Journal:  Histochem Cell Biol       Date:  1999-02       Impact factor: 4.304

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Authors:  Ryan R Hansen; Heather J Avens; Raveesh Shenoy; Christopher N Bowman
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  9 in total

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Journal:  Acta Pharmacol Sin       Date:  2017-04-17       Impact factor: 6.150

4.  Cell Death Persists in Rapid Extrusion of Lysis-Resistant Coated Cardiac Myoblasts.

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5.  The Role of Surface Receptor Density in Surface-Initiated Polymerizations for Cancer Cell Isolation.

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6.  Interfacial polymerization for colorimetric labeling of protein expression in cells.

Authors:  Jacob L Lilly; Phillip R Sheldon; Liv J Hoversten; Gabriela Romero; Vivek Balasubramaniam; Brad J Berron
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7.  Comparison of eosin and fluorescein conjugates for the photoinitiation of cell-compatible polymer coatings.

Authors:  Jacob L Lilly; Anuhya Gottipati; Calvin F Cahall; Mohamed Agoub; Brad J Berron
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8.  Bioinformatics tools allow targeted selection of chromosome enumeration probes and aneuploidy detection.

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Journal:  J Histochem Cytochem       Date:  2012-11-29       Impact factor: 2.479

9.  Protective Polymer Coatings for High-Throughput, High-Purity Cellular Isolation.

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  9 in total

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