A 3D Human Lung Tissue Model for Functional Studies on Mycobacterium tuberculosis Infection

Note: Human peripheral blood from healthy anonymous blood donors purchased at the blood bank of Linköping University Hospital, Sweden was used as the source of immune cells for this study. This protocol is designed for 24 mm 6-well plate inserts. Direct adaptation to other well formats is not recommended since the tissue model contracts both vertically and horizontally during development.

1. Preparation of Materials, Media and Culture of Bacteria/ Cell Lines

1. Culture of bacteria:
   1. Grow the mycobacterial strain M. tuberculosis H37Rv carrying the pFPV2 plasmid to constitutively express green fluorescent protein (GFP), in Middlebrook 7H9 medium containing 0.05% Tween-80, 0.5% glycerol, kanamycin (20 µg/ml), and supplemented with Middlebrook albumin, dextrose and catalase enrichment (Middlebrook ADC Enrichment), at 37 °C with 5% CO₂ for 7-10 days.
      Note: All experimental steps involving live virulent M. tuberculosis strains should be performed in a BSL-3 facility.
2. Prepare 1x Dulbecco’s Modified Eagle’s Medium (DMEM) complete medium (supplemented with 1 mM sodium pyruvate, 2 mM L-glutamine, 100 U/ml penicillin, 100 µg/ml streptomycin, 10 mM HEPES, 0.1 mM non-essential amino acids and 10% heat-inactivated fetal bovine serum (FBS)). Prepare also antibiotic-free DMEM complete medium.
3. Prepare 1x Minimum Essential Medium (MEM) complete medium (1 mM sodium pyruvate, 2 mM L-glutamine, 100 U/ml penicillin, 100 µg/ml streptomycin, 10 mM HEPES, 0.1 mM non-essential amino acids and 10% heat-inactivated fetal bovine serum (FBS)).
4. Preparation of fibronectin/collagen-coated flasks (total 10 ml):
   1. Pipette 8.8 ml sterile 1x phosphate buffered saline (PBS) into a clean tube. Add 1 ml bovine serum albumin (1 mg/ml), 100 µl type I bovine collagen (3 mg/ml) and 100 µl recombinant human fibronectin (1 mg/ml).
   2. Mix the solution by turning the tube upside-down 5 times. Flasks are coated with a fibronectin/collagen solution (1 ml for a T-25 and 2 ml for a T-75 flask). Leave it O/N at 37 °C. After incubation, remove the solution and store the coated flasks at RT.
      Note: The collected solution can be stored at 4 °C and reused for three times. Storage for more than 2 weeks may cause the liquid to turn brown (formation of crystals), where upon it must be discarded.
5. Culture of fibroblasts:
   1. Grow and maintain MRC-5, (a human lung fibroblast cell line derived from normal lung tissue of a 14-week old male foetus), in complete DMEM in 5% CO₂ at 37 °C. Use the fibroblasts at passages 24-26 and grow until 70-80% confluent.
      Note: MRC-5 cell line at passage >30 tend to lose the morphology and is not recommended for use in the tissue model.
6. Culture of epithelial cells:
   1. Obtain 16HBE14o- (16HBE), an immortalized human bronchial epithelial cell line that retains the differentiated morphology and function of normal human airway epithelia, (this was a gift from Dr. Dieter Gruenert, Mt. Zion Cancer Center, University of California, San Fransisco, USA ¹⁰. ). Culture 16HBE cells in fibronectin/collagen-coated flasks and maintain the cells in complete MEM in 5% CO₂ at 37 °C.
7. Preparation of 5x DMEM
   1. Prepare 5x DMEM by dissolving 13.4 g of DMEM powder and 3.7 g of sodium bicarbonate in 150 ml of sterile distilled water. Adjust the pH of the medium to 7.3, make up the volume to 200 ml and filter it using 0.22 µm membrane filter. Collect the filtered medium in a sterile container and stored until use at RT.

2. Preparation of Collagen-embedded Fibroblasts

1. Thaw frozen aliquots of FBS and L-glutamine in a 37 °C water bath. After thawing keep the samples on ice. Place Sodium bicarbonate (71.2 mg/ml) and Gentamicin (50 mg/ml) at 4 °C. Pre-cool 50 ml centrifuge tubes and 10 ml sterile pipettes to 4 °C.
   Note: All materials used (except the 5x DMEM) are chilled on ice prior to use and all steps are performed on ice. Type I Bovine Collagen (1.1 mg/ml) must be kept cold, as this prevents solidification of collagen.
2. Prepare the fibroblast cells:
   1. Warm Trypsin in a 37 °C water bath and incubate sufficient quantity with Lung fibroblasts (MRC-5) cells for 10 min at 5% CO₂ at 37 °C. Neutralize the trypsin by adding 1x DMEM complete. Aspirate the cell suspension and centrifuge at 300 x g for 5 min. Aspirate the supernatant and resuspend the cells at 2.3 x 10⁵ cells/ml in DMEM complete. Place the cells on ice until ready for use.
3. Prepare the pre-mix:
   1. Add the following to a tube labeled “pre-mix”; 395 µl of 5x DMEM, 40 µl L-Glutamine, 120 µl NaHCO3 (71.2 mg/ml), 440 µl FBS , 5 µl Gentamicin (50 mg/ml), Total volume 1,000 µl, then swirl the pre-mix well and put on ice.
      Note: The volumes given are for one 24 mm 6-well culture insert. Calculate the specific amounts required for the total number of inserts but add one extra to be sure, enough pre-mix is prepared.
4. Prepare the acellular collagen mixture:
   1. To each culture add 1 ml of acellular collagen mixture. Add the following to a 50-ml conical tube on ice in the given order; 686 µl of 1.1 mg/ml collagen, 250 µl Pre-mix and 64 µl 1x complete DMEM to a total volume of 1,000 µl. Mix the solution well ensuring no air bubbles. Work fast and add the collagen on the wall of the tube to avoid air bubbles.
   2. Add 1 ml of the acellular layer mixture to the insert placed in the 6 well plate. Do not add any medium to the well outside the insert. Incubate for 30 min in a 37 °C incubator. Make sure the acellular mixture covers the entire insert without any air bubbles.
5. Prepare the cellular collagen mixture:
   1. Mix components of the cellular layer in a 50 ml conical tube kept on ice in the following order; 2 ml Collagen, 615 µl Pre-mix, 58 µl of 1x complete DMEM and 327 µl cell suspension Lung fibroblasts (MRC-5) to make up the total volume to 3,000 µl. Each culture requires 3 ml of cellular collagen mixture.
      CRITICAL STEP: Make sure to mix the collagen and premix carefully before addition of the cell suspension. This will neutralize the pH of the collagen to avoid toxic effects on the fibroblasts.
   2. Add the cellular layer (3 ml) on top of the acellular collagen layer and incubate for 2 hr in a 37 °C incubator. Work fast and add the collagen on the wall of the tube to avoid air bubbles.
   3. Following polymerization, add 2 ml of DMEM complete to the bottom of the 6 well plate (under the insert) and incubate for 24 hr.
      NOTE: If polymerization did not occur, discard the plate inserts containing the fibroblast-collagen matrix and start-over again. The most likely cause is an error in addition or incorrect volume of one of the above listed reagents.

3. Continuous Culture of the Fibroblast-collagen Matrix

1. Carefully lift the insert using a clean forceps and aspirate the culture media from the bottom of the well. Add 2 ml complete DMEM to the bottom of the well followed by 2 ml complete DMEM within the insert. Avoid introducing air bubbles under the insert, as this will prevent the diffusion of nutrients between the outer and inner chambers. Remove air bubbles with a micropipette tip.
2. Change the culture media (inside and below the insert) every second day and culture for approximately 5-7 days. Take care in removing the media from the insert. To avoid contact with the fibroblast-collagen matrix, slightly tilt the insert using a clean forceps and aspirate the media from the insert walls.
   CRITICAL STEP: The fibroblasts in the collagen matrix should get an elongated phenotype, and remodel the collagen, which then contracts. In about 5-7 days, the matrix has contracted to form a platform (10-14 mm in diameter) in the center of the insert. The contracted matrix is ready for use in the next step. To obtain a uniform contraction of the matrix it is critical that the fibroblasts are well mixed with the collagen prior to seeding (Step 2.6.1).

4. Seeding of Immune Cells (Infected/Uninfected Monocyte-macrophage Mixture)

Note: The following experimental steps involve virulent mycobacteria and therefore must be performed in a BSL-3 facility.

1. Preparation of primary monocytes and macrophages:
   1. Isolate peripheral blood monocytes from donor blood using an established protocol. Isolate monocytes on the same day as setting up the tissue model and culture and differentiate them into macrophages for approximately 7 days before infection with M. tuberculosis.
      NOTE: This will ensure both the macrophages and the contracted fibroblast-collagen matrix are available after 7 days. Also isolate fresh monocytes that will be added together with the infected macrophages.
2. Preparation of M. tuberculosis -infected macrophages
   1. Harvest the cultured bacteria, wash with 1x PBS containing 0.05% Tween-80, resuspend in antibiotic-free complete DMEM, pass through a truncated sterile 27 G needle to disperse bacterial clumps and measure the optical density.
      Note: Pre-determine the M. tuberculosis colony forming unit equivalents of optical density in the laboratory. This will give an estimate of the number of bacteria to be used for infection.
   2. Incubate the macrophages for 4 hr with M. tuberculosis at the multiplicity of infection (MOI) 10). After infection, wash 3x with 1x PBS to remove the extracellular bacteria. Use uninfected macrophages cultured in the same way but without M. tuberculosis, as controls.
   3. Detach the macrophages from the culture plate by treatment with 2 mM EDTA for 10 min at 37 °C and resuspended the cells in antibiotic-free complete DMEM.
3. Labelling of monocytes
   Note: Isolation and labeling of monocytes can be performed in the BSL-2 bench and then taken into BSL-3 facility for further processing.
   1. Stain freshly prepared monocytes (2 x 10⁷ cells) with a final concentration of 2 µM PKH26 red dye for 5 min, according to the manufacturer’s instructions. Wash 3x and resuspend the cells with antibiotic-free complete DMEM at a density of 1 x 10⁷ cells/ml.
4. Addition of immune cells to fibroblast-collagen matrix
   1. After 5-7 days of culture of the fibroblast-collagen matrix, aspirate the culture media from the outer and inner chambers and add 1.5 ml of fresh antibiotic-free DMEM complete to the outer chamber.
   2. Prepare a labeled monocyte-macrophage (uninfected/infected) mixture with a ratio of MO:MQ (5:1) in 50 µl DMEM complete. For 50,000 macrophages, take 250,000 labeled monocytes.
   3. Add 50 µl MO:MQ mixture to the fibroblast-collagen matrix and incubate for 1 hr in 5 % CO₂ at 37 °C. After incubation, gently add 2 ml of culture media into the insert and incubate for an additional 24 hr in 5% CO₂ at 37 °C.
      Note: As cells added are loosely attached, addition of media should be slow by gently adding on the walls of the insert.

5. Seeding of Lung Epithelial Cells (16HBE)

Note: The following steps must be performed in a BSL-3 facility.

1. Seed lung epithelial cells (16HBE) on top of the MO:MQ-fibroblast-collagen layer. To perform this, first dissociate 16HBE cells from the flask by treating with trypsin (as in 2.2.1.) and resuspend at 4 x 10⁶ cells/ml in antibiotic-free DMEM.
2. Aspirate the culture media inside and outside of the insert. Then add 1.5 ml antibiotic-free DMEM complete in the bottom of the well outside the insert.
3. Add 50 µl of 16HBE on top of the immune cell-fibroblast collagen matrix. Leave for 2 min in the hood and incubate for 1 hr in 37 °C incubator with 5% CO₂. After incubation, add gently 2 ml of antibiotic-free DMEM complete within the insert and culture at 37 °C for 3 days. The culture step facilitates proliferation of epithelial cells in the tissue model.
   Note: As cells added are loosely attached, addition of media should be slow and gentle by sliding through the walls of the insert.

6. Air-exposure of the 3D Lung Model

Note: After day 5 post addition of infected macrophages, the tissue models are air-exposed and the following steps must be performed in a BSL-3 facility.

1. Aspirate the culture media inside and outside of the insert.
   Note: In this step supernatants can be collected for detection of secreted factors. Centrifuge, sterile-filter and store supernatants at -70 °C.
2. Add 1.8 ml antibiotic-free DMEM complete in the outer chamber and incubate in 5% CO₂ at 37 °C incubator for 2 days. Do not add culture media within the insert.
   NOTE: Air-lifting of the tissue model facilitates the formation of stratified epithelia and mucus secretion, which provides the strength to the tissue and physiological resemblance to human lung tissue.

7. Harvesting and Mounting the 3D Lung Tissue Model

Note: The following steps must be performed in a BSL-3 facility.

1. On day 7 post implantation of infected macrophages, the tissue models are ready for harvesting. Remove the culture media entirely from the tissue model. Fix the tissue model with 4% paraformaldehyde for 30 min in the dark at RT. This step kills the bacteria and fixes the tissue/ cell morphology for further processing.
2. Using a scalpel, separate the membrane from the well insert. Transfer the membrane containing the tissue to a well containing 1x PBS.
3. Cut and remove the sides of the tissue model using a clean scalpel. Then slice the tissue model into 4 approximately equal square pieces. Transfer a piece of tissue onto a superfrost glass slide. Store the tissue pieces in 1x PBS at 4 °C.
4. Dry the tissue for 5 min and mount using ProLong Gold antifade with DAPI and coverslip. Leave the slides without disturbing in the dark at RT until dry.
   Note: The thickness of the tissue may vary between the center and periphery, causing slight tilting of the coverslip. To avoid this, a spacer (for instance parafilm) may be placed on the corner of the cover slip.
5. Apply nail polish to the edges of the coverslip and allow it to dry. Immerse the slides in 70% ethanol to make them safe to bring out of the BSL-3 facility.

8. Visualization, Acquisition and Quantitative 3D Analysis

1. Visualize the tissue slides using a confocal microscope system with lasers emitting at 488 nm for excitation of GFP (green channel), 420 nm for DAPI (blue) and 555 nm for the PKH26-labeled monocytes (red) respectively.
2. Acquire 3D images at a 512×512 resolution with Z-stacks covering at a minimum of 20 µm thickness and having 1 – 1.5 µm separation between stacks. Acquire 5-10 different fields covering the entire piece of tissue.
   Note: Use the configuration such as Nyqvist for optimal settings of optical resolution (wavelength, laser power/exposure, pixel size and zoom). Avoid under or over saturation of pixels.
3. Analyze the confocal images with 3D image processing software. For 3D quantification of cell clusters, the following steps are recommended for optimal analysis.
4. Open the 3D image processing software and load the image. Measure the dimensions of objects to be analysed in the image, for example, the size of a nucleus, individual monocyte and single bacteria. These observations are useful for defining or filtering the objects.
5. Using a display adjustment tool, optimise volume rendering by adjusting each channel for image contrast, brightness and blend opacity. This step is to minimise the interference of noise in volume rendering.
   Note: Gamma correction may lead to manipulation of images and thus should be avoided.
6. Create surfaces by choosing the red channel (monocytes) and set the threshold (automatic or manual selection). If required, use filters to restrict the selection of red monocytes or to exclude the background. Similarly, create surfaces for green (M. tuberculosis) and blue (nuclei) channels as described above.
7. Export the data into Ms-Excel files. It is possible to export a particular parameter or all the data. The parameters that are relevant for analysis of cell clustering are volume, intensity, number of objects, number of voxels and sphericity.
8. Save and export the images in a suitable picture format preferably TIFF.
   NOTE: Animations can also be made using the animation menu and saved as a media file.
9. Save the analysis settings of each channel using the Add parameters option and can be retrieved later using the Rebuild function. Simultaneously analyse more files using the Batch processing tool.
   Note: All the images to be compared must be acquired, processed and analyzed in the same manner. For instance a 8 bit image (256 integer) should not be compared with a 12 bit image (4096 integer).