Latest revision as of 14:23, 4 October 2013

Ethanol precipitation

This method is used to purify and/or concentrate DNA, RNA and polysaccarides.

Protocol :

1. Measure the volume of the DNA sample.

2. Add 3x volumes of ethanol 100%

3. Add 1/10x volume of sodium acetate (3 M, pH 5.2)

4. Add 1µL of glycogen

5. Incubate the solution at -20°C for 30min or more

6. Centrifuge at > 14,000 x g for 30min at 4°C

7. Discard supernatant being careful not to throw out DNA pellet which may or may not be visible.

8. Wash with 1mL of ethanol 70%

9. Centrifuge at > 14,000 x g for 15min at 4°C

10. Discard supernatant, air dry pellet and dissolve pellet in desired buffer or water

@@ Line 4: / Line 4: @@
 This method is used to purify and/or concentrate DNA, RNA and polysaccarides.
-Add in a volume of DNA :
+'''Protocol :'''
-.	3 volumes of ethanol 100%
+.	Measure the volume of the DNA sample.
-.	1/10 of volume of sodium acetate 3M
+.      Add 3x volumes of ethanol 100%
-.	1µL of glycogen
+.	Add 1/10x volume of sodium acetate (3 M, pH 5.2)
-.	Let the solution at -20°C during 30min
+.	Add 1µL of glycogen
-.	Centrifuge at maximal speed during 30min at 4°C
+.	Incubate the solution at -20°C for 30min or more
-.	Put away the supernatant
+.	Centrifuge at > 14,000 x g for 30min at 4°C
-.	Wash with 1mL of ethanol 70%
+.	Discard supernatant being careful not to throw out DNA pellet which may or may not be visible.
-.	Centrifuge 10-15 min at 4°C
+.	Wash with 1mL of ethanol 70%
-.	Put away the supernatant, dry (speed vacuum 4 min)
+.	Centrifuge at > 14,000 x g for 15min at 4°C
-.	Repeat with water or TE
+.	Discard supernatant, air dry pellet and dissolve pellet in desired buffer or water