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methods:protocols:protocolimmunofluorenceperirhinalcortex

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methods:protocols:protocolimmunofluorenceperirhinalcortex [2024/04/03 05:08] igrovesmethods:protocols:protocolimmunofluorenceperirhinalcortex [2024/04/03 05:16] (current) igroves
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 //Example//: 1L of TBS X1 = 100ml of TBS X10 + 900ml dH20 //Example//: 1L of TBS X1 = 100ml of TBS X10 + 900ml dH20
  
-TBSTTBS X1 + 0.2% of Triton X100. Mix well.+TBST TBS X1 + 0.2% of Triton X100. Mix well.
 //Example//: 100ml of TBST = 200μl Triton X100 + 100ml of TBS X1 //Example//: 100ml of TBST = 200μl Triton X100 + 100ml of TBS X1
  
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 **DAY 1:** **DAY 1:**
  
-  - Step 1: Gather desired slides into a 4x6 well plate. Cut a transfer pipette to allow wider width and use this to collect slides and anti-freeze from storage well plates to working well plate. Have two wells designated as controls, one without primary antibody, one without secondary antibody. +  - Gather desired slides into a 4x6 well plate. Cut a transfer pipette to allow wider width and use this to collect slides and anti-freeze from storage well plates to working well plate. Have two wells designated as controls, one without primary antibody, one without secondary antibody. 
- +  - Wash slides in TBST for 10 min, 3 times on agitator (room temp.). Remove the liquid from each well with a thinned transfer pipette and then fill the wells around half way (~1ml) with TBST. 
-  - Step 2: Wash slides in TBST for 10 min, 3 times on agitator (room temp.). Remove the liquid from each well with a thinned transfer pipette and then fill the wells around half way (~1ml) with TBST. +  - Block in TBST + NDS (1ml/well) for 60 min on agitator in fridge. 
- +  - While waiting for block, prepare primary antibody. c-Fos antibody 1/8000 concentration in TBST + NDS (1/8000 = 0.125μl of primary in 1ml of TBST + NDS. //Example:// 36 wells = 0.125μl * 36 = 4.5μl of primary + (36000μl – 4.5μl) 35995.5μl of TBST + NDS = TOTAL volume of 36000μl (36ml). 
-  - Step 3: Block in TBST + NDS (1ml/well) for 60 min on agitator in fridge. +  - Remove block and then add in solution containing primary antibody (1ml/well) to all wells except for primary control (add in TBST + NDS to control well). Leave in fridge on very slow agitation overnight (not 24 h later). 
- + 
-  - Step 4: While waiting for block, prepare primary antibody. c-Fos antibody 1/8000 concentration in TBST + NDS (1/8000 = 0.125μl of primary in 1ml of TBST + NDS. +
-//Example:// 36 wells = 0.125μl * 36 = 4.5μl of primary + (36000μl – 4.5μl) 35995.5μl of TBST + NDS = TOTAL volume of 36000μl (36ml). +
- +
-  - Step 5: Remove block and then add in solution containing primary antibody (1ml/well) to all wells except for primary control (add in TBST + NDS to control well). Leave in fridge on very slow agitation overnight (not 24 h later). +
  
 **DAY 2:** **DAY 2:**
  
-  - Step 1: Wash slides in TBST for 10 min, 3 times on agitator (room temp.). Remove the liquid from each well with a thinned transfer pipette and then fill the wells around half way (~1ml) with TBST. +  - Wash slides in TBST for 10 min, 3 times on agitator (room temp.). Remove the liquid from each well with a thinned transfer pipette and then fill the wells around half way (~1ml) with TBST. 
- +  -  Prepare secondary antibody. Donkey anti-Rabbit, Alexa 488 1/200 concentration in TBST (1/200 = 5ul of secondary in 1ml of TBST) //Example:// 36 wells = 5μl * 36 = 180μl of primary + (36000μl – 180μl) 35820μl of TBST = TOTAL volume of 36000μl (36ml).NOTE: Alexa 488 is light-sensitive, prepare solutions in dark and hold in a falcon tube covered in aluminium foil. 
-  - Step 2: Prepare secondary antibody. Donkey anti-Rabbit, Alexa 488 1/200 concentration in TBST (1/200 = 5ul of secondary in 1ml of TBST) +  - Remove TBST and introduce solution secondary antibody (1ml/well) to all wells except for secondary control (add in TBST to this control well). Cover plate in foil and put on slow agitation in the fridge for 1 h. 
-//Example:// 36 wells = 5μl * 36 = 180μl of primary + (36000μl – 180μl) 35820μl of TBST = TOTAL volume of 36000μl (36ml). +  - In a dark room wash slides in TBS for 10 min, 3 times on agitator (room temp.). Remove the liquid from each well with a thinned transfer pipette and then fill the wells around half way (~1ml) with TBS. 
-NOTE: Alexa 488 is light-sensitive, prepare solutions in dark and hold in a falcon tube covered in aluminium foil. +  - Fill a flat circular dish with TBS and transfer the desired slides (one well at a time) into the container. From there, mount slides onto a gelled microscope slide. Add Fluromount-G+DAPI (kept in fridge – about 1 drop per tissue section) and then place a coverslip on top. Allow slide to dry in a dark place. When ready, place slides in slide holder and store in fridge until imaging.
- +
-  - Step 3: Remove TBST and introduce solution secondary antibody (1ml/well) to all wells except for secondary control (add in TBST to this control well). Cover plate in foil and put on slow agitation in the fridge for 1 h. +
- +
-  - Step 4: In a dark room wash slides in TBS for 10 min, 3 times on agitator (room temp.). Remove the liquid from each well with a thinned transfer pipette and then fill the wells around half way (~1ml) with TBS. +
- +
-  - Step 5: Fill a flat circular dish with TBS and transfer the desired slides (one well at a time) into the container. From there, mount slides onto a gelled microscope slide. Add Fluromount-G+DAPI (kept in fridge – about 1 drop per tissue section) and then place a coverslip on top. Allow slide to dry in a dark place. When ready, place slides in slide holder and store in fridge until imaging.+
  
  
  
methods/protocols/protocolimmunofluorenceperirhinalcortex.1712135310.txt.gz · Last modified: 2024/04/03 05:08 by igroves