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In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

The present protocol describes methods for evaluating DNA damage repair proteins in patient-derived ovarian cancer organoids. Included here are comprehensive plating and staining methods, as well as detailed, objective quantification procedures.

Abstract

Immunofluorescence is one of the most widely used techniques to visualize target antigens with high sensitivity and specificity, allowing for the accurate identification and localization of proteins, glycans, and small molecules. While this technique is well-established in two-dimensional (2D) cell culture, less is known about its use in three-dimensional (3D) cell models. Ovarian cancer organoids are 3D tumor models that recapitulate tumor cell clonal heterogeneity, the tumor microenvironment, and cell-cell and cell-matrix interactions. Thus, they are superior to cell lines for the evaluation of drug sensitivity and functional biomarkers. Therefore, the ability to utilize immunofluorescence on primary ovarian cancer organoids is extremely beneficial in understanding the biology of this cancer. The current study describes the technique of immunofluorescence to detect DNA damage repair proteins in high-grade serous patient-derived ovarian cancer organoids (PDOs). After exposing the PDOs to ionizing radiation, immunofluorescence is performed on intact organoids to evaluate nuclear proteins as foci. Images are collected using z-stack imaging on confocal microscopy and analyzed using automated foci counting software. The described methods allow for the analysis of temporal and special recruitment of DNA damage repair proteins and colocalization of these proteins with cell-cycle markers.

Introduction

Ovarian cancer is the leading cause of death due to gynecologic malignancy. The majority of patients are treated with DNA-damaging drugs such as carboplatin, and those with homologous recombination repair (HRR)-deficient tumors can be given poly (ADP-ribose) polymerase (PARP) inhibitors1,2. However, most patients develop resistance to these therapies and die within 5 years of diagnosis. Dysregulation of the DNA damage response (DDR) has been associated with the development of ovarian cancer and both chemotherapy and PARP inhibitor resistance3. Thus, study of the DDR is imperative in understanding the pathophysiology of ovarian cancer, potential biomarkers, and novel targeted therapies.

Current methods to evaluate the DDR utilize immunofluorescence (IF), as this allows for the accurate identification and localization of DNA damage proteins and nucleotide analogs. Once there is a double-stranded break (DSB) in the DNA, the histone protein H2AX is rapidly phosphorylated, forming a focus where DNA damage repair proteins congregate4. This phosphorylation can be easily identified utilizing IF; in fact, the ɣ-H2AX assay has commonly been employed to confirm the induction of a DSB5,6,7,8,9. Increased DNA damage has been associated with platinum sensitivity and efficacy of DNA damaging agents10,11,12, and ɣ-H2AX has been proposed as a biomarker associated with chemotherapy response in other cancer treatments13. Upon a DSB, a cell proficient in HRR performs a series of events that leads to BRCA1 and BRCA2 recruiting RAD51 to replace replication protein A (RPA) and bind to the DNA. HRR repair uses a DNA template to faithfully repair the DSB. However, when tumors are deficient in HRR, they rely on alternative repair pathways such as non-homologous end joining (NHEJ). NHEJ is known to be error-prone and creates a high mutational burden on the cell, which uses 53BP1 as a positive regulator14. These DNA damage proteins can all be accurately identified as foci using IF. In addition to staining for proteins, IF can be used to study fork protection and single-stranded DNA gap formation. The ability to have stable forks has been correlated with platinum response, and recently, gap assays have shown the potential to predict the response to PARP inhibitors6,15,16,17. Therefore, staining for the nucleotide analogs after introduction into the genome is another way to study the DDR.

To date, evaluation of the DDR in ovarian cancer has been largely limited to homogenous 2D cell lines that do not recapitulate the clonal heterogeneity, microenvironment, or architecture of in vivo tumors18,19. Recent research suggests organoids are superior to 2D cell lines in studying complex biologic processes such as DDR mechanisms6. The present methodology evaluates RAD51, ɣ-H2AX, 53BP1, RPA, and geminin in PDOs. These methods assess the intact organoid and allow for the study of DDR mechanisms in a setting more similar to the in vivo tumor microenvironment. Together with confocal microscopy and automated foci counting, this methodology can aid in understanding the DDR pathway in ovarian cancer and personalizing treatment plans for patients.

Protocol

Tumor tissue and ascites were obtained after obtaining patient consent as part of a gynecologic oncology biorepository that was approved by the Washington University in St. Louis Institutional Review Board (IRB). Patients were included if they had advanced stage high-grade serous ovarian cancer (HGSOC). All procedures were performed at room temperature on the bench unless otherwise specified. All reagents were prepared at room temperature (unless otherwise indicated) and stored at 4 °C.

1. Organoid generation

  1. Generate the organoids following the previously published report20.

2. Plating and irradiation of organoids

  1. Using organoids in culture, dislodge the tabs of the organoids from the culture dish through manual manipulation of a pipette tip. Collect the organoids in a 15 mL conical tube.
  2. Centrifuge the conical tube at 1,650 x g for 5 min at 4 °C. Using a pipette, aspirate off the supernatant carefully.
  3. Add 1,000 µL of an animal origin-free, recombinant enzyme to the pellet (see Table of Materials). Mix the solution and incubate for 15 min at 37 °C.
  4. Centrifuge the solution at 1,650 x g for 5 min at 4 °C. Using a pipette, carefully aspirate off the supernatant.
  5. After centrifugation and aspiration, resuspend the pellet in 1,000 µL of phosphate-buffered saline.
  6. Transfer 10 µL of the solution to a 1.5 mL microcentrifuge tube and mix with 10 µL of trypan blue.
  7. Take 10 µL of the trypan blue cell solution into a cell counting chamber slide and insert it into the cell counting machine (see Table of Materials).
  8. Plate 40,000 cells per 20 µL of basement membrane extract (BME) into an 8-well glass chamber slide (see Table of Materials). This maintains the organoids for 3-5 days to allow the cells to form organoids and grow to a suitable size.
  9. To induce double-strand DNA breaks, radiate the plated organoids with 10 Gray (Gy) of ɣ-irradiation (see Table of Materials for irradiator details).
    NOTE: This could take up to 5-10 min.
  10. Incubate the organoids in their culture media in a humidified incubator at 37 °C and 5% CO2 for 4 h.

3. Immunofluorescence staining

NOTE: Volumes refer to the amount per well of the 8-well chamber slide (~300 µL).

  1. After irradiation and incubation of the organoids, aspirate the media with a pipette, carefully so as not to disrupt the 3D matrix. Wash with 300 µL of PBS.
  2. Fix the organoids in 300 µL of 2% paraformaldehyde (PFA) for 10 min.
    NOTES: Do not leave for too long, as the BME will depolymerize and could be aspirated off.
  3. Wash the organoids with 300 µL of staining buffer (see Table of Materials). Place on a shaker for 5 min.
  4. For permeabilization, gently add 300 µL of permeabilization buffer (see Table of Materials) and incubate for 20 min. Wash with 300 µL of staining buffer. Place on a shaker for 5 min.
  5. Add 300 µL of staining buffer to block the permeabilization step. Place on a shaker for 30 min. Aspirate off the staining buffer using a pipette.
  6. Add 300 µL of primary antibodies (rabbit anti-RAD51, mouse anti-Geminin, rabbit anti-RPA, mouse anti-ɣH2AX, rabbit anti-Geminin, mouse anti-53BP1; see Table of Materials) diluted in staining buffer. Incubate at 4 °C for 16 h.
    NOTE: Avoid co-staining with the same host animal. Leave the lid off to avoid the antibodies mixing into neighboring wells.
  7. Remove the primary antibody solution. Perform three washes with 300 µL of staining buffer for 5 min each on the shaker.
  8. Add 300 µL of secondary antibody (goat anti-mouse Alexa fluor 488 and goat anti-rabbit Alexa fluor 647; see Table of Materials) solution diluted in staining buffer and incubate for 1 h in the dark.
    NOTE: All subsequent steps must be performed in the dark.
  9. Aspirate the secondary antibody solution. Add 300 µL of diluted DAPI. Place on a shaker for 5 min.
  10. Perform three washes with 300 µL of staining buffer for 5 min each on the shaker. Remove the staining buffer and detach the chambers using the removal kit included with the chamber slides (see Table of Materials).
    NOTE: Ensure not to push too far forward so as to disrupt the 3D matrix.
  11. Using a p200 pipette tip with the tip cut off, add mounting medium (see Table of Materials) to cover each well with an organoid tab (e.g., 20-30 µL for each organoid tab).
  12. Place a coverslip over the specimen, avoiding bubbles.
  13. Take clear nail polish and paint it onto the sides of the cover glass to seal the slide. Let it harden for 1 h and place it at -20 °C.
    ​NOTE: After imaging, the slide can be stored for at least 6 months with minimal loss of fluorescence.

4. Imaging

  1. Acquire images using a confocal microscope (see Table of Materials) at 63x objective with immersion oil.
    NOTE: If imaging nuclear proteins, 63x is advantageous, but 40x is also acceptable.
  2. Use DAPI to locate the organoids through the eyepiece. Select the appropriate filters for microscopy based on the fluorophores used. Set the parameters for capturing the z-stack images.
    NOTE: The fluorophores used in the study were DAPI, 488, and 647. The 405, 488, and 638 lasers were turned on to visualize the staining.
    NOTE: The recommended z-stack depends on the resolving power of the objective.
  3. Adjust the live image: set focus, laser intensity, etc.
    NOTE: The higher the laser intensity, the more likely the sample will photo-bleach. Therefore, select an optimum laser intensity.
  4. Acquire the z-stack.
    NOTE: This could take up to 5-10 min.
  5. From the images collected in the z-stack, screenshot at least three images per stack.
    NOTE: Ensure to obtain screenshots throughout the stack so as to not duplicate the nuclei when quantifying.
  6. Save each file as a TIFF and proceed to analysis (step 5).

5. Analysis

NOTE: Use JCountPro for all image analysis following the previously published report21. To obtain this software, reference the associated publication.

  1. Under the object analysis panel (top of the program) in the file selection tab (bottom of the program), select the TIFF files.
  2. Click Add to move the selected files to the selected files group. Select Display.
  3. Under the segmentation tab, select blue as the color of the nuclei. Select Auto segmentation to optimize the threshold of the nuclei.
    NOTE: If the auto segmentation does not accurately identify the objects, then the user can adjust the fine tune and raw tune to the image or see the user manual to further optimize the segmentation.
  4. Under the objects panel, select Auto split large objects and optimize the size of the nuclei.
    NOTE: The nuclei typically have an unconditional size of 5,000 pixels, while the conditional size is 1,500 pixels. See the user manual to further optimize the size of the objects.
  5. Select Identify objects to test the parameters.
    NOTE: If these parameters are not accurate, the size and tuning can be adjusted along with other settings. See the user manual for instructions regarding further optimization.
  6. After adjusting the parameters to the image, select Identify Objects in All Images to identify the nuclei in all the images selected.
  7. Select the Foci Analysis panel (top of the program).
  8. Under the select files tab (bottom of the program), select the TIFF files that were used for object analysis and select the Arrow Buttons (>>) to move the images to the image files group.
  9. In the directory group underneath the image files that were moved, double click the Manual Edit folder and select to move the ioc files into the object collection files group.
    NOTE: All TIFFs selected must have matched ioc files.
  10. Press Select to move the files into the selected files group. Select the Foci counting tab at the bottom of the program.
  11. Optimize the parameters following the steps below.
    1. Top hat settings index: 12.
    2. Focus channel: Select the color of the foci (green: ɣ-H2AX; red: RAD51).
    3. H dome settings: dome height %: 30; threshold %: 28 and 28.
    4. Shape/size setting: Min focus size, pixels: 5. Select Apply Shape/Size. Max focus size (conditional): 32. Min roundness, x100: 96. Max focus, pixels: 60.
    5. Noise filter: size 1.
      NOTE: If determining if a nucleus is positive for geminin staining, under the second channel select green, and under analysis select intensity.
  12. To test the parameters set, select the below buttons in order: Top Hat > H-Dome > Foci Count.
    NOTE: If these parameters do not work, the size and tuning can be adjusted along with other settings. See user manual to learn more about how the image can be further optimized.
  13. Once the parameters are optimized for the selected images, select Auto count to count the foci in each image per nuclei. If the second channel is desired, the program will determine the intensity which can be used.

Results

The presented protocol can successfully stain, visualize, and quantify nuclear DNA damage repair proteins in organoids. This technique was used to stain and evaluate PDOs both before and after irradiation. PDOs were exposed to 10 Gy of radiation and evaluated for the following biomarkers: ɣ-H2AX (Figure 1), a marker of DNA damage; RAD51 (Figure 2), a marker for HRR; 53BP1, a marker of NHEJ; RPA, a marker of replication stress (Figure 3<...

Discussion

The DNA damage response plays an integral role in both the development of ovarian cancer and chemotherapy resistance. Therefore, a thorough understanding of DNA repair mechanisms is imperative. Here, a methodology is presented to study DNA damage repair proteins in 3D, intact organoids. A reproducible, reliable protocol is developed utilizing hallmark antibodies to evaluate DNA damage, homologous recombination, non-homologous end joining, and replication stress. Importantly, these methods are validated using genetically ...

Disclosures

The authors have nothing to disclose.

Acknowledgements

We are grateful for the guidance of Pavel Lobachevsky, PhD in establishing this protocol. We'd also like to acknowledge Washington University's School of Medicine in St. Louis's Department of Obstetrics and Gynecology and Division of Gynecologic Oncology, Washington University's Dean's Scholar Program, Gynecologic Oncology Group Foundation, and the Reproductive Scientist Development Program for their support of this project.

Materials

NameCompanyCatalog NumberComments
1x phosphate buffered saline with calcium and magnesium (PBS++)Sigma14-040-133
1x phosphate buffered saline without calcium and magnesium (PBS)Fisher Scientific ICN1860454
Ant-53BP1 Antibody BD Biosciences612522diluted to 1:500 in staining buffer
Ant-Geminin Antibody Abcamab104306diluted to 1:200 in staining buffer
Anti-Geminin Antibody ProteinTech10802-1-APdiluted to 1:400 in staining buffer
Anti-RAD51 Antibody Abcamab133534diluted to 1:1000 in staining buffer
Anti-yH2AX Antibody Millipore-Sigma05-636diluted to 1:500 in staining buffer
Ant-phospho-RPA32 (S4/S8) AntibodyBethyl Laboratories A300-245A-Mdiluted to 1:200 in staining buffer
Bovine Serum Albumin (BSA)Fisher Scientific BP1605 100
Centrifuge; Sorvall St 16R CentrifugeThermo Scientific 75004240
Confocal Microscope, Leica SP5 confocal system DMI4000Leica 389584
Conical Tubes, 15 mLCorning 14-959-53A
Countess 3 FL Automated Cell Counter (Cell Counting Machine) Thermo Scientific AMQAF2000
Countess Cell Counting Chamber SlidesThermo Scientific C10228
Cover SlipLA ColorsAny clear nail polish will suffice
Cultrex RGF Basement Membrane Extract, Type 2 R&D Systems 3533-010-02Could probably use Matrigel or other BME Matrix 
DAPI Thermo Scientific  R37606NucBlue Fixed Cell ReadyProbes Reagent, Diluted in 1x PBS 
Glycine Fisher Scientific NC0756056
JCountProJCountProFor access to the software, Email: jcountpro@gmail.com 
Microcentrifuge Tubes Fisher Scientific 07-000-243
Nail Polish StatLabSL102450
Parafomraldehyde (PFA), 2% Electron Microscopy Sciences 157-4Dilute to 4% PFA in PBS++ to obtain 2% PFA
Permeabilization BufferMade in Lab0.2% X-100 Triton in PBS++ 
PipetteRainin17014382
Pipette Tips Rainin 17014967
ProLong Gold Antifade MountantThermo Scientific  P36930
Staining Buffer Made in Lab0.5% BSA, 0.15% Glycine, 0.1% X-100 Triton in PBS++ 
Thermo Scientific Nunc Lab-Tek II Chamber Slide System Thermo Scientific 12-565-8
Triton X-100Sigma-Alderich 11332481001
Trypan Blue Solution, 0.4%Thermo Scientific 15250061
TrypLE ExpressInvitrogen12604013animal origin-free, recombinant enzyme
X-RAD 320 Biological Irradiator Precision X-Ray Irradiation X-RAD320

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