Team:UNICAMP-EMSE Brazil/protocols/Ligation

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Revision as of 15:18, 27 September 2011

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Ligation:

Quantificate the plasmid using absorbance at 260 nm and 280 nm.
Concentration of plasmid (μg/mL) = A260*50*dilution
Ratio 260/280 nm should be between 1,8-2,0.

Use [http://www.promega.com/techserv/tools/biomath/calc06.htm this online tool] to calculate how much insert to calculate how much insert we will need to use in the reaction (http://www.promega.com/techserv/tools/biomath/calc06.htm).

Or

[length of insert (kb)/ length of vector (kb)]* ng of vector = ng of insert for a 1:1 ratio

It´s better to use at least 100 ng of vector and a reaction ratio of 3:1 (insert:vector)

Example:

Length of insert (in kb) = 0.7
Amount of vector (in ng) = 100
Length of vector (in kb) = 5

You need 14 ng de insert for a 1:1 molar ratio
For the 3:1= 42 ng de inserto.

Ligation (protocol adapted from Fermentas)

-Plasmid (~50-60ng) -Insert DNA purified (the ratio was determined according to the fragment and plasmid sizes, ranging from 1:1 to 1:4) - 2μl of T4 DNA Ligase Buffer - 1μl of T4 DNA Ligase - Sterile water ___________ 20μl

Add the reaction components to a sterile 0,2 sterile tube. Mix gently.

Keep the tubes at 22˚C for 1 hour or overnight at 4˚C.

@@ Line 30: / Line 30: @@
 ::*For the 3:1= 42 ng de inserto.
-===Ligation reaction (using invitrogen ligase)===
-*5x T4 DNA Ligase - 4uL
+===Ligation (protocol adapted from Fermentas)===
-*Vector – 42 ng
-*Insert – 100 ng
+-Plasmid (~50-60ng)
-*T4 DNA Ligase – 1 uL
+-Insert DNA purified (the ratio was determined according to the fragment and plasmid sizes, ranging from 1:1 to 1:4)
-*Final Volume - 20ul
+- 2μl of T4 DNA Ligase Buffer
+- 1μl of T4 DNA Ligase
+- Sterile water
+___________
+μl
+Add the reaction components to a sterile 0,2 sterile tube. Mix gently.
+Keep the tubes at 22˚C for 1 hour or overnight at 4˚C.