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--- protein_electrophoresis [2023/06/16 04:40] – quality_manager
+++ protein_electrophoresis [2025/01/08 16:15] (current) – external edit 127.0.0.1
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 [[quality_manual|QM home]]
 ^Name^Unique ID^Edition^Date of Edition^
-|Documentary procedure for protein electrophoresis|LSSTH/A/QM/01| 1 | 01-03-2023|
+|Documentary procedure for protein electrophoresis|LSSTH/A/QM/01| 1 | 15-06-2023|
 ^Preparing authority^Approving authority^Review period^
@@ Line 32: / Line 32: @@
 [[5% glacial acetic acid]]
+[[Sample Preparation]]
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 **Gel preparation**
-Clean the glass slide with tape water and and dry it with tissue paper.
-Cut a rectangle four borders from Xray plate and Stick Xray plate to periphery of glass slide so the thickness of gel is same as thickness of Xray plate.
+  - Clean the glass slide with tape water and and dry it with tissue paper.
+  - Cut a rectangle four borders from X-ray plate and Stick X-ray plate with feviquick to the periphery of glass slide so the thickness of gel is same as thickness of X-ray plate.
+  - Prepare 1% Agarose and pour hot agarose gel to non siliconized rough glass slide.
+  - Cover the gel with [[siliconized glass]] slide carefully without entrapping air bubbles.
+  - Allow the gel to get solidify for 10 minutes.
+  - After 10 minutes removes siliconized glass slide by sliding movement and take care so that gel does not broken down.
+  - Gel is ready for sample application.
+  - Immediately apply the sample to prevent excess drying.
+**Sample Applicator Preparation**
+Prepare comb from the stainless steel as shown in image.
+Attach the magnetic strip to the ruler.
+Stick the ruler with the platform by feviquick.
+Stick the Applicator to magnetic strip. Applicator can be move up and down.
+**Sample application**
+  - Put Rough non sliconized glass slide below the sample applicator.
+  - Apply 4 micro liter sample over the sample applicator at the edge of applicator as shown in figure. so that excess sample will be removed on glass slide.
+  - Lift up the sample applicator and wipe the back side of applicator so that backward running of sample can be prevented.
+  - Replace the rough glass slide with glass slide having prepared gel.
+  - Apply the sample near the one end of gel with the applicator and wait for 2 minutes to allow the samples to get completely absorbed within the gel.
+  - Remove the applicator.
+**Running the samples in electrophoresis tank**
+  - Clean the electrophoresis tank with DI water and dry it with tissue paper before use.
+  - Put the electrophoresis tank on a table having even & leveled surface.
+  - Fill the cold buffer in the two compartment. Put the gel slide in electrophoresis chamber in such a way that sample applied should remain on cathodic side.
+  - Connect the gel with buffer through strip of filter paper wick & cover the chamber with its lid.
+  - Connect the electrode on the side of slide containing sample well to the cathode (-) & other electrode to the anode of the power supply.
+  - Set voltage at 300 volt and & run for 10 minutes.
+  - After 10 minutes,switch off the power supply & remove the slide.
+**Fixation**
+Put the slide in to methanol for 10 minutes for fixation so that proteins get denatured and remain at same position even after staining and destaining.
+**Drying of gel**
+Put the fixated glass slide in to hot air Owen at 50-60° C for 20 minutes.
+**Staining**
+Place the gel slide in to Amido black staining solution for 2 minutes.
+**Destaining**
+Remove the excess stain by putting the gel in to destaining solution for 15 minutes so that background becomes clear.
+**Interpretation of the  result**