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

Latest 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 1^st 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 2^nd 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

@@ Line 20: / Line 20: @@
 ==== '''Day1:''' ====
-==== Seed HEK293T cells 1:40 in 6 well plate. 1 well for each transfection approach ====
+* Seed HEK293T cells 1:40 in 6 well plate. 1 well for each transfection approach
 ==== '''Day2:''' ====
@@ Line 36: / Line 36: @@
 ==== '''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

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

Latest revision as of 09:47, 20 May 2025

Contents

Procedure

Day1:

Day2:

Day3:

Day4:

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

Latest revision as of 09:47, 20 May 2025

Procedure

Day1:

Day2:

Day3:

Day4:

Navigation menu

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