Name: 视频: 使用暗场显微镜进行抗体偶联纳米颗粒定量:从体液中捕获和定量特定外泌体的程序 - 概念
Uploaded: 2023-04-30T13:43:25.000+00:00
Duration: 1 min 44 s
Description: 1.1K 次观看. 来源:Wan， M. et al.使用纳米等离子体增强散射和低放大倍率显微镜成像来量化肿瘤衍生的外泌体。J. Vis. Exp.（2019 年） 该视频介绍了如何使用低放大倍率、暗场显微镜来定量小体积生物流体样品中的特定外泌体。这样鉴定的外泌体可以作为潜在的癌症生物标志物。

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1. Preparation of Nanoparticle Probes
NOTE: This assay utilizes Functionalized Gold Nanorods (AuNRs; 25 nm diameter x 71 nm length) that are covalently conjugated with neutravidin polymers (AV) and have a surface plasmon resonance peak that produces a red (641 nm peak) scattering signal upon DFM illumination.
<ol>
	<li>Wash 40 &#181;L of AuNR-AV (2.56 x 1011&#160;particles) three times with 200 &#181;L PBS (pH 7.0) by centrifugation and aspiration (8,500 x&#160;g&#160;at 4 &#176;C for 10 minutes), followed by a final centrifugation and aspiration step after which the AuNR-AV pellet is suspended in 40 &#181;L PBS.</li>
	<li>Mix this AuNR-AV suspension with 10 &#181;L biotinylated antibody (0.5 mg/mL) specific for an antigen on the surface of the exosome subtype of interest and 150 &#181;L of PBS and then mix at 4 &#176;C for 2 h using a mixer to allow neutravidin-biotin binding to reach completion.</li>
	<li>Wash the resulting antibody-conjugated AuNRs (AuNR-IgG) three times by centrifugation and aspiration (6,500 x&#160;g&#160;at 4 &#176;C for 10 minutes) and then suspend them in 200 &#181;L PBS and store them at 4 &#176;C until use. 
	NOTE: Sterile technique and short storage times must be used to avoid contamination and degradation of the AuNR-IgG. It is best to use antibody-conjugated AuNRs within 24 hours of their conjugation.</li>
</ol>
2. Preparation of EV Capture Slides
<ol>
	<li>Dilute selected exosome capture antibodies to 0.025 mg/mL in PBS and add 1 &#181;L/well of this dilution onto a multi-well protein A/G slide and then incubate this slide at 37 &#176;C for 1 h in a humidified chamber to allow capture antibody binding to protein A/G immobilized on the slide.</li>
	<li>Aspirate wells to remove unbound antibodies and wash them three times by the addition and aspiration of 1 &#181;L/well of PBS. Then, load each well with 1 &#181;L of blocking buffer (see&#160;Table of Materials) and incubate the slide for 2 h at 37 &#176;C in a humidified chamber to block any remaining protein binding sites.</li>
	<li>Aspirate wells to remove blocking buffer, wash wells three times by the addition and aspiration of 1 &#181;L/well of PBS, and immediately use the blocked slides for exosome capture and analysis.</li>
</ol>
3. Standard Curve Preparation
<ol>
	<li>To accurately quantify the absolute or relative abundance of a specific exosome subtype, the user must generate a standard curve with a pure exosome population that uniformly expresses the exosome surface biomarker of interest. This study analyses the abundance of exosomes expressing a metastasis-associated membrane protein, Ephrin A2 receptor, which has a reported relationship with pancreatic cancer stage and prognosis. 
	NOTE: The human pancreatic cancer cell line PANC-1 and its exosomes are known to express this protein and isolated exosomes from this cell line were used to generate a standard curve to quantify the number of exosomes that express this protein in complex exosome samples.</li>
	<li>Culture cells for 48 hours at 37 &#176;C in serum-free culture media to allow exosome accumulation in the media, then isolate cell culture supernatants by centrifugation of suspension cultures or direct aspiration of culture media from adherent cell cultures.</li>
	<li>Centrifuge the collected media at 2000 x&#160;g&#160;for 30 min to remove debris and recover the supernatant.</li>
	<li>Filter the clarified culture supernatant through a 0.45 &#181;m low protein binding filter unit of appropriate capacity (e.g., a 250 mL polyether sulfone vacuum filtration unit).</li>
	<li>Concentrate the resulting filtrate by centrifugation at 3200 x&#160;g&#160;using a 100,000 nominal molecular weight limit filter system to a 250 &#181;L final volume. Collect the retained volume from this filter, then wash the filter with 200 &#181;L PBS, and combine this wash volume with the collected exosome sample volume.</li>
	<li>Centrifuge this sample at 21,000 x&#160;g&#160;for 45 minutes and carefully recover the supernatant, taking care not to collect any precipitated material.</li>
	<li>Centrifuge the recovered supernatant at 100,000 x&#160;g&#160;for 3 hours to precipitate the exosomes. Aspirate away the supernatant and collect the exosome pellet in 100 &#181;L PBS.</li>
	<li>Store the resulting exosome suspensions at 4 &#176;C if used within 24 hours or at -80 &#176;C for long-term storage. 
	NOTE: Do not subject exosome samples to repeat freeze-thaw cycles.</li>
	<li>Quantify an aliquot of the exosome suspension after mixing by direct measurement of exosome numbers (e.g., by nanoparticle tracking analysis or tuneable resistive pulse sensing or by measuring the protein concentration of exosome lysates by micro-bicinchoninic acid assay, or an equivalent method, as a means to approximate exosome quantity).</li>
	<li>Generate a set of serial dilutions of the exosome suspension to allow comparison of nanoparticle signal to input exosome number or protein content.</li>
	<li>Transfer 1 &#181;L of each exosome standard to each of its replicate wells on the assay plate. 
	NOTE: Standard curves can be used to calculate the slope of the correlation line between nanoparticle signal and exosome concentration to (1) evaluate assay performance and (2) determine the relative concentration of target exosomes in experimental samples.</li>
</ol>
4. Processing Human Plasma or Serum Samples
<ol>
	<li>Collect plasma or serum samples by standard methods and store at -80 &#176;C until needed for exosome analysis. Rapidly thaw samples in a room temperature water bath. Repeatedly mix the thawed samples by inversion to promote homogenous suspension. 
	NOTE: Results from serum and plasma samples may not be equivalent since there is a significant release of exosomes during the clotting reaction.</li>
	<li>Centrifuge plasma or serum samples at 500 x g for 15 min to precipitate protein aggregates and other debris. Transfer an aliquot of the plasma or serum sample to a fresh tube and add PBS to generate a 1:1 dilution. Mix the diluted sample by gentle vortexing or inversion, as appropriate. Transfer 1 &#181;L of each plasma or serum suspension to each of its replicate wells on the assay plate.</li>
</ol>
5. Exosome Capture and Detection
<ol>
	<li>Load wells of a blocked EV capture slide with 1 &#181;L/well of exosome sample, using 8 replicates per sample, and incubate the slide overnight at 4 &#176;C in a humidified chamber. Aspirate all sample wells and then add 1 &#181;L/well of PBS to wash wells and remove unbound exosomes and other contaminants from the loaded exosome sample.</li>
	<li>Load sample wells with 1 &#181;L/well of a previously prepared AuNR-IgG suspension (see section 1 above) and incubate the slide for 2 h at 37 &#176;C in a humidified chamber. Aspirate the nanoparticle solution and wash the slide in PBS supplemented with 0.01% Tween-20 (PBST) for 10 min using a mixer, then aspirate and wash all sample wells with deionized water for 10 min using a rotating mixer and air-dry for subsequent LMDFM imagery. 
	NOTE: Inter-assay coefficients of variation (CVs) are assessed from eight replicates of the same sample. Samples that exhibit CVs &#62;20% are considered non-informative and should be repeated, if there is sufficient sample.</li>
</ol>

<table><tbody><tr><td>Eppendorf Repeater stream</td><td>Fisher Scientific</td><td>05-401-040</td><td></td></tr><tr><td>Eppendorf Research plus</td><td>Eppendorf</td><td>3120000011</td><td>0.1 &amp;ndash; 2.5 &amp;micro;L, dark gray</td></tr><tr><td>Functionalized Gold Nanorods</td><td>Nanopartz</td><td>C12-25-650-TN-DIH-50-1</td><td>In vitro neutravidin polymer&lt;br/&gt; functionalization</td></tr><tr><td>HulaMixer Sample Mixer</td><td>Thermo Fisher Scientific</td><td>15920D</td><td></td></tr><tr><td>Incu-shaker 10L</td><td>Benchmark Scientific</td><td>H1010</td><td></td></tr><tr><td>Inverted Research Microscope</td><td>Nikon</td><td>Ti-DH</td><td>With Dark field condenser, DS-Ri2&lt;br/&gt; camera, and Ti-SH-U universal&lt;br/&gt; holder, and motorized stage</td></tr><tr><td>NIS-Elements</td><td>Nikon</td><td></td><td>Microscope imaging software</td></tr><tr><td>Phosphate Buffered Saline (1X)</td><td>GE Healthcare Life Sciences</td><td>SH30256.02</td><td>HyClone</td></tr><tr><td>Protein A/G Treated Glass&lt;br/&gt; Substrate Slides</td><td>Arrayit Corp.</td><td>AGMSM192BC</td><td>Premium microarray substrate</td></tr><tr><td>Q500 Sonicator</td><td>Qsonica, LLC</td><td>Q500-110</td><td>With standard probe (#4220)</td></tr><tr><td>Superblock blocking buffer</td><td>Thermo Scientific</td><td></td><td></td></tr><tr><td>TWEEN 20</td><td>Sigma Life Sciences</td><td>9005-64-5</td><td></td></tr></tbody></table>

antibody conjugated nanoparticle-based quantification using dark field microscopy: a procedure to capture and quantify specific exosomes from body fluids

Source: Wan, M. et al. <a href="https://www.jove.com/video/59177" target="_blank">Using Nanoplasmon-Enhanced Scattering and Low-Magnification Microscope Imaging to Quantify Tumor-Derived Exosomes.</a> J. Vis. Exp. (2019)
This video describes the use of low-magnification, dark-field microscopy to quantify specific exosomes in small volume biofluidic samples. The exosomes thus identified can serve as potential cancer biomarkers.

Antibody Conjugated Nanoparticle-based Quantification Using Dark Field Microscopy: A Procedure to Capture and Quantify Specific Exosomes from Body Fluids

Source: Wan, M. et al. Using Nanoplasmon-Enhanced Scattering and Low-Magnification Microscope Imaging to Quantify Tumor-Derived Exosomes. J. Vis. Exp. ...

Exosomes are small, membrane-enclosed structures that are secreted by the cells into the extracellular space. Exosomes are abundantly present in biofluids.
To identify and capture specific exosomes from body fluids, begin by taking a multi-well immunoassay slide. This slide is functionalized with proteins that act as antigens and bind to specific antibodies.&#160;
Supplement the slide with the desired primary antibody solution and incubate. These antibodies bind to the pre-coated antigens on the slide surface.
Aspirate the remaining solution to remove any unbound antibodies. Now, add a blocking buffer that blocks the free antigens, thereby preventing the nonspecific binding of exosomes.
Then, remove the blocking buffer, load the exosomes containing serum suspension onto the slide, and incubate. This allows the exclusive binding of target-specific exosomes to the captured primary antibodies.
Next, load a suspension of gold nanoparticle conjugated secondary antibodies onto the slide surface. These antibodies attach to the pre-bound exosomes and form a detection complex.
Finally, using a pipette, discard any unbound secondary antibodies. Visualize the slides under a dark-field microscope. Gold nanoparticles present on the surface of exosomes scatter light and appear as bright spots against the dark background.&#160;&#160;

antibody-conjugated-nanoparticle-based-quantification-using-dark

Research

JoVE Encyclopedia of Experiments

Cancer Research

Head and Neck Cancer

Assays & techniques

1.1K 次观看. 来源:Wan， M. et al.使用纳米等离子体增强散射和低放大倍率显微镜成像来量化肿瘤衍生的外泌体。J. Vis. Exp.（2019 年） 该视频介绍了如何使用低放大倍率、暗场显微镜来定量小体积生物流体样品中的特定外泌体。这样鉴定的外泌体可以作为潜在的癌症生物标志物。 

视频: 使用暗场显微镜进行抗体偶联纳米颗粒定量:从体液中捕获和定量特定外泌体的程序 - 概念

Rapid Fluorescence-based Characterization of Single Extracellular Vesicles in Human Blood with Nanoparticle-tracking Analysis

Extracellular vesicles (EVs), including exosomes, are specialized membranous nano-sized vesicles found in bodily fluids that are constitutively released from many cell types and play a pivotal role in regulating cell-cell communication and a diverse range of biological processes. Many different methods for the characterization of EVs have been described. However, most of these methods have the disadvantage that the preparation and characterization of the samples are very time-consuming, or it is extremely difficult to analyze specific markers of interest due to their small size and due to the lack of discrete populations. While methods for analysis of EVs have been considerably improved over the last decade, there is still no standardized method for characterization of single EVs. Here, we demonstrate a semi-automated method for characterization of single EVs by fluorescence-based nanoparticle-tracking analysis. The protocol that is presented addresses the common problem of many researchers in this field and provides the complete workflow for rapid isolation of EVs and characterization with PKH67, a general cell membrane linker, as well as with specific surface markers such as CD63, CD9, vimentin, and lysosomal-associated membrane protein 1 (LAMP-1). The presented results show a high level of reproducibility, as confirmed by other methods, such as Western blotting. In the conducted experiments, we exclusively used EVs isolated from human serum samples, but this method is also suitable for plasma or other body fluids and can be adjusted for characterization of EVs from cell culture supernatants. Irrespective of the future progress of research on EV biology, the protocol that is presented here provides a rapid and reliable method for rapid characterization of single EVs with specific markers.

In this protocol, we describe the complete workflow for rapid isolation of extracellular vesicles from human whole blood and characterization of specific markers by fluorescence-based nanoparticle-tracking analysis. The presented results show a high level of reproducibility and can be adjusted to cell culture supernatants.

基于荧光的人体血液单细胞外囊快速表征

Extracellular vesicles (EVs), including exosomes, are specialized membranous nano-sized vesicles found in bodily fluids that are constitutively released ...

科研

JoVE Journal

生物化学

Rapid Nanoprobe Signal Enhancement by In Situ Gold Nanoparticle Synthesis

The use of nanoprobes such as gold, silver, silica or iron-oxide nanoparticles as detection reagents in bioanalytical assays can enable high sensitivity and convenient colorimetric readout. However, high densities of nanoparticles are typically needed for detection. The available synthesis-based enhancement protocols are either limited to gold and silver nanoparticles or rely on precise enzymatic control and optimization. Here, we present a protocol to enhance the colorimetric readout of gold, silver, silica, and iron oxide nanoprobes. It was observed that the colorimetric signal can be improved by up to a 10000-fold factor. The basis for such signal enhancement strategies is the chemical reduction of Au3+ to Au0. There are several chemical reactions that enable the reduction of Au3+ to Au0. In the protocol, Good&#39;s buffers and H2O2 are used and it is possible to favor the deposition of Au0 onto the surface of existing nanoprobes, in detriment of the formation of new gold nanoparticles. The protocol consists of the incubation of the microarray with a solution consisting of chloroauric acid and H2O2 in 2-(N-morpholino)ethanesulfonic acid pH 6 buffer following the nanoprobe-based detection assay. The enhancement solution can be applied to paper and glass-based sensors. Moreover, it can be used in commercially available immunoassays as demonstrated by the application of the method to a commercial allergen microarray. The signal development requires less than 5 min of incubation with the enhancement solution and the readout can be assessed by naked eye or low-end image acquisition devices such as a table-top scanner or a digital camera.

Rapid Nanoprobe Signal Enhancement by In Situ Gold Nanoparticle Synthesis

In this work, a protocol for signal enhancement of nanoprobe-based biosensing is presented. The protocol is based on the reduction of chloroauric acid onto the surface of existing nanoprobes that consist of gold, silver, silica or iron-oxide nanoparticles.

原位金纳米粒子合成快速 Nanoprobe 信号增强

The use of nanoprobes such as gold, silver, silica or iron-oxide nanoparticles as detection reagents in bioanalytical assays can enable high sensitivity ...

化学

Visualizing Diffusional Dynamics of Gold Nanorods on Cell Membrane using Single Nanoparticle Darkfield Microscopy

Analyzing the diffusional dynamics of nanoparticles on cell membrane plays a significant role in better understanding the cellular uptake process and provides a theoretical basis for the rational design of nano-medicine delivery. Single particle tracking (SPT) analysis could probe the position and orientation of individual nanoparticles on cell membrane, and reveal their translational and rotational states. Here, we show how to use traditional dark-field microscopy to monitor the dynamics of gold nanorods (AuNRs) on live cell membrane. We also show how to extract the location and orientation of AuNRs using ImageJ and MATLAB, and how to characterize the diffusive states of AuNRs. Statistical analysis of hundreds of particles show that single AuNRs perform Brownian motion on the surface of U87 MG cell membrane. However, individual long trajectory analysis shows that AuNRs have two distinctly different types of motion states on the membrane, namely long-range transport and limited-area confinement. Our SPT methods can be potentially used to study the surface or intracellular particle diffusion in different biological cells and can become a powerful tool for investigations of complex cellular mechanisms.

Here, we show the use of traditional dark-field microscopy to monitor the dynamics of gold nanorods (AuNRs) on cell membrane. The location and orientation of single AuNRs are detected using ImageJ and MATLAB, and the diffusive states of AuNRs are characterized by single particle tracking analysis.

使用单纳米粒子暗场显微镜可视化细胞膜上金纳米棒的扩散动力学

Analyzing the diffusional dynamics of nanoparticles on cell membrane plays a significant role in better understanding the cellular uptake process and ...

Antibody Conjugated Nanoparticle-based Quantification Using Dark Field Microscopy: A Procedure to Capture and Quantify Specific Exosomes from Body Fluids

成績單

Antibody Conjugated Nanoparticle-based Quantification Using Dark Field Microscopy: A Procedure to Capture and Quantify Specific Exosomes from Body Fluids