Local retention of antibodies in vivo with an injectable film embedded with a fluorogen-activating protein

Liu, Wen; Saunders, Matthew; Bagia, Christina; Freeman, Eric C.; Fan, Yong; Gawalt, Ellen S.; Waggoner, Alan S.; Meng, Wilson S.

doi:10.1016/j.jconrel.2016.03.032

Cited by 16 publications

(8 citation statements)

References 60 publications

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“…For example, peptide and protein self-assemblies are under considerable investigation for many non-immunological applications such as tissue engineering and cell scaffolds, 14, 15, 45 drug delivery, 16, 20, 2146–48 antimicrobials, 49 wound healing, 19, 50 and others. 51, 52 In this broad range of applications, any antibody response against proteins, peptides, or other antigenic components incorporated into the materials could lead to blockage of the factors’ function, early clearance of the material, or at worst, inflammatory rejection responses, although in general peptide assemblies have been found to be non-inflammatory to date.…”

Section: Discussionmentioning

confidence: 99%

Switching the Immunogenicity of Peptide Assemblies Using Surface Properties

et al. 2016

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Biomaterials created from supramolecular peptides, proteins, and their derivatives have been receiving increasing interest for both immunological applications such as vaccines and immunotherapies, as well as ostensibly non-immunological applications such as therapeutic delivery or tissue engineering. However, simple rules for either maximizing immunogenicity or abolishing it have yet to be elucidated, even though immunogenicity is a prime consideration for the design of any supramolecular biomaterial intended for use in vivo. Here we investigated a range of physicochemical properties of fibrillized peptide biomaterials, identifying negative surface charge as a means for completely abolishing antibody and T cell responses against them in mice, even when they display a competent epitope. The work was facilitated by the modularity of the materials, which enabled the generation of a set of co-assembled fibrillar peptide materials with broad ranges of surface properties. It was found that negative surface charge, provided via negatively charged amino acid residues, prevented T cell and antibody responses to antigen-carrying assemblies because it prevented uptake of the materials by antigen presenting cells (APCs), which in turn prevented presentation of the epitope peptide in the APCs’ major histocompatibility (MHC) class II molecules. Conversely, positive surface charge augmented the uptake of fibrillized peptides by APCs. These findings suggest that some surface characteristics such as extensive negative charge should be avoided in vaccine design using supramolecular peptide assemblies. More importantly, it provides a strategy to switch off potentially problematic immunogenicity for using these materials in non-immunological applications.

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Section: Discussionmentioning

confidence: 99%

Switching the Immunogenicity of Peptide Assemblies Using Surface Properties

et al. 2016

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“…This paper lays the groundwork for future investigations of GABA A R trafficking with the γ2 pH FAP sensor. Importantly, this technique can be further extended toward pharmacology-focused efforts in high-throughput screenings (Fisher et al, 2014;Snyder et al, 2015), assay development based on flow cytometry (Saunders et al, 2012;Wu et al, 2014) or high-resolution 96-well plate assays (Larsen et al, 2016) and for in vivo protein labeling (Liu et al, 2016;Zhang et al, 2015). In summary, our γ2 pH FAP is the first protein-FAP conjugate characterized in primary neurons, providing a unique tool to monitor multistage GABA A R trafficking in living cells with relevance both for basic science research and applied pharmacology.…”

Section: Discussionmentioning

confidence: 99%

A versatile optical tool for studying synaptic GABAA receptor trafficking

Lorenz-Guertin

Wilcox

Zhang

et al. 2017

Journal of Cell Science

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Live-cell imaging methods can provide critical real-time receptor trafficking measurements. Here, we describe an optical tool to study synaptic γ-aminobutyric acid (GABA) type A receptor (GABAR) dynamics through adaptable fluorescent-tracking capabilities. A fluorogen-activating peptide (FAP) was genetically inserted into a GABAR γ2 subunit tagged with pH-sensitive green fluorescent protein (γ2FAP). The FAP selectively binds and activates Malachite Green (MG) dyes that are otherwise non-fluorescent in solution. γ2FAP GABARs are expressed at the cell surface in transfected cortical neurons, form synaptic clusters and do not perturb neuronal development. Electrophysiological studies show γ2FAP GABARs respond to GABA and exhibit positive modulation upon stimulation with the benzodiazepine diazepam. Imaging studies using γ2FAP-transfected neurons and MG dyes show time-dependent receptor accumulation into intracellular vesicles, revealing constitutive endosomal and lysosomal trafficking. Simultaneous analysis of synaptic, surface and lysosomal receptors using the γ2FAP-MG dye approach reveals enhanced GABAR turnover following a bicucculine-induced seizure paradigm, a finding not detected by standard surface receptor measurements. To our knowledge, this is the first application of the FAP-MG dye system in neurons, demonstrating the versatility to study nearly all phases of GABAR trafficking.

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“…In combination with polymeric materials, targeted biosensor have been developed to distinct subcellular structures within living cells 56 . More recently, Meng group 57 reported an injectable film by which antibodies can be localized in vivo . Their system builds upon a bifunctional polypeptide consisting of a FAP and a β -fibrillizing peptide ( β FP).…”

Section: The Application Of the Fap Technologymentioning

confidence: 99%

Fluorogen-activating proteins: beyond classical fluorescent proteins

2018

Acta Pharmaceutica Sinica B

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Fluorescence imaging is a powerful technique for the real-time noninvasive monitoring of protein dynamics. Recently, fluorogen activating proteins (FAPs)/fluorogen probes for protein imaging were developed. Unlike the traditional fluorescent proteins (FPs), FAPs do not fluoresce unless bound to their specific small-molecule fluorogens. When using FAPs/fluorogen probes, a washing step is not required for the removal of free probes from the cells, thus allowing rapid and specific detection of proteins in living cells with high signal-to-noise ratio. Furthermore, with different fluorogens, living cell multi-color proteins labeling system was developed. In this review, we describe about the discovery of FAPs, the design strategy of FAP fluorogens, the application of the FAP technology and the advances of FAP technology in protein labeling systems.

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Local retention of antibodies in vivo with an injectable film embedded with a fluorogen-activating protein

Cited by 16 publications

References 60 publications

Switching the Immunogenicity of Peptide Assemblies Using Surface Properties

Switching the Immunogenicity of Peptide Assemblies Using Surface Properties

A versatile optical tool for studying synaptic GABAA receptor trafficking

Fluorogen-activating proteins: beyond classical fluorescent proteins

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