An Experimental Model to Study Tuberculosis-Malaria Coinfection upon Natural Transmission of Mycobacterium tuberculosis and Plasmodium berghei

Safety Measures and Ethics Statement

The studies presented herein involve work with the human pathogen Mtb and the rodent malaria parasite Plasmodium berghei (P. berghei). Experiments with Mtb (strain H37Rv) and P. berghei must be carried out under the appropriate biosafety conditions. Biosafety level (BSL) 2 laboratories are required for rodent malaria parasites such as P. berghei and BSL 3 for Mtb and hence, for all coinfection studies described herein. NOTE: Mice infected with Mtb do not spread the infection to other mice within immediate vicinity (our own observation). Spread to the experimenter can therefore be excluded; however appropriate protective clothing has to be worn inside the BSL 3 laboratory at all times. According to our rules, experimenters wear surgical scrubs, hair nets, disposable respirators, and two pairs of gloves, of which the outer one is discarded anytime arms are withdrawn from the cabinet. New ones are put on before entering the cabinet again. Two containers, one with 2% Buraton (NOTE: other disinfectants approved to inactivate Mtb can be used at the approved concentration) for liquid and infectious waste material and one for surface decontamination, are prepared before the experiment and placed inside the cabinet. In addition, plastic bags will be used for solid noninfectious waste. According to German rules, all work involving the handling and processing of Mtb cultures or tissue derived from Mtb infected mice must be carried out in a class 2 biosafety cabinet within a BSL3 lab. While handling mycobacteria, measures have to be taken to avoid the generation of aerosols at all times.

Female C57BL/6 mice (Charles River) aged between 6-8 weeks were used for all coinfection experiments and maintained under specific barrier conditions in BSL 3 facilities. Animal care and experimentation were performed in accordance with protocols approved by the Ethics Committee for Animal Experiments of the Ministry for Agriculture, Environment, and Rural Areas of the State of Schleswig-Holstein

For obtaining malarial mosquito stages, NMRI mice were purchased from Charles River Laboratory, Sulzfeld, Germany and kept under specific pathogen-free conditions within the University Heidelberg animal facility (IBF). All animal experiments were performed according to European regulations and approved by the state authorities of Baden-Württemberg (Regierungspräsidium Karlsruhe).

1. Aerosol Infection of Mice with Mtb using a Glas-Col Aerosol Chamber

The best way to standardize aerosol infection of experimental animals with Mtb is to use mycobacteria from frozen stocks with known CFU titers. To prepare stock cultures, culture Mtb in Middlebrook 7H9 broth supplemented with OADC (Oleic acid, Albumin, Dextrose, Catalase) enrichment medium and 0.05% Tween 80, a carbon source for mycobacteria and measure to avoid bacterial clumping at the same time. Cultures should have an OD ≤ 1 at the time of harvest. At higher OD, bacterial clumping increases and viability decreases. Store 1 ml aliquots at -80 °C. Determine the number of viable colony forming units (CFU) in frozen stocks by plating a series of 10-fold dilutions of three independent vials on 7H11 agar plates supplemented with 0.5% glycerol, 1 g/L asparagine, and OADC and enumerate colonies after 4 weeks of incubation at 37 °C. Perform aerosol infection as described below.

1. Thaw Mtb stocks of known CFU titer and carefully mix the suspension five times to disperse bacterial clumps using a 1 ml syringe fitted with a 27 G needle. Avoid the production of aerosols.
2. Depending on the desired infection dose, transfer the required volume of the mycobacterial stock into a 50 ml tube containing sterile PBS. The final volume is 6 ml. NOTE: By varying the number of microorganism in this suspension, the proportion of bacteria bearing aerosol droplets is varied. We usually aim at an uptake of 100 viable bacilli per lung (low-dose infection). In our experience, this requires around 1-2 x 10⁶ Mtb/ml in a total volume of 6 ml of which 5.5 ml are nebulized (see below). It is recommended to do a series of experimental aerosol challenges with different concentrations of bacteria to find the ideal conditions for your infection. Whereas high dose infections with up to 5,000 mycobacteria can be done to speed up the infectious process, as few as 5 bacteria can be used to successfully infect mice by aerosol. The infection rate is commonly 100%.
3. Remove sufficient volume (prepared in excess of final volume required) for plating to determine the inoculum titer; we usually remove 500 µl to plate technical triplicates.
4. Place animals in a compartmented mesh basket (one mouse per basket) within the circular aerosol chamber and close the lid of the aerosol chamber. NOTE: Other models are equipped with a pie-shaped basket composed of five individual compartments, each of which can accommodate 20 mice.
5. Attach the Venturi-nebulizer unit to the three stainless steel socket joints.
6. Remove the mycobacterial suspension from the 50 ml tube with a 10 ml syringe fitted with an 18 G blunt needle and carry the syringe to the aerosol chamber in a closed transport box.
7. Remove the screw cap of the nebulizer unit and carefully inject the mycobacteria suspension into the nebulizer. Avoid the generation of aerosols. Discard the syringe into a sharps container containing 2% Buraton. Seal the nebulizer with the screw cap.
8. Switch on the main power switch and the UV lamp. The display on the control keypad shows “Glas-Col Apparatus Co”.
9. Turn the program switch on. The display will show “Is the nebulizer ready?” “Is the basket loaded?” Press enter when ready”. Press enter.
10. The display shows “Enter Preheat Time 900”; this means the preheat time for the incinerator (which decontaminates the exhaust air) is 900 sec. Press enter.
11. The display will show “Enter Nebulizing time 1,800”; this means the nebulizing time is set to 1,800 sec as default. In order to extend the nebulizing time, enter “2,400” and press enter. NOTE: During the nebulizing cycle, air under pressure atomizes the suspension, thereby generating small aerosol droplets containing mycobacteria. With the main air flow, these droplets (approximately 2-5 µm in size) are carried into the aerosol chamber.
12. The display will show “Enter C.D. Time 1,800”; this means that the decay cycle takes 1,800 sec. Set to “2,400” and press enter. NOTE: During this cycle, the cloud which has been built up in the aerosol chamber during the nebulizing cycle can decay. The small droplets are inhaled by the experimental animals.
13. The display will show “Enter Dec Time 900”; this means that the UV light decontamination cycle will take 900 sec. Press enter. The machine will start cycling through preheat, nebulizing, cloud decay and UV decontamination.
    CAUTION: The vacuum flow meter should indicate 60 cubic feet/hr (check when preheat cycle starts; adjust vacuum control valve if necessary) and the compressed air flow meter 10 cubic feet/hr (check when nebulizing cycle starts; adjust air control valve accordingly).
14. When the cycle is complete, the keypad will show “Process Complete – Remove Specimen”. Turn off the program, UV and main power switch.
15. Check if the mycobacterial suspension has been nebulized completely and if not, record the remaining volume by carefully removing the suspension with an appropriate syringe fitted with an 18 G blunt needle. The remaining volume should not be more than 1 ml.
16. Remove the nebulizer from the joints and place it in a pan containing 2% Buraton for a minimum of 2 hr, usually disinfection is done O/N. Afterwards, transfer the nebulizer to a fresh pan and rinse thoroughly with water. Leave nebulizer to air-dry.
17. Open the aerosol chamber and return animals to their cages. Bag the baskets in autoclave bags and autoclave. Wipe clean the surfaces of the inside of the aerosol chamber with 2% Buraton. NOTE: For safety reasons, a powered air purifying respirator should be worn during this procedure.
18. Using the remaining 500 µl of the mycobacterial suspension (see step 1.3) plate 10-fold dilutions of a technical triplicate (3 x 100 µl) on 7H11 agar plates.

2. Verify Uptake of Desired CFU in Lungs

One day after aerosol infection of experimental animals determine the bacterial load in the lungs of designated control animals in order to verify the uptake of the desired CFU. NOTE: We usually designate an extra group of 3-5 mice for day 1 CFU determination.

To monitor the course of Mtb infection over time, the mycobacterial tissue burden can be examined by plating serial dilutions of whole organ homogenates for CFU determination. The lung is the primary site for disease manifestation in tuberculosis however spleen, liver and lymph nodes are usually analyzed accordingly. The dilutions to be plated depend on the expected mycobacterial load in the organs, which depend on the initial inoculum (low dose vs. high dose), which gives rise to different bacterial loads in tissue, as well as on the organ and time point to be analyzed. Upon low dose infection, the bacterial load of Mtb H37Rv in the lung usually reaches a plateau between day 25-30.

1. Place euthanized animals (Euthanasia: CO₂ asphyxiation or terminal anesthesia) on absorbent paper on a dissecting board in a class II biosafety cabinet and disinfect mice with 70% ethanol. NOTE: 70% alcohol is for surface decontamination only and will not kill Mtb.
2. Make a small incision in the middle of the abdomen and retract the mouse skin above the head.
3. Open the abdomen and the thoracic cage with surgical scissors and remove the thoracic wall so that the lungs are accessible.
4. Remove the lungs and transfer into a 15 ml tube with homogenization buffer (sterile water/1% v/v Tween 80/1% w/v albumin).
5. Using the plunger of a 5 ml syringe strain lungs through 100 µm sieves into a small Petri dish.
6. Flush sieves several times using a 1 ml pipette equipped with a barrier tip and distribute the lung homogenate among 8 agar plates (ca. 250 µl/plate; make sure they have a well dried surface).
7. Carefully plate the samples using disposable spreaders which are discarded into 2% Buraton.
8. Leave agar plates to dry inside the cabinet. Seal every single plate with parafilm, wrap in aluminum foil and incubate upright at 37 °C for at least 4 weeks.

3. Construction of Escape-proof Mosquito Cages

Rodent Plasmodium strains are not harmful to humans. However, since Mtb-infected mice are the recipients of the parasite and work is done under BSL 3 conditions, precautions are necessary to prevent the mosquitoes from escaping their cages. Depending on the planned infection regimen, autoclavable and reusable metal-frame cages or self-made disposable cages can be used. The latter ones are recommended if by bite infection of experimental animals is required to be carried out by a defined number of mosquitoes per mouse. If self-made cages are required, prepare cages to exact specifications as the health of the mosquitoes and the safety of the laboratory depends upon their sound construction (Figure 2).

1. Take a carton such as a half-pint ice cream carton or paper coffee cup (Figure 2).
2. Cut a small opening into the side of the carton and cover with a double layer of latex with a slit cut in each piece to create a secure entrance for the mosquitoes. NOTE: The opening has an overall size of 2 cm x 2 cm, the tubing (aspirator device) that we use to bring in and/or take-out mosquitoes is a modified 15 ml Falcon tube attached to a vacuum pump and hence serves as an aspirator with a diameter of 1.5 cm.
3. Tape a piece of filter paper on the inside bottom of the carton to soak up drips.
4. Close off ice cream cups with netting (double layer of Nylon mesh, size 1 mm x 1 mm) and fix to the carton by tape and elastic band.
5. For infection experiments where defined numbers of mosquitoes per mouse are required, prepare cages with 10-15 infected mosquitoes, each of which ideally contains an average of 10,000 wild-type salivary gland P. berghei sporozoites.
6. Ideally, starve mosquitoes for 24 hr prior to performing the blood meal.

4. Malaria Infection of Mice by Mosquito Bite

The rodent malaria parasite used herein is P. berghei however any other rodent Plasmodium strain of interest can be used. To obtain infectious mosquitoes for sporozoite transmission the whole life cycle of the parasite is maintained in both the vertebrate host (mouse) and the mosquito vector. Parasite maintenance is carried out in an insectary. For natural transmission experiments, the minimum number of sporozoites per salivary gland should be no less than 10,000. For detailed protocols on parasite maintenance we refer to Methods in Malaria Research by Moll et al., 2013.

1. Anaesthetize naïve mice or animals preinfected for 40 days with Mtb with Ketamine (100 mg/kg) and Xylazine (7 mg/kg) solution by intraperitoneal injection (200 µl/mouse). NOTE: The time between Mtb and Plasmodium infection can be adjusted depending on the underlying research question. Likewise, the order of pathogen challenges can be reversed, i.e. mice can be exposed to infectious mosquito bite prior to Mtb infection.
2. Place anaesthetized mice onto the netting of the mosquito cages (one mouse per mosquito cage for defined mosquito to mouse ratio) and allow the mosquitoes to feed through the membrane for 10-15 min. NOTE: The presence of blood in the mosquito guts implies feeding and thus, sporozoite transmission.
3. Transfer mice back into their cages and supervise constantly until they wake up from anesthesia. NOTE: Place mice on paper towel and not on bedding (risk of suffocation) and keep warm (place closely together and cover bodies with paper towel).
4. Kill the mosquitoes by spraying them with 70% ethanol or other disinfectants through the netting of the cage. Autoclave cages and discard if disposable ones were used.

5. Monitoring Parasitemia

1. Puncture tail veins at the very end with a needle and collect one drop of blood at each end of a slide.
2. Use another slide to pull one drop of blood over half of the slide's length. Flip over the spreader to use the other edge for the second smear. Leave slides to air dry.
3. Giemsa stain
   1. Place slides in slide holders and fix the blood smears by brief immersion in absolute methanol. NOTE: Because the use of glass ware should be kept at minimum in the BSL 3 we use polypropylene cuvettes for all solutions.
   2. Immerse the smears in Giemsa (1:10 in deionized water). After 10 min, dip the slides in and out of staining cuvettes filled with deionized water a few times to rinse away the excess stain.
   3. Finally, air dry slides in a vertical position.
4. ALTERNATIVE STAIN: Wright´s stain
   1. Dissolve Wright´s stain at a concentration of 1 mg/ml in methanol.
   2. Filter through folded filter prior to use.
   3. Immerse the blood smears in staining solution and incubate for 4 min (NOTE: methanol fixation of smears is not necessary as the staining solution is methanol based).
   4. Wash by rinsing slides in deionized water as described above and leave slides to air dry.
   5. Once Giemsa/Wright´s stain is complete, gently transfer all reagents used into a Buraton-containing disposal pot.
5. Blood smear analysis
   1. Analyze stained blood smears by light microscopy at a 100-fold magnification with oil immersion.
   2. Count uninfected and infected erythrocytes in an area of the blood smear where erythrocytes are arranged in a monolayer.
   3. In order to achieve a well-defined parasitemia, count at least 10 different fields of view displaying an erythrocyte monolayer.
   4. Calculate the relative parasitemia (in %) by dividing the number of parasitized erythrocytes by the number of erythrocytes and multiplying by 100.