Name: characterization of small bowel neuroendocrine tumor spheroids using immunofluorescence
Uploaded: 2025-04-28T12:09:56.000+00:00
Duration: 1 min 16 s
Description: Source: Ear, P. H., et. al. Establishment and Characterization of Small Bowel Neuroendocrine Tumor Spheroids. J. Vis. Exp. (2019)This video demonstrates ...

characterization of small bowel neuroendocrine tumor spheroids using immunofluorescence

Characterization of Small Bowel Neuroendocrine Tumor Spheroids Using Immunofluorescence

Fix the organoids by adding 500 microliters of paraformaldehyde and incubating them for 15 minutes. After the incubation, wash the culture twice with 1 milliliter of PBS. Add 500 microliters of PBS with 3% BSA and 0.1% Triton X-100 to permeabilize the culture. Incubate the tube for five minutes, then wash the organoids three times with 1 milliliter of PBS and 3% BSA.Next, incubate the culture with primary antibodies for one hour, then repeat the washes with PBS and BSA. Incubate with the secondary antibodies and repeat the washes, making sure to aspirate and discard all supernatant.To image the spheroids, add 5 microliters of mounting medium containing DAPI, and use a P20 pipette to transfer 5 microliters of the spheroids to a glass slide. Seal the slide with a cover slip, and image with a fluorescence microscope using the 10, 20, and 40 times objectives.

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1.&#160;Small bowel neuroendocrine tumor (SBNET) collection and cell dissociation<ol><li>Obtain resected patient SBNET samples after tumor tissue confirmation from the Surgical Pathology Core.</li><li>Cut SBNETs into 5 mm cubes and store them in 25 mL of Dulbecco's Modified Eagle Medium (DMEM)/F12 medium in a conical tube for transportation to the laboratory.</li><li>Transfer the tumors to DMEM containing 1% fetal bovine serum or FBS, 1% penicillin/streptomycin (Pen/Strep), and 1% glutamine (Wash Medium), and incubate in this Wash Medium for 15 min.</li><li>Transfer the tumors to a new dish and mince them into pieces less than 1 mm in diameter using sterile curved scissors.</li><li>Transfer the minced tissues to a new 50 mL tube containing 25 mL of Wash Medium.</li><li>Centrifuge the sample at 500 x&#160;g for 15 min at 4 &#176;C.</li><li>Discard the supernatant and resuspend the pellets in 10 mL of Wash Medium containing collagenase (100 U/mL) and DNase (0.1 mg/mL).</li><li>Allow the minced tumors to be digested in a 37 &#176;C incubator with slow shaking (50 rpm) for 1.5 h.</li></ol>2. Culture of SBNETs as tumor spheroids in Extra Cellular Matrix (ECM)<ol><li>After digestion is completed (step 1.8), centrifuge at 500 x&#160;g for 15 min at 4 &#176;C, discard the supernatant and resuspend the pellet in 15 mL of Wash Medium.</li><li>Place a 70 &#181;m cell strainer on top of a new 50 mL tube and transfer 10 mL of the Wash Medium over the cell strainer. Swirl the Wash Medium to cover the side of the plastic tube to prevent NET cells from sticking to the side of the plastic tube.</li><li>Filter the cell suspension through a cell strainer.</li><li>Centrifuge at 500 x&#160;g for 15 min at 4 &#176;C, discard the supernatant, resuspend the pellet in 200 &#181;L of Wash Medium (total volume is ~ 250 &#181;L), and place it on ice.</li><li>Transfer 5 &#181;L of cells to 500 &#181;L of Wash Medium (1/100 dilution factor). Use the diluted cells for cell counting using a hemocytometer to obtain the number of cells per milliliter. Multiply by 100 to correct for the dilution factor.</li><li>Multiply the number of cells per mL obtained in step 2.5 by the total volume of cells in suspension obtained in step 2.4 (~ 250 &#181;L).</li><li>Centrifuge at 500 x&#160;g for 15 min at 4 &#176;C, discard the supernatant, and resuspend the cells in liquid ECM (1 x 106&#160;cells/mL), and keep on ice.</li><li>Transfer 5-20 &#181;L of SBNET spheroids in ECM to a 96-well plate and allow the liquid ECM to solidify by placing the plate in a 37 &#176;C incubator for 5 min.</li><li>Add 200 &#181;L of SBNET culture medium (DMEM/F12 + 10% FBS + 1% PEN/STREP + 1% Glutamine + 10 mM nicotinamide + 10 &#181;g/mL insulin) to each well of the 96-well plate containing the SBNET spheroids in ECM.</li><li>Alternatively, culture SBNET organoids in stem cell media similar to what has previously been described for growing either human liver or pancreatic organoids and listed in the&#160;Table of Materials.</li><li>Change media every 5-7 days.</li></ol>3. Characterization of SBNETS spheroids by immunofluorescence<ol><li>Transfer the organoids grown in ECM to a 1.5 mL tube using a P1000 pipette.</li><li>Centrifuge at 1,500 x&#160;g for 1 min and remove the supernatant.</li><li>Wash the organoid culture by adding 1 mL of phosphate buffer saline or PBS, mix, centrifuge at 1,500 x&#160;g for 1 min and remove the supernatant.</li><li>Fix the organoids by adding 500 &#181;L of 4% paraformaldehyde and incubate for 15 min.</li><li>Wash the culture twice with 1 mL of PBS.</li><li>Permeabilize the culture by adding 500 &#181;L of PBS + 3% Bovine serum albumin or BSA + 0.1% Triton X 100 for 5 min.</li><li>Then, wash three times with 1 mL of PBS + 3% BSA.</li><li>Incubate for 1 h with primary antibodies against synaptophysin (SYP) at 1/600 dilution or chromogranin A (CgA) and somatostatin receptor 2 (SSTR2) at 1/400 dilution in antibody buffer (2.5% bovine serum albumin, 0.1% sodium azide, 25 mM Tris pH 7.4, 150 mM sodium chloride). &#160;NOTE: Use 300 &#181;L or more of antibody solution per tube.</li><li>Wash three times with 1 mL of PBS + 3% BSA.</li><li>Incubate with secondary antibodies coupled to FITC at 1/500 dilution in antibody buffer for 1 h. Use 300 &#181;L or more of antibody solution per tube.</li><li>Wash 3 times with 1 mL of PBS + 3% BSA. Make sure to aspirate and discard all the supernatant.</li><li>Add 5 &#181;L of mounting medium containing the nuclear stain DAPI.</li><li>Use a P20 pipette to transfer 5 &#181;L of the SBNET spheroids from step 4.12 to a glass slide and seal with a cover slip.</li><li>Take images using a fluorescent microscope using the 10x, 20x or 40x objectives.</li></ol>

<figure class='table' style='width:646pt;'><table class='ck-table-resized'><colgroup><col style='width:23.07%;'><col style='width:23.68%;'><col style='width:16.25%;'><col style='width:37%;'></colgroup><tbody><tr><td style='height:14.5pt;width:149pt;'>Anti-rabbit FITC</td><td style='width:153pt;'>Jackson ImmunoResearch</td><td style='width:105pt;'>11-095-152</td><td style='width:239pt;'>Secondary antibody couple to a green fluorophore</td></tr><tr><td style='height:14.5pt;width:149pt;'>Autostainer Link 48</td><td style='width:153pt;'>Agilent Dako</td><td style='width:105pt;'>Not Available</td><td style='width:239pt;'>Automated system for antibody staining</td></tr><tr><td style='height:14.5pt;width:149pt;'>Cell freezing container</td><td style='width:153pt;'>Thermo Scientific</td><td style='width:105pt;'>5100-0001</td><td style='width:239pt;'>Container to for freezing cells</td></tr><tr><td style='height:14.5pt;width:149pt;'>CellSence</td><td style='width:153pt;'>Olympus</td><td style='width:105pt;'>Version 1.18</td><td style='width:239pt;'>Computer software for using fluorescent microscope</td></tr><tr><td style='height:14.5pt;width:149pt;'>Chromogranin A antibody</td><td style='width:153pt;'>Abcam-45179</td><td style='width:105pt;'>RB-9003-PO</td><td style='width:239pt;'>Antibodies for IF</td></tr><tr><td style='height:14.5pt;width:149pt;'>Collagenase</td><td style='width:153pt;'>Sigma</td><td style='width:105pt;'>C0130</td><td style='width:239pt;'>Enzyme for digesting tumor tissue</td></tr><tr><td style='height:14.5pt;width:149pt;'>DMEM</td><td style='width:153pt;'>Gibco</td><td style='width:105pt;'>11965-092</td><td style='width:239pt;'>Medium for tissue preparation</td></tr><tr><td style='height:14.5pt;width:149pt;'>DMEM/F12</td><td style='width:153pt;'>Gibco</td><td style='width:105pt;'>11320-033</td><td style='width:239pt;'>Medium for organoid cultures</td></tr><tr><td style='height:14.5pt;width:149pt;'>DNAse</td><td style='width:153pt;'>Sigma</td><td style='width:105pt;'>DN25</td><td style='width:239pt;'>Enzyme for digesting tumor tissue</td></tr><tr><td style='height:14.5pt;width:149pt;'>FBS</td><td style='width:153pt;'>Gibco</td><td style='width:105pt;'>16000044</td><td style='width:239pt;'>Reagent for culture media</td></tr><tr><td style='height:14.5pt;width:149pt;'>Fluorescent microscope</td><td style='width:153pt;'>Olympus</td><td style='width:105pt;'>CKX35</td><td style='width:239pt;'>Microscope for taking pictures of SBENT spheroids</td></tr><tr><td style='height:14.5pt;width:149pt;'>Glutamine</td><td style='width:153pt;'>Gibco</td><td style='width:105pt;'>A2916801</td><td style='width:239pt;'>Reagent for culture media</td></tr><tr><td style='height:14.5pt;width:149pt;'>Insulin</td><td style='width:153pt;'>Sigma</td><td style='width:105pt;'>I0516</td><td style='width:239pt;'>Reagent for culture media</td></tr><tr><td style='height:14.5pt;width:149pt;'>Matrigel</td><td style='width:153pt;'>Corning</td><td style='width:105pt;'>356235</td><td style='width:239pt;'>Matrix to embed and anchore organoids</td></tr><tr><td style='height:15.75pt;width:149pt;'>Mounting medium (VECTASHIELD)</td><td style='width:153pt;'>Vector Laboratories</td><td style='width:105pt;'>H-1200</td><td style='width:239pt;'>Fixative for labelled-cells with a nuclear stain</td></tr><tr><td style='height:15.75pt;width:149pt;'>Nicotinamide</td><td style='width:153pt;'>Sigma</td><td style='width:105pt;'>72340</td><td style='width:239pt;'>Reagent for culture media</td></tr><tr><td style='height:15.75pt;width:149pt;'>Paraformaldehyde</td><td style='width:153pt;'>Electron Microscopy Sciences</td><td style='width:105pt;'>15710</td><td style='width:239pt;'>Reagent to fix cells</td></tr><tr><td style='height:15.75pt;width:149pt;'>PEN/STREP</td><td style='width:153pt;'>Gibco</td><td style='width:105pt;'>15140-122</td><td style='width:239pt;'>Reagent for culture media</td></tr><tr><td style='height:15.75pt;width:149pt;'>SSTR2 antibody</td><td style='width:153pt;'>GeneScritp</td><td style='width:105pt;'>A01591</td><td style='width:239pt;'>Antibodies for IF</td></tr><tr><td style='height:15.75pt;width:149pt;'>Synaptophysin antibody</td><td style='width:153pt;'>Abcam</td><td style='width:105pt;'>32127</td><td style='width:239pt;'>Antibodies for IF</td></tr><tr><td style='height:15.75pt;width:149pt;'>TritonX</td><td style='width:153pt;'>Mallinckrodt</td><td style='width:105pt;'>3555 KBGE</td><td style='width:239pt;'>Reagent to permeablize cells</td></tr><tr><td style='height:15.75pt;width:149pt;'>Y-2763 ROCK inhibitor</td><td style='width:153pt;'>Adipogen</td><td style='width:105pt;'>AG-CR1-3564-M005</td><td style='width:239pt;'>To improve SBNET spheroid viability after freeze thaw</td></tr></tbody></table></figure>

<a href='https://app.jove.com/v/60303/establishment-characterization-small-bowel-neuroendocrine-tumor'>Source: Ear, P. H., et. al. Establishment and Characterization of Small Bowel Neuroendocrine Tumor Spheroids. J. Vis. Exp. (2019)</a>This video demonstrates the immunofluorescence staining of small bowel neuroendocrine tumor spheroids. The spheroids are fixed, permeabilized, and blocked and are then incubated with primary and secondary antibodies. A dye is added to stain nuclei before mounting and visualizing them under a fluorescent microscope.

Source: Ear, P. H., et. al. Establishment and Characterization of Small Bowel Neuroendocrine Tumor Spheroids. J. Vis. Exp. (2019)This video demonstrates ...

Take small bowel neuroendocrine tumor spheroids in a tube.Add a fixative solution to preserve the cells.&#160;To wash, centrifuge, and replace the fixative with buffer.Centrifuge and discard the supernatant to remove any remaining fixative.Add a buffer containing detergent and a blocking agent to permeabilize the cellular membranes and prevent non-specific antibody binding.Wash with buffer to remove excess detergent and blocking agent.Incubate with primary antibodies, which bind to the target protein specific to the neuroendocrine cell.Wash with buffer to remove unbound antibodies.Add fluorophore-tagged secondary antibodies that bind to the primary antibodies.Rinse with buffer to remove excess antibodies.Add a mounting medium containing a dye to stain the nucleus.Transfer the spheroids onto a slide and mount with a cover slip.Use a Fluorescence microscope to visualize neuroendocrine cells of the spheroid expressing specific proteins.

4 vistas. Characterization of Small Bowel Neuroendocrine Tumor Spheroids Using Immunofluorescence

Video: Characterization of Small Bowel Neuroendocrine Tumor Spheroids Using Immunofluorescence - Experimento

Generation of High-Throughput Three-Dimensional Tumor Spheroids for Drug Screening

Cancer cells have routinely been cultured in two dimensions (2D) on a plastic surface. This technique, however, lacks the true environment a tumor mass is exposed to in vivo. Solid tumors grow not as a sheet attached to plastic, but instead as a collection of clonal cells in a three-dimensional (3D) space interacting with their neighbors, and with distinct spatial properties such as the disruption of normal cellular polarity. These interactions cause 3D-cultured cells to acquire morphological and cellular characteristics which are more relevant to in vivo tumors. Additionally, a tumor mass is in direct contact with other cell types such as stromal and immune cells, as well as the extracellular matrix from all other cell types. The matrix deposited is comprised of macromolecules such as collagen and fibronectin.
In an attempt to increase the translation of research findings in oncology from bench to bedside, many groups have started to investigate the use of 3D model systems in their drug development strategies. These systems are thought to be more physiologically relevant because they attempt to recapitulate the complex and heterogeneous environment of a tumor. These systems, however, can be quite complex, and, although amenable to growth in 96-well formats, and some now even in 384, they offer few choices for large-scale growth and screening. This observed gap has led to the development of the methods described here in detail to culture tumor spheroids in a high-throughput capacity in 1536-well plates. These methods represent a compromise to the highly complex matrix-based systems, which are difficult to screen, and conventional 2D assays. A variety of cancer cell lines harboring different genetic mutations are successfully screened, examining compound efficacy by using a curated library of compounds targeting the Mitogen-Activated Protein Kinase or MAPK pathway. The spheroid culture responses are then compared to the response of cells grown in 2D, and differential activities are reported. These methods provide a unique protocol for testing compound activity in a high-throughput 3D setting.

Across a wide variety of disease indications, more physiologically relevant models are being developed and implemented into drug discovery programs. The new model system described here demonstrates how three-dimensional tumor spheroids can be cultured and screened in a high-throughput 1536-well plate-based system to search for new oncology drugs.

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Investigación

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Investigación sobre el cáncer

Physiologic Patient Derived 3D Spheroids for Anti-neoplastic Drug Screening to Target Cancer Stem Cells

In this protocol, we outline the procedure for generation of tumor spheroids within 384-well hanging droplets to allow for high-throughput screening of anti-cancer therapeutics in a physiologically representative microenvironment. We outline the formation of patient derived cancer stem cell spheroids, as well as, the manipulation of these spheroids for thorough analysis following drug treatment. Specifically, we describe collection of spheroid morphology, proliferation, viability, drug toxicity, cell phenotype and cell localization data. This protocol focuses heavily on analysis techniques that are easily implemented using the 384-well hanging drop platform, making it ideal for high throughput drug screening. While we emphasize the importance of this model in ovarian cancer studies and cancer stem cell research, the 384-well platform is amenable to research of other cancer types and disease models, extending the utility of the platform to many fields. By improving the speed of personalized drug screening and the quality of screening results through easily implemented physiologically representative 3D cultures, this platform is predicted to aid in the development of new therapeutics and patient-specific treatment strategies, and thus have wide-reaching clinical impact.

This protocol describes generation of patient-derived spheroids, and downstream analysis including quantification of proliferation, cytotoxicity testing, flow cytometry, immunofluorescence staining and confocal imaging, in order to assess drug candidates&#8217; potential as anti-neoplastic therapeutics. This protocol supports precision medicine with identification of specific drugs for each patient and stage of disease.

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Establishing 3-Dimensional Spheroids from Patient-Derived Tumor Samples and Evaluating their Sensitivity to Drugs

Despite remarkable advances in understanding tumor biology, the vast majority of oncology drug candidates entering clinical trials fail, often due to a lack of clinical efficacy. This high failure rate illuminates the inability of the current preclinical models to predict clinical efficacy, mainly due to their inadequacy in reflecting tumor heterogeneity and the tumor microenvironment. These limitations can be addressed with 3-dimensional (3D) culture models (spheroids) established from human tumor samples derived from individual patients. These 3D cultures represent real-world biology better than established cell lines that do not reflect tumor heterogeneity. Furthermore, 3D cultures are better than 2-dimensional (2D) culture models (monolayer structures) since they replicate elements of the tumor environment, such as hypoxia, necrosis, and cell adhesion, and preserve the natural cell shape and growth. In the present study, a method was developed for preparing primary cultures of cancer cells from individual patients that are 3D and grow in multicellular spheroids. The cells can be derived directly from patient tumors or patient-derived xenografts. The method is widely applicable to solid tumors (e.g., colon, breast, and lung) and is also cost-effective, as it can be performed in its entirety in a typical cancer research/cell biology lab without relying on specialized equipment. Herein, a protocol is presented for generating 3D tumor culture models (multicellular spheroids) from primary cancer cells and evaluating their sensitivity to drugs using two complementary approaches: a cell-viability assay (MTT) and microscopic examinations. These multicellular spheroids can be used to assess potential drug candidates, identify potential biomarkers or therapeutic targets, and investigate the mechanisms of response and resistance.

The present protocol describes generating 3D tumor culture models from primary cancer cells and evaluating their sensitivity to drugs using cell-viability assays and microscopic examinations.

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Characterization of Small Bowel Neuroendocrine Tumor Spheroids Using Immunofluorescence

Transcripción

Characterization of Small Bowel Neuroendocrine Tumor Spheroids Using Immunofluorescence