Preparation of Digestion-Tracking Bacteria: Difference between revisions
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===New Protocol=== | |||
# Inoculate with the Bacteria Digest 1 (Clone RC-094) bacteria, and grow overnight shaking at 37°C. | ====Materials:==== | ||
# The next morning prepare 40 mL of LB media with 50 µg/mL kanamycin, and inoculate using the whole 4 mL overnight culture prepared in step 2. Incubate, shaking at 37°C, for 1.5 hours. | |||
# At the 1.5 hour mark, add 1 mM IPTG and 25 µM biliverdin. Return to the shaker and incubate at 37°C, for 4 hours. | *One of: | ||
# At 4 hours remove the flask from the shaker. Prepare a serial dilution, and prepare spread plates on LB-Kan of the 10<sup>-9</sup>, 10<sup>-10</sup>, 10<sup>-11</sup>, 10<sup>-12</sup> | **RFP BL21 ''E. coli'' (RC-105, kanamycin resistant) | ||
# Recover the cells by centrifugation, wash once with PBS, and then store in the fridge in 1.5 mL PBS + 25 µM biliverdin. | ** GFP BL21 ''E. coli'' (RC-108, ampicillin resistant) | ||
# The next day use the serial dilution to calculate the CFU/mL in the refrigerator stock. Dilute the stock to 10 x 10<sup>7</sup>/mL in PBS + 20% glycerol, aliquot into PCR tubes (200 µL/tube) and freeze at -80°C until needed. | **GFP + RFP BL21 ''E. coli'' (RC-110, kanamycin + ampicillin resistant) | ||
**RFP+smURF BL21 ''E. coli'' (RC-094, kanamycin resistant) | |||
* LB medium | |||
*1,000X stocks of the appropriate antibiotic(s) | |||
**50 mg/mL kanamycin | |||
** 100 mg/mL ampicillin | |||
*1,000X stock of IPTG (1 M, 0.238g/mL) | |||
*25 mM stock solution of biliverdin if using RC-094 or another smURF containing vector | |||
====Preparing the Bacteria:==== | |||
#Prepare ~2 mL of LB + the appropriate antibiotic(s) at a 1X concentration in a 14 mL snap-cap tube. | |||
#Inoculate with a loop of the desired bacteria from the frozen stock. | |||
#Grow overnight, 37°C, shaking. | |||
#Prepare 2 mL of fresh LB + sufficient antibiotics for 2.5 mL of medium in a 14 mL snap-cap tube. | |||
#Inoculate this new tube with 400 µL of the overnight culture. | |||
#Grow for 1 hr, 37°C, shaking. | |||
#Add 2.5 µL IPTG to the culture. | |||
#*If using a smURF-containing bacteria, add 2.5 µL (25 µM) biliverdin at this time. | |||
#Incubate overnight, 37°C, shaking. | |||
#Make a 1:10 dilution of the bacteria into LB with a minimum volume of 150 µL. Use this to measure the OD<sub>600</sub> of the culture (see '''Table 1'''). | |||
#Remove 1 x 10<sup>8</sup> bacteria from this culture, dilute to 1 mL in PBS, and pellet by centrifugation. Remove the supernatant, resuspend in 1 mL of PBS, and repellet. | |||
#Suspend the bacterial pellet in 700 µL of PBS, and add to this 300 µL of 16% PFA. Incubate at room temperature, in the dark, for 30 min. | |||
#Pellet by centrifugation, remove the supernatant, resuspend in 1 mL of PBS, and repellet. | |||
#Resuspend in 1 mL of PBS (e.g. 1 x 10<sup>8</sup> bacteria/mL). Store at 4°C, wrapped in foil, for up to 1 week. | |||
#Bacteria are typically added to phagocytosis assays at a rate of 10-30/macrophage, or 10,000-30,000 per mm<sup>2</sup> ('''Table 2'''). | |||
#*Add desired number of bacteria into the dish/well. | |||
#*Mix gently with a pipette to distribute the bacteria evenly. | |||
#*If synchronized phagocytosis is required, spin at ~250 x g, 1 min, in the centrifuge. | |||
#*Proceed with assay as required. | |||
{| class="wikitable" | |||
|+'''Table 1:''' '''CFU/OD600 of Various Bacterial Strains''' | |||
!Bacteria | |||
!Stock | |||
!CFU/mL/OD<sub>600</sub> | |||
|- | |||
|DH5α | |||
| -- | |||
|2.7 x 10<sup>9</sup> CFU/mL/OD<sub>600</sub> | |||
|- | |||
|BL21 | |||
| -- | |||
|8.0 x 10<sup>8</sup> CFU/mL/OD<sub>600</sub> | |||
|- | |||
|RFP | |||
|RC-105 | |||
|1.6 x 10<sup>8</sup> CFU/mL/OD<sub>600</sub> | |||
|- | |||
|GFP | |||
|RC-108 | |||
|* | |||
|- | |||
|GFP+RFP | |||
|RC-110 | |||
|4.4 x 10<sup>8</sup> CFU/mL/OD<sub>600</sub> | |||
|- | |||
|RFP+smURF | |||
|RC-094 | |||
|* | |||
|} | |||
''*Not yet determined'' | |||
{| class="wikitable" | |||
|+Table 2: Common Bacterial Additions for Phagocytosis Assays | |||
!Chamber | |||
!Well diameter/side | |||
!Well area | |||
!Low (10k/mm<sup>2</sup>) | |||
!High (30k/mm<sup>2</sup>) | |||
|- | |||
|12-well plate | |||
|18 mm (coverslip) | |||
|~250 mm<sup>2</sup> | |||
|2.5 x 10<sup>6</sup> | |||
|7.5 x 10<sup>6</sup> | |||
|- | |||
|35 mm dish | |||
|34.4 mm (dish) | |||
|930 mm<sup>2</sup> | |||
|9.3 x 10<sup>6</sup> | |||
|2.8 x 10<sup>7</sup> | |||
|- | |||
|µ-Slide 18 Well | |||
|5.7 x 6.1 mm | |||
|35 mm<sup>2</sup> | |||
|350,000 | |||
|1.0 x 10<sup>6</sup> | |||
|- | |||
|21-well chamber | |||
|5 mm | |||
|20 mm<sup>2</sup> | |||
|200,000 | |||
|600,000 | |||
|- | |||
|32-well chamber | |||
|4.5 mm | |||
|16 mm<sup>2</sup> | |||
|160,000 | |||
|480,000 | |||
|- | |||
|36-well chamber | |||
|4.0 mm | |||
|12.6 mm<sup>2</sup> | |||
|126,000 | |||
|378,000 | |||
|} | |||
---- | |||
===Old Protocol=== | |||
#Measure out 4 mL of LB media and add kanamycin to a final concentration of 50 µg/mL. | |||
#Inoculate with the Bacteria Digest 1 (Clone RC-094) bacteria, and grow overnight shaking at 37°C. | |||
#The next morning prepare 40 mL of LB media with 50 µg/mL kanamycin, and inoculate using the whole 4 mL overnight culture prepared in step 2. Incubate, shaking at 37°C, for 1.5 hours. | |||
#At the 1.5 hour mark, add 1 mM IPTG and 25 µM biliverdin. Return to the shaker and incubate at 37°C, for 4 hours. | |||
#At 4 hours remove the flask from the shaker. Prepare a serial dilution, and prepare spread plates on LB-Kan of the 10<sup>-9</sup>, 10<sup>-10</sup>, 10<sup>-11</sup>, 10<sup>-12</sup> | |||
#Recover the cells by centrifugation, wash once with PBS, and then store in the fridge in 1.5 mL PBS + 25 µM biliverdin. | |||
#The next day use the serial dilution to calculate the CFU/mL in the refrigerator stock. Dilute the stock to 10 x 10<sup>7</sup>/mL in PBS + 20% glycerol, aliquot into PCR tubes (200 µL/tube) and freeze at -80°C until needed. | |||
To use Digestion-Tracking Bacteria in a phagocytosis assay: | To use Digestion-Tracking Bacteria in a phagocytosis assay: | ||
# Split MH-S cells onto coverslips (250,000 cells/well), and let recover overnight in 37°C incubator. | #Split MH-S cells onto coverslips (250,000 cells/well), and let recover overnight in 37°C incubator. | ||
# The next morning, discard the media in the wells and replace with 400 μL fresh RPMI media, with 6 μL antibiotic antimycotic solution (10,000 IU/mL penicillin, 10,000 μg/mL streptomycin, 25 μg/mL amphotericin B) | #The next morning, discard the media in the wells and replace with 400 μL fresh RPMI media, with 6 μL antibiotic antimycotic solution (10,000 IU/mL penicillin, 10,000 μg/mL streptomycin, 25 μg/mL amphotericin B) | ||
# | #Thaw 1 tube of Digest Tracking bacteria and add entire tube to a 1.5 mL centrifuge tube. Fill the rest of the tube’s volume with PBS. | ||
# Centrifuge tube at 21,100 g for 3 minutes. | #Centrifuge tube at 21,100 g for 3 minutes. | ||
# Carefully remove supernatant and resuspend pellet in 200 μL imaging buffer. | #Carefully remove supernatant and resuspend pellet in 200 μL imaging buffer. | ||
# Add entire tube to coverslip, and live cell image. | #Add entire tube to coverslip, and live cell image. | ||
Latest revision as of 13:31, 18 May 2023
New Protocol
Materials:
- One of:
- RFP BL21 E. coli (RC-105, kanamycin resistant)
- GFP BL21 E. coli (RC-108, ampicillin resistant)
- GFP + RFP BL21 E. coli (RC-110, kanamycin + ampicillin resistant)
- RFP+smURF BL21 E. coli (RC-094, kanamycin resistant)
- LB medium
- 1,000X stocks of the appropriate antibiotic(s)
- 50 mg/mL kanamycin
- 100 mg/mL ampicillin
- 1,000X stock of IPTG (1 M, 0.238g/mL)
- 25 mM stock solution of biliverdin if using RC-094 or another smURF containing vector
Preparing the Bacteria:
- Prepare ~2 mL of LB + the appropriate antibiotic(s) at a 1X concentration in a 14 mL snap-cap tube.
- Inoculate with a loop of the desired bacteria from the frozen stock.
- Grow overnight, 37°C, shaking.
- Prepare 2 mL of fresh LB + sufficient antibiotics for 2.5 mL of medium in a 14 mL snap-cap tube.
- Inoculate this new tube with 400 µL of the overnight culture.
- Grow for 1 hr, 37°C, shaking.
- Add 2.5 µL IPTG to the culture.
- If using a smURF-containing bacteria, add 2.5 µL (25 µM) biliverdin at this time.
- Incubate overnight, 37°C, shaking.
- Make a 1:10 dilution of the bacteria into LB with a minimum volume of 150 µL. Use this to measure the OD600 of the culture (see Table 1).
- Remove 1 x 108 bacteria from this culture, dilute to 1 mL in PBS, and pellet by centrifugation. Remove the supernatant, resuspend in 1 mL of PBS, and repellet.
- Suspend the bacterial pellet in 700 µL of PBS, and add to this 300 µL of 16% PFA. Incubate at room temperature, in the dark, for 30 min.
- Pellet by centrifugation, remove the supernatant, resuspend in 1 mL of PBS, and repellet.
- Resuspend in 1 mL of PBS (e.g. 1 x 108 bacteria/mL). Store at 4°C, wrapped in foil, for up to 1 week.
- Bacteria are typically added to phagocytosis assays at a rate of 10-30/macrophage, or 10,000-30,000 per mm2 (Table 2).
- Add desired number of bacteria into the dish/well.
- Mix gently with a pipette to distribute the bacteria evenly.
- If synchronized phagocytosis is required, spin at ~250 x g, 1 min, in the centrifuge.
- Proceed with assay as required.
| Bacteria | Stock | CFU/mL/OD600 |
|---|---|---|
| DH5α | -- | 2.7 x 109 CFU/mL/OD600 |
| BL21 | -- | 8.0 x 108 CFU/mL/OD600 |
| RFP | RC-105 | 1.6 x 108 CFU/mL/OD600 |
| GFP | RC-108 | * |
| GFP+RFP | RC-110 | 4.4 x 108 CFU/mL/OD600 |
| RFP+smURF | RC-094 | * |
*Not yet determined
| Chamber | Well diameter/side | Well area | Low (10k/mm2) | High (30k/mm2) |
|---|---|---|---|---|
| 12-well plate | 18 mm (coverslip) | ~250 mm2 | 2.5 x 106 | 7.5 x 106 |
| 35 mm dish | 34.4 mm (dish) | 930 mm2 | 9.3 x 106 | 2.8 x 107 |
| µ-Slide 18 Well | 5.7 x 6.1 mm | 35 mm2 | 350,000 | 1.0 x 106 |
| 21-well chamber | 5 mm | 20 mm2 | 200,000 | 600,000 |
| 32-well chamber | 4.5 mm | 16 mm2 | 160,000 | 480,000 |
| 36-well chamber | 4.0 mm | 12.6 mm2 | 126,000 | 378,000 |
Old Protocol
- Measure out 4 mL of LB media and add kanamycin to a final concentration of 50 µg/mL.
- Inoculate with the Bacteria Digest 1 (Clone RC-094) bacteria, and grow overnight shaking at 37°C.
- The next morning prepare 40 mL of LB media with 50 µg/mL kanamycin, and inoculate using the whole 4 mL overnight culture prepared in step 2. Incubate, shaking at 37°C, for 1.5 hours.
- At the 1.5 hour mark, add 1 mM IPTG and 25 µM biliverdin. Return to the shaker and incubate at 37°C, for 4 hours.
- At 4 hours remove the flask from the shaker. Prepare a serial dilution, and prepare spread plates on LB-Kan of the 10-9, 10-10, 10-11, 10-12
- Recover the cells by centrifugation, wash once with PBS, and then store in the fridge in 1.5 mL PBS + 25 µM biliverdin.
- The next day use the serial dilution to calculate the CFU/mL in the refrigerator stock. Dilute the stock to 10 x 107/mL in PBS + 20% glycerol, aliquot into PCR tubes (200 µL/tube) and freeze at -80°C until needed.
To use Digestion-Tracking Bacteria in a phagocytosis assay:
- Split MH-S cells onto coverslips (250,000 cells/well), and let recover overnight in 37°C incubator.
- The next morning, discard the media in the wells and replace with 400 μL fresh RPMI media, with 6 μL antibiotic antimycotic solution (10,000 IU/mL penicillin, 10,000 μg/mL streptomycin, 25 μg/mL amphotericin B)
- Thaw 1 tube of Digest Tracking bacteria and add entire tube to a 1.5 mL centrifuge tube. Fill the rest of the tube’s volume with PBS.
- Centrifuge tube at 21,100 g for 3 minutes.
- Carefully remove supernatant and resuspend pellet in 200 μL imaging buffer.
- Add entire tube to coverslip, and live cell image.