OPTIC (Opa protein triggered integrin clustering): Difference between revisions

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Created page with "{| class="wikitable" |+ !Materials |- |1x PBS |- |Trypsin/EDTA |- |GC-Agar plates with CAM/ERM and without antibiotics Coverslips (round, 12 mm) |- |24 well plate |- |HEK culture medium (DMEM + 10% CS) Suspension medium (DMEM + 0.25% BSA) 4% paraformaldehyde (PFA) in PBS |- |Permeabilization solution (0.4% Triton-X-100 in PBS) Blocking solution (10% heat inactivated CS in PBS) Mounting medium |} === Procedure === ==== '''Day1:''' ==== ==== Seed HEK293T cells 1:40 in 6..."
 
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==== '''Day4:''' ====
==== '''Day4:''' ====
§   In the morning seed 2*10^5 HEK cells on coated coverslips in suspension medium and let adhere for 2h.


§   In the meantime resuspend bacteria from plate in 1ml 1xPBS and stain with pacific blue (1:1000, 30 min, 37°C). Wash 3x with PBS and determine cell number using the formula: OD550 x 8.6 x 10^7 bacteria/ml
* In the morning seed 2*10^5 HEK cells on coated coverslips in suspension medium and let adhere for 2h.
 
* In the meantime resuspend bacteria from plate in 1ml 1xPBS and stain with pacific blue (1:1000, 30 min, 37°C). Wash 3x with PBS and determine cell number using the formula: OD550 x 8.6 x 10^7 bacteria/ml
§   After 2h infect HEK cells with MOI 20-50 in suspension medium for 1h at 37°C
* After 2h infect HEK cells with MOI 20-50 in suspension medium for 1h at 37°C
 
* After infection remove medium and fix cells with 4% PFA/PBS
§   After infection remove medium and fix cells with 4% PFA/PBS
* Wash 3x with PBS
 
* Add 300 µl of permeabilization solution and incubate for 6 min
§   Wash 3x with PBS
* Wash 3x with PBS
 
* Add 300 µl of blocking solution, incubate for 10 min.
§   Add 300 µl of permeabilization solution and incubate for 6 min
* Add 25 µl of 1<sup>st</sup> antibody at appropriate dilution in blocking solution. Apply to the center of the coverslip (make sure coverslip does not touch wall of the well)
 
* Incubate for 1h in humidified chamber
§   Wash 3x with PBS
* Wash 3x with PBS
 
* Add 300 µl of blocking solution and incubate 10 min
§   Add 300 µl of blocking solution, incubate for 10 min.
* Add 25µl of 2<sup>nd</sup> antibody at appropriate dilution in blocking solution in the center of the coverslip (make sure that coverslips does not touch wall of the well)
 
* Incubate for 45 min in humidified chamber
§   Add 25 µl of 1<sup>st</sup> antibody at appropriate dilution in blocking solution. Apply to the center of the coverslip (make sure coverslip does not touch wall of the well)
* Wash 3x with PBS
 
* Transfer coverslips to microscope slide (mounting medium from Dako)
§   Incubate for 1h in humidified chamber
* Analyze at confocal microscope
 
§   Wash 3x with PBS
 
§   Add 300 µl of blocking solution and incubate 10 min
 
§   Add 25µl of 2<sup>nd</sup> antibody at appropriate dilution in blocking solution in the center of the coverslip (make sure that coverslips does not touch wall of the well)
 
§   Incubate for 45 min in humidified chamber
 
§   Wash 3x with PBS
 
§   Transfer coverslips to microscope slide (mounting medium from Dako)
 
§   Analyze at confocal microscope

Revision as of 09:47, 20 May 2025

Materials
1x PBS
Trypsin/EDTA
GC-Agar plates with CAM/ERM and without antibiotics Coverslips (round, 12 mm)
24 well plate
HEK culture medium (DMEM + 10% CS) Suspension medium (DMEM + 0.25% BSA) 4% paraformaldehyde (PFA) in PBS
Permeabilization solution (0.4% Triton-X-100 in PBS) Blocking solution (10% heat inactivated CS in PBS) Mounting medium

Procedure

Day1:

Seed HEK293T cells 1:40 in 6 well plate. 1 well for each transfection approach

Day2:

  • Prepare transfection approach according to transfection protocol for HEK cells described previously.
  • Use 2.5 µg of the OPTIC receptor construct or the control plasmid + 2.5 µg of the cytoplasmic protein of interest.
  • Add 2 µl of chloroquine to the cells and transfect cells with 200 µl of the transfection approach.
  • Exchange medium after 6-8h
  • In the evening streak out N. gonorrhoeae (N309) on GC agar plates containing Chloramphenicol and Erythromycin using a three eyelet smear

Day3:

  • Coat coverslips in 24 well plate with poly L-Lysine (10 µg/ml) and incubate over night at 4°C
  • In the afternoon, not more than 24 h after plating the bacteria, select a number of opaque colonies and streak them further on GC agar w/o antibiotics

Day4:

  • In the morning seed 2*10^5 HEK cells on coated coverslips in suspension medium and let adhere for 2h.
  • In the meantime resuspend bacteria from plate in 1ml 1xPBS and stain with pacific blue (1:1000, 30 min, 37°C). Wash 3x with PBS and determine cell number using the formula: OD550 x 8.6 x 10^7 bacteria/ml
  • After 2h infect HEK cells with MOI 20-50 in suspension medium for 1h at 37°C
  • After infection remove medium and fix cells with 4% PFA/PBS
  • Wash 3x with PBS
  • Add 300 µl of permeabilization solution and incubate for 6 min
  • Wash 3x with PBS
  • Add 300 µl of blocking solution, incubate for 10 min.
  • Add 25 µl of 1st antibody at appropriate dilution in blocking solution. Apply to the center of the coverslip (make sure coverslip does not touch wall of the well)
  • Incubate for 1h in humidified chamber
  • Wash 3x with PBS
  • Add 300 µl of blocking solution and incubate 10 min
  • Add 25µl of 2nd antibody at appropriate dilution in blocking solution in the center of the coverslip (make sure that coverslips does not touch wall of the well)
  • Incubate for 45 min in humidified chamber
  • Wash 3x with PBS
  • Transfer coverslips to microscope slide (mounting medium from Dako)
  • Analyze at confocal microscope
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