Your search keyword '"Durst, Richard A."' showing total 6 results

1. Ganglioside-liposome immunoassay for the detection of botulinum toxin

Author

Ahn-Yoon, Soohyoun, DeCory, Thomas, Durst, Richard, Ahn-Yoon, Soohyoun, DeCory, Thomas, and Durst, Richard

Abstract

A rapid and highly sensitive receptor immunoassay for botulinum toxin (BT) has been developed using ganglioside-incorporated liposomes. Botulism outbreaks are relatively rare, but their results can be very severe, usually leading to death from respiratory failure. To exert their toxicity, the biological toxins must first bind to receptors on the cell surface, and the trisialoganglioside GT1b has been identified as the cell receptor for BT. Therefore, in this study, GT1b was used to prepare the ganglioside-liposomes by spontaneous insertion into the phospholipid bilayer. In a sandwich-based, hybrid receptor immunoassay, BT is detected as a colored band on a nitrocellulose membrane strip, where BT bound to the GT1b-liposomes are captured by anti-BT antibodies immobilized in a band across the strip. The intensity of the colored band can be visually estimated, or measured by densitometry using computer software. The limit of detection (LOD) for BT in the lateral-flow assay system was 15pgmL−1, which is comparable to the limits of detection achieved with the most sensitive assays previously reported. However, this rapid assay can be completed in less than 20min. These results demonstrate that the sandwich assay using GT1b-liposomes for detection of BT is rapid and very sensitive, suggesting the possibility for detecting BT in field screening, simply and reliably, without the need for complex instrumentation

Published

2018

2. Liposome encapsulation of fluorescent nanoparticles: Quantum dots and silica nanoparticles

Author

Chen, Chien-Sheng, Yao, Jie, Durst, Richard, Chen, Chien-Sheng, Yao, Jie, and Durst, Richard

Abstract

Quantum dots (QDs) and silica nanoparticles (SNs) are relatively new classes of fluorescent probes that overcome the limitations encountered by organic fluorophores in bioassay and biological imaging applications. We encapsulated QDs and SNs in liposomes and separated nanoparticle-loaded liposomes from unencapsulated nanoparticles by size exclusion chromatography. Fluorescence correlation spectroscopy was used to measure the average number of nanoparticles inside each liposome. Results indicated that nanoparticle-loaded liposomes were formed and separated from unencapsulated nanoparticles by using a Sepharose gel. As expected, fluorescence self-quenching of nanoparticles inside liposomes was not observed. Each liposome encapsulated an average of three QDs. These studies demonstrated that nanoparticles could be successfully encapsulated into liposomes and provided a methodology to quantify the number of nanoparticles inside each liposome by fluorescence correlation spectroscopy

Published

2018

3. A novel extraction method for peanut allergenic proteins in chocolate and their detection by a liposome-based lateral flow assay

Author

Wen, Hsiao-Wei, Borejsza-Wysocki, Wlodzimierz, DeCory, Thomas, Baeumner, Antje, Durst, Richard, Wen, Hsiao-Wei, Borejsza-Wysocki, Wlodzimierz, DeCory, Thomas, Baeumner, Antje, and Durst, Richard

Abstract

In this study, conditions for extracting the major peanut allergen (Ara h1) from chocolate were optimized, and the extracted samples were analyzed by a lateral flow assay (LFA) using liposomal nanovesicles. The optimal conditions using peanut-spiked chocolate were found to be extraction with a mixture of phosphate buffered saline and hexane for 30min at 35°C. After centrifugation, the buffer portion was treated with insoluble poly(vinylpolypyrrolidone) to remove phenolic compounds, and then analyzed by the LFA. The entire analysis, including sample preparation and LFA, could be easily completed within 2h, and the detection limit was 158μg of peanuts/g of chocolate

4. Development of a competitive liposome-based lateral flow assay for the rapid detection of the allergenic peanut protein Ara h1

Author

Wen, Hsiao-Wei, Borejsza-Wysocki, Wlodzimierz, DeCory, Thomas, Durst, Richard, Wen, Hsiao-Wei, Borejsza-Wysocki, Wlodzimierz, DeCory, Thomas, and Durst, Richard

Abstract

A competitive lateral flow assay for detecting the major peanut allergen, Ara h1, has been developed. The detector reagents are Ara h1-tagged liposomes, and the capture reagents are anti-Ara h1 polyclonal antibodies. Two types of rabbit polyclonal antibodies were raised either against the entire Ara h1 molecules (anti-Ara h1 Ab) or against an immunodominant epitope on Ara h1 (anti-peptide Ab). All of them reacted specifically with Ara h1 in Western Blot against crude peanut proteins. Moreover, the anti-Ara h1 Ab was chosen for this assay development because of its highest immunoactivity to Ara h1-tagged liposomes in the lateral flow assay. The calculated limit of detection (LOD) of this assay is 0.45μgmL−1 of Ara h1 with a dynamic range between 0.1 and 10μgmL−1 of Ara h1 in buffer. Additionally, the visually determined detection range is from 1 to 10μgmL−1 of Ara h1 in buffer. Results using this assay can be obtained within 30min without the need of sophisticated equipment or techniques; therefore, this lateral flow assay has the potential to be a cost-effective, fast, simple, and sensitive method for on-site screening of peanut allergens

5. Liposome encapsulation of fluorescent nanoparticles: Quantum dots and silica nanoparticles

Author

Chen, Chien-Sheng, Yao, Jie, Durst, Richard, Chen, Chien-Sheng, Yao, Jie, and Durst, Richard

Abstract

Quantum dots (QDs) and silica nanoparticles (SNs) are relatively new classes of fluorescent probes that overcome the limitations encountered by organic fluorophores in bioassay and biological imaging applications. We encapsulated QDs and SNs in liposomes and separated nanoparticle-loaded liposomes from unencapsulated nanoparticles by size exclusion chromatography. Fluorescence correlation spectroscopy was used to measure the average number of nanoparticles inside each liposome. Results indicated that nanoparticle-loaded liposomes were formed and separated from unencapsulated nanoparticles by using a Sepharose gel. As expected, fluorescence self-quenching of nanoparticles inside liposomes was not observed. Each liposome encapsulated an average of three QDs. These studies demonstrated that nanoparticles could be successfully encapsulated into liposomes and provided a methodology to quantify the number of nanoparticles inside each liposome by fluorescence correlation spectroscopy

6. Ganglioside-liposome immunoassay for the detection of botulinum toxin

Author

Ahn-Yoon, Soohyoun, DeCory, Thomas, Durst, Richard, Ahn-Yoon, Soohyoun, DeCory, Thomas, and Durst, Richard

Abstract

A rapid and highly sensitive receptor immunoassay for botulinum toxin (BT) has been developed using ganglioside-incorporated liposomes. Botulism outbreaks are relatively rare, but their results can be very severe, usually leading to death from respiratory failure. To exert their toxicity, the biological toxins must first bind to receptors on the cell surface, and the trisialoganglioside GT1b has been identified as the cell receptor for BT. Therefore, in this study, GT1b was used to prepare the ganglioside-liposomes by spontaneous insertion into the phospholipid bilayer. In a sandwich-based, hybrid receptor immunoassay, BT is detected as a colored band on a nitrocellulose membrane strip, where BT bound to the GT1b-liposomes are captured by anti-BT antibodies immobilized in a band across the strip. The intensity of the colored band can be visually estimated, or measured by densitometry using computer software. The limit of detection (LOD) for BT in the lateral-flow assay system was 15pgmL−1, which is comparable to the limits of detection achieved with the most sensitive assays previously reported. However, this rapid assay can be completed in less than 20min. These results demonstrate that the sandwich assay using GT1b-liposomes for detection of BT is rapid and very sensitive, suggesting the possibility for detecting BT in field screening, simply and reliably, without the need for complex instrumentation