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W tym Artykule

  • Podsumowanie
  • Streszczenie
  • Wprowadzenie
  • Protokół
  • Wyniki
  • Dyskusje
  • Ujawnienia
  • Podziękowania
  • Materiały
  • Odniesienia
  • Przedruki i uprawnienia

Podsumowanie

The present protocol describes establishing a murine colonic organoid system to study the activity and functioning of colonic stem cells in a claudin-7 knockout model.

Streszczenie

The intestinal epithelium regenerates every 5-7 days, and is controlled by the intestinal epithelial stem cell (IESC) population located at the bottom of the crypt region. IESCs include active stem cells, which self-renew and differentiate into various epithelial cell types, and quiescent stem cells, which serve as the reserve stem cells in the case of injury. Regeneration of the intestinal epithelium is controlled by the self-renewing and differentiating capabilities of these active IESCs. In addition, the balance of the crypt stem cell population and maintenance of the stem cell niche are essential for intestinal regeneration. Organoid culture is an important and attractive approach to studying proteins, signaling molecules, and environmental cues that regulate stem cell survival and functions. This model is less expensive, less time-consuming, and more manipulatable than animal models. Organoids also mimic the tissue microenvironment, providing in vivo relevance. The present protocol describes the isolation of colonic crypts, embedding these isolated crypt cells into a three-dimensional gel matrix system and culturing crypt cells to form colonic organoids capable of self-organization, proliferation, self-renewal, and differentiation. This model allows one to manipulate the environment-knocking out specific proteins such as claudin-7, activating/deactivating signaling pathways, etc.-to study how these effects influence the functioning of colonic stem cells. Specifically, the role of tight junction protein claudin-7 in colonic stem cell function was examined. Claudin-7 is vital for maintaining intestinal homeostasis and barrier function and integrity. Knockout of claudin-7 in mice induces an inflammatory bowel disease-like phenotype exhibiting intestinal inflammation, epithelial hyperplasia, weight loss, mucosal ulcerations, epithelial cell sloughing, and adenomas. Previously, it was reported that claudin-7 is required for intestinal epithelial stem cell functions in the small intestine. In this protocol, a colonic organoid culture system is established to study the role of claudin-7 in the large intestine.

Wprowadzenie

Intestinal organoid culture is a three-dimensional (3D) ex vivo system in which stem cells are isolated from the intestinal crypts of primary tissue and plated into a gel matrix1,2. These stem cells are capable of self-renewal, self-organization, and organ functionality2. Organoids mimic the tissue microenvironment and are more similar to in vivo models than two-dimensional (2D) in vitro cell culture models, although less manipulatable than cells3,4. This model eliminates obstacles encountered in 2D models, such as a lack of proper cell-cell adhesions, cell-matrix interactions, and homogenous populations, and also reduces the limitations of animal models, including high costs and lengthy periods of time5. Intestinal organoids-also referred to as colonoids for those grown from colonic crypt-derived stem cells-are essentially mini-organs that contain an epithelium including all cell types that would be present in vivo, as well as a lumen. This model allows manipulation of the system to study many aspects of the intestine, such as the stem cell niche, intestinal physiology, pathophysiology, and gut morphogenesis3,5,6. It also provides a great model for drug discovery, studying human intestinal disorders such as inflammatory bowel disease (IBD) and colorectal cancer, patient-specific personalized treatment development, and studying tissue regeneration4,7,8,9. In addition, the organoid system can also be used to study cellular communication, drug metabolism, viability, proliferation, and response to stimuli7,8. While animal models may be used to test potential therapeutics for intestinal pathologic conditions, they are quite limited, as studying multiple drugs at once poses a challenge. There are more confounding variables in vivo, and associated cost and time are high and long, respectively. On the other hand, the organoid culture system allows for the screening of many therapeutics at once in a shorter time period and also allows for personalized treatment through the use of patient-derived organoid culture4,8. The ability of colonic organoids to mimic tissue organization, microenvironment, and functionality also makes them an excellent model for studying regeneration and tissue repair9. Our lab has established a small intestine organoid culture system to study the effect of claudin-7 on small intestine stem cell functions10. In this study, a large intestinal organoid culture system is established to study stem cells' ability, or lack of ability, to self-renew, differentiate, and proliferate in a conditional claudin-7 knockout (cKO) model.

Claudin-7 is a very important tight junction (TJ) protein that is highly expressed in the intestine and is essential for maintaining TJ function and integrity11. cKO mice suffer from an IBD-like phenotype, exhibiting severe inflammation, ulcerations, epithelial cell sloughing, adenomas, and increased cytokine levels11,12. While it is widely accepted that claudins are vital for epithelial barrier function, new roles for claudins are emerging; they are involved in proliferation, migration, cancer progression, and stem cell function10,12,13,14,15,16,17. It is currently unknown how claudin-7 impacts the stem cell niche and function of colonic stem cells. As the intestine rapidly self-renews approximately every 5-7 days, maintenance of the stem cell niche and proper functioning of the active stem cells is vital18. Here, a system is established to examine the potential regulatory effects of claudin-7 on the colonic stem cell niche.

Protokół

All animal experiments and procedures were approved by the East Carolina University (ECU) Animal Care and Use Committee (IACUC) and conducted in compliance with guidelines from the National Institutes of Health and ECU on laboratory animal care and use. Inducible, intestinal-specific claudin-7 knockout mice were generated by crossing C57BL6 claudin-7-flox transgenic mice with Villin-CreERT2 mice19. Male and female mice aged 3 months were used in this study.

1. Reagent/equipment preparation

  1. Cool the following reagents/equipment before starting their associated experiments: phosphate buffered saline (PBS) for washing colon tissue during crypt isolation; a rocker/rotator (place in a 4 °C refrigerator) for incubation with epithelial dissociation media.
    1. Remove the gel matrix (see Table of Materials) from -20 °C and thaw on ice before plating.
    2. Pre-cool the centrifuge to 4 °C prior to spinning down crypts for plating.
    3. Cool 0.1% sodium citrate buffer (see Table of Materials) and keep on ice prior to in situ cell death detection.
  2. Warm the following reagents before starting their associated experiments: a 96-well culture plate for 24 h before plating; L-WRN media (see Table of Materials) before adding to plated crypts and before each media change.
    1. Heat the water bath to 94 °C before staining.

2. Murine colonic crypt isolation

  1. Prepare the necessary media following the steps below.
    NOTE: The media volumes are calculated here for the colonic tissue of two mice.
    1. Prepare epithelial dissociation media: 30 mL of 1x PBS + 400 µL of 0.5 M EDTA + 50 µL of 10 mM Y-27632 dihydrochloride (see Table of Materials). Keep on ice until use.
    2. Prepare crypt dissociation media: 10 mL of 1x PBS + 10 µL of 10 mM Y-27632 dihydrochloride. Keep on ice until use.
    3. Supplement L-WRN media: 50 mL of L-WRN media + 47.5 mL of DMEM high glucose with L-Glutamine + 500 µL of L-glutamine + 500 µL of pennicilin/streptomycin + 1,000 µL of B-27 supplement (50x) + 500 µL of N2 supplement (100x) + 50 µL of HEPES (1 M) buffer solution (see Table of Materials).
    4. Filter the complete (supplemented) L-WRN media and aliquot for storage at -20 °C for up to 3 months.
      NOTE: Thawed media is stable at 4 °C for up to 2 weeks.
  2. Perform the crypt isolation.
    1. For general anesthesia, add 1 mL of isoflurane to cotton and place it inside a plastic cassette within a 0.09 cubic feet anesthesia chamber (see Table of Materials). Place the mouse in the anesthesia chamber until breathing halts (approximately 3-5 min) and then perform cervical dislocation20.
    2. Make an approximately 2 in incision down the midline of the mouse, pinning the back skin to expose the abdomen. Isolate the colon by cutting just below the cecum from the proximal side and above the rectum from the distal side21.
    3. Using forceps, remove the adipose tissue attached to the colon. Gently push feces out utilizing the flat end of the forceps and cut the tissue open longitudinally.
    4. Wash the tissue 10-15 times with cold 1x PBS using forceps to "swirl" the tissue around in PBS between washes.
    5. Using clean, sharp scissors, cut the tissue into small pieces, approximately 3-5 mm in size.
    6. Repeat the process for the second mouse and combine the tissue pieces in a 50 mL tube containing cold epithelial dissociation media (step 2.1.1).
    7. Incubate the colon tissue pieces in epithelial dissociation media for 90 min at 4 °C with gentle rocking.
    8. Allow the tissue fragments to sink to the bottom of the tube, then carefully discard the epithelial dissociation media without disrupting the tissue. Repeat this process when washing the tissue 10-15 times with cold 1x PBS. Discard as much PBS as possible during the final wash.
    9. Add crypt dissociation media (step 2.1.2) to the 50 mL tube containing colon tissue pieces and continuously shake for 5-10 min by hand.
      NOTE: The media must become cloudy from the dissociated crypts.
    10. Under the cell culture hood, filter the tissue and media with a 70 µm nylon cell strainer (see Table of Materials) into a fresh 50 mL tube.
    11. Centrifuge at 200 x g for 10 min at room temperature and discard the supernatant without disturbing the crypt-containing pellet.
      NOTE: Depending on the equipment, one may transfer the strained media to a 15 mL tube for centrifuging.
    12. Resuspend the pellet in ~3-4 mL of cold 1x PBS.
    13. Pipette 10 µL of the isolated crypts in a line on a microscope slide. Under the microscope, count the number of full, long crypts to estimate crypt concentration per 10 µL.
    14. Calculate the appropriate volume of crypts to spin down in order to plate 10 crypts/µL in a 96-well plate.

3. Crypt plating

  1. Centrifuge an appropriate volume of isolated crypts in a 1.5 mL microcentrifuge tube at 200 x g for 5 min at 4 °C.
  2. Carefully remove the supernatant using a 1,000 µL pipette without disrupting the pelleted crypts.
  3. Add 100 µL of gel matrix (enough for nine wells) to the pelleted crypts and pipette carefully to avoid introducing air bubbles.
    NOTE: See the Discussion section for a detailed description of how to mix the gel matrix and crypts. Typically, 100 µL is sufficient for nine wells.
  4. Allow the gel matrix to partially solidify (~1-2 min).
  5. Plate 10 µL of the gel matrix mixed with the crypts in each well of a pre-warmed 96-well culture plate to form a dome shape.
    NOTE: Place the dome in the center of the well. Be careful not to allow the gel matrix to spread to the sides of the well. See the Discussion section for a detailed description on solidification and plating.
  6. Allow the gel matrix to be fully set for 10-20 min in an incubator at 37 °C with 5% CO2.
  7. Prepare the final working solution of L-WRN media.
    1. Add 100 µL pennicilin/streptomycin to a 10 mL aliquot of L-WRN media (see step 2.1.3) (stable for 2 weeks at 4 °C).
    2. Add supplements to 900 µL of L-WRN media with pennicilin/streptomycin: 0.9 µL of 1 mg/mL EGF + 0.9 µL of 10 mM Y-27632 dihydrochloride.
      NOTE: The volumes are based upon nine wells. Y-27632 dihydrochloride is only added on day 0 (at the time of plating).
  8. Add 100 µL of media to each well. Be careful not to disrupt the dome.
  9. Incubate at 37 °C with 5% CO2 for 24 h.

4. Creating claudin-7 knockout in culture

  1. Allow the crypts to grow normally in culture for 24 h after plating.
  2. In a 1.5 mL microcentrifuge tube, add 2.7 µL of 1 mmol/L 4-hydroxytamoxifen (4OH-Tamoxifen) to 900 µL of L-WRN media (final concentration of 3 µmol/L) + 0.9 µL of 1 mg/mL EGF.
    NOTE: The stock solution of 4OH-Tamoxifen is prepared by mixing powdered 4OH-Tamoxifen (see Table of Materials) with 1x PBS to a concentration of 1 mmol/L.
  3. Remove old media from the wells via vacuum suction.
  4. Add 100 µL of 4OH-Tamoxifen-containing media to each well and label them as claudin-7 cKO/4OH-TAM.
    NOTE: DMSO needs to be added to the control wells. Fresh 4OH-Tamoxifen-containing media must be added every 2 days.
  5. Incubate at 37 °C until the next media change (~2-3 days).

5. Colonic organoid maintenance

NOTE: Media must be changed every 2-3 days. Culture up to 12 days.

  1. Prepare a fresh final working solution of L-WRN media: 900 µL of L-WRN media + 0.9 µL of 1 mg/mL EGF.
  2. Remove old media from the wells via vacuum suction. Add fresh media to the wells.
    NOTE: Be careful not to disrupt the dome.
  3. Incubate at 37 °C until the next media change.
    ​NOTE: Cultures can be maintained and passaged for the duration desired for the experiment. The cultures for the present study were typically maintained for between 9-12 days, but one may wish to continue further, for 15 or 20 days.

6. Harvesting and embedding colonic organoids

  1. Remove old media from the wells via vacuum suction.
  2. Fix the organoids with 4% paraformaldehyde (PFA) for 1 h at room temperature.
    NOTE: PFA is a toxic material. Take precautions when using this reagent.
  3. Remove 4% PFA from the wells via vacuum suction and add 30% sucrose for 24 h at 4 °C.
  4. Label a plastic mold and fill it to 90% with optimum cutting temperature (OCT) compound (see Table of Materials).
  5. Remove 30% sucrose from the wells via vacuum suction. Add 10 µL of 1x PBS to each well.
  6. With a pipette tip, gently scratch the bottom of the well to dissociate the dome containing organoids.
  7. With a pipette, remove the PBS containing the dissociated organoids and load the liquid into the mold containing OCT.
    NOTE: Avoid introducing bubbles into the OCT compound.
  8. Continue this process until all organoids have been removed from all wells.
  9. In a stainless-steel Dewar flask, add dry ice pellets and 2-methylbutane (enough to cover the dry ice pellets) (see Table of Materials).
  10. Steadily hold the organoid-containing OCT block above 2-methylbutane to flash freeze.
  11. Store the organoid-containing OCT block at -80 °C until ready to section (can be stored for up to 1 year).

7. Immunofluorescence

  1. Section the organoid-containing OCT block at a 5 µm thickness using a cryostat (see Table of Materials) at -20 °C.
  2. For each section, check under the microscope to ensure an organoid was captured. When sectioning is complete, store the slides at -80 °C until ready to stain (can be stored for up to 6 months).
  3. Heat the slides in 10 mM sodium citrate buffer for 10 min at 94 °C.
    NOTE: The buffer is made by dissolving sodium citrate in deionized water. Adjust the pH to 6 with hydrochloric acid.
  4. Allow the slides to cool on the benchtop for 20 min. Rinse with distilled water for 5 min.
  5. Assemble the slides in a staining rack (see Table of Materials) with 0.2% Triton X-100 and incubate with 100 mM glycine for 15 min.
  6. Rinse three times with 1x PBS for 5 min each. Block with 5% bovine serum albumin (BSA) for 45 min at room temperature.
  7. Incubate with claudin-7 anti-murine rabbit primary antibody22 (diluted in 1% BSA) overnight at 4 °C. Rinse three times with 1x PBS for 10 min each.
  8. Incubate with Cy3 anti-rabbit secondary antibody23 (diluted in 1% BSA) for 1 h at room temperature. Rinse three times with 1x PBS for 10 min each.
  9. Mount the slides with an appropriate mounting medium (see Table of Materials) with DAPI and add a coverslip.

8. Cell death detection

  1. Fix the organoids inside the wells with 4% paraformaldehyde for 1 h at room temperature. Rinse with 1x PBS for 5 min.
  2. Incubate the culture plate on ice with 0.1% Triton X-100 in cold 0.1% sodium citrate buffer for 2 min. Rinse twice with 1x PBS for 5 min each.
  3. Prepare TUNEL reaction24,25 using TMR Red, an in situcell death detection kit (see Table of Materials). Add 50 µL of TUNEL reaction reagents to each well.
  4. Incubate in a humidified atmosphere for 1 h at 37 °C in the dark.
    NOTE: All the remaining steps must be completed in the dark.
  5. Rinse three times with 1x PBS for 5 min each. Incubate with 1:2,500 Hoechst (diluted in 1x PBS, see Table of Materials) for 3 min.
  6. Rinse three times with 1x PBS for 5 min each. Utilize the TRITC filter to visualize images on a fluorescent microscope (see Table of Materials).

Wyniki

In order to examine the regulatory effects of claudin-7 on colon stem cells, colonic crypts were isolated from murine colon tissue as described above and shown in Figure 1A. Once the crypts were isolated from the primary tissue, they were plated in a 3D matrix in a 96-well plate to grow for 11 days (Figure 1). Normal healthy crypts will close the lumen and become spheroids by day 2 and eventually begin budding and forming the various epithelial cell types at app...

Dyskusje

Organoid culture is an excellent model for studying stem cell function, intestinal physiology, drug discovery, human intestinal diseases, and tissue regeneration and repair7,8,9,10,11,26. While it has many advantages, it can be challenging to establish. Care must be taken in all steps throughout the protocol, but most importa...

Ujawnienia

The authors declare no conflicts of interest.

Podziękowania

This study was funded by NIH DK103166.

Materiały

NameCompanyCatalog NumberComments
0.09 cubic feet space-saver vacuum desiccator United States Plastic Corp78564anesthesia chamber
0.5 M EDTA pH 8.0InvitrogenAM9261
1.5 mL microcentrifuge tubesThermoFisher69715
15 mL conical centrifuge tubesFisher Scientific14-959-53A
1x Dulbecco’s Phosphate buffered salineGibco14190-144
2-methylbutaneSigma277258
4% paraformaldehydeThermoFisherJ61899.AK
4-hydroxytamoxifen (4OH-TAM)Sigma579002
50 mL conical centrifuge tubesFisher Scientific14-432-22
70 µm nylon cell strainerCorning352350
96 well culture plateGreiner Bio-One655180
B-27 Supplement (50x)Gibco12587-010
Bovine serum albuminFisher ScientificBP1605-100
Claudin-7 anti-murine rabbit antibodyImmuno-Biological Laboratories 18875
Cover glass (24 x 50-1.5)Fisher Scientific12544E
Cryomoldsvwr25608-916
Cultrex RCF BME, Type 2R&D Systems3533-005-02gel matrix
Cy3 anti-rabbit antibodyJackson Immunoresearch111-165-003
Dewar FlaskThomas Scientific1173F61
DMEM High Glucose with L-GlutamineATCC30-2002
EVOS FLoid Imaging SystemThermoFisher4477136
Fluoro-Gel II with DAPIElectron Microscopy Sciences17985-50
GlutaMAX (100x)Gibco35050-061
GlycineJT Baker4059-02
HEPES (1 M) Buffer SolutionGibco15630-080
HoechstThermoFisher62249
In situ cell death detection kit, TMR RedRoche12156792910
IsofluranePivetal07-893-8440
L-WRN MediaHarvard Medical School Gastrointestinal Organoid Derivation and Culture CoreN/A
Mouse surgical kitKent Scientific CorporationINSMOUSEKIT
Murine EGFPeproTech315-09-500UG
N2 Supplement (100x)Gibco17502-048
Optimum cutting temperature (OCT) compound Agar ScientificAGR1180
Penicillin-StreptomycinGibco15140-122
Sequenza Rackvwr10129-584
Sodium CitrateFisher ScientificS-279
SucroseSigmaS9378
Triton X-100SigmaX100
Vacuum filter (0.22 µm; cellulose acetate)Corning430769
Y-27632 dihydrochlorideTocris Bioscience1254

Odniesienia

  1. Hughes, C. S., Postovit, L. M., Lajoie, G. A. Matrigel: a complex protein mixture required for optimal growth of cell culture. Proteomics. 10 (9), 1886-1890 (2010).
  2. Sato, T., et al. Long-term expansion of epithelial organoids from human colon, adenoma, adenocarcinoma, and Barrett's epithelium. Gastroenterology. 141 (5), 1762-1772 (2011).
  3. Wallach, T. E., Bayrer, J. R. Intestinal organoids: new frontiers in the study of intestinal disease and physiology. Journal of Pediatric Gastroenterology and Nutrition. 64 (2), 180-185 (2017).
  4. Shankaran, A., Prasad, K., Chaudhari, S., Brand, A., Satyamoorthy, K. Advances in development and application of human organoids. 3 Biotech. 11 (6), 257 (2021).
  5. Angus, H., Butt, A., Schultz, M., Kemp, R. Intestinal organoids as a tool for inflammatory bowel disease research. Frontiers in Medicine. 6, 334 (2020).
  6. Fan, Y., Davidson, L. A., Chapkin, R. S. Murine colonic organoid culture system and down stream assay applications. Methods in Molecular Biology. 1576, 171-181 (2019).
  7. Gupta, N., et al. Microfluidics-based 3D cell culture models: Utility in novel drug discovery and delivery research. Bioengineering and Translational Medicine. 1 (1), 63-81 (2016).
  8. Yoo, J., Donowitz, M. Intesitnal enteroids/organoids: A novel platform for drug discovery in inflammatory bowel diseases. World Journal of Gastroenterology. 25 (30), 4125-4147 (2019).
  9. Qu, M., et al. Establishment of intestinal organoid cultures modeling injury-associated epithelial regeneration. Cell Research. 31 (3), 259-271 (2021).
  10. Xing, T., et al. Tight junction protein claudin-7 is essential for intestinal epithelial stem cell self-renewal and differentiation. Cellular and Molecular Gastroenterology and Hepatology. 9 (4), 641-659 (2020).
  11. Ding, L., et al. Inflammation and disruption of the mucosal architecture in claudin-7-deficient mice. Gastroenterology. 142 (2), 305-315 (2012).
  12. Lu, Z., Ding, L., Lu, Q., Chen, Y. H. Claudins in intestines: distribution and functional significance in health and diseases. Tissue Barriers. 1 (3), 24978 (2013).
  13. Ding, L., Lu, Z., Lu, Q., Chen, Y. H. The claudin family of proteins in human malignancy: a clinical perspective. Cancer Management and Research. 5, 367-375 (2013).
  14. Bhat, A. A., et al. Claudin-7 expression induces mesenchymal to epithelial transformation (MET) to inhibit colon tumorigenesis. Oncogene. 34 (35), 4570-4580 (2015).
  15. Lu, Z., et al. A non-tight junction function of claudin-7-interaction with integrin signaling in suppressing lung cancer cell proliferation and detachement. Molecular Cancer. 14, 120 (2015).
  16. Wang, K., Xu, C., Li, W., Ding, L. Emerging clinical significance of claudin-7 in colorectal cancer: a review. Cancer Management and Research. 10, 3741-3752 (2018).
  17. Wang, K., et al. Claudin-7 downregulation induces metastasis and invasion in colorectal cancer via the promotion of epithelial-mesenchymal transition. Biochemical and Biophysical Research Communications. 508 (3), 797-804 (2019).
  18. Wang, F., et al. Isolation and characterization of intestinal stem cells based on surface marker combinations and colony-formation assay. Gastroenterology. 145 (2), 383 (2013).
  19. Li, W., et al. Severe intestinal inflammation in the small intestine of mice induced by controllable deletion of claudin-7. Digestive Diseases and Sciences. 63 (5), 1200-1209 (2018).
  20. Donovan, J., Brown, P. Euthanasia. Current Protocols in Immunology. 73 (1), (2006).
  21. Khalil, H., Nie, W., Edwards, R. A., Yoo, J. Isolation of primary myofibroblasts from mouse and human colon tissue. Journal of Visual Experiments. (80), e50611 (2013).
  22. Sugimoto, K., et al. Cell adhesion signals regulate the nuclear receptor activity. Proceedings of the National Academy of Sciences. 116 (49), 24600-24609 (2019).
  23. Mansour, H., et al. Connexin 30 expression and frewuency of connexin heterogeneity in astrocyte gap junction plaques increase with age in the rat retina. PLoS One. 8 (3), 57038 (2013).
  24. Miranda, M., et al. Antioxidants rescue photoreceptors in rd1 mice: relationship with thiol metabolism. Free Radical Biology and Medicine. 48 (2), 216-222 (2010).
  25. Wang, L., et al. Mesenchymal stromal cells ameliorate oxidative stress-induced islet endothelium apoptosis and functional impairment via Wnt4-β-catenin signaling. Stem Cell Research and Therapy. 8 (1), 188 (2017).
  26. Almeqdadi, M., Mana, M., Roper, J., Yilmaz, O. Gut organoids: mini-tissues in culture to study intestinal physiology and disease. American Journal of Physiology-Cell Physiology. 317 (3), 405-419 (2019).

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