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Revision as of 13:24, 12 September 2008

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Checking our ligases

Because we couldn't be sure of the results of yesterday experiment, we decided to carry it out one more time.

Digestion

Before excision

After ecxision

DNA used for digestion: MP101
2 digestion were carried out:

one with EcoRI (D202), that cuts the plasmid only one time
the other with BspHI (D203), that cuts the plasmid three times

Reaction mixture

10 µL of DNA
6µL of 10X buffer 2
0,6 µL of 100X BSA
2 µL of enzyme (EcoRI or BspHI)
41,4 µL of water

2h30 at 37°C and then 20 min at 65°C

well n°	1	2	3	4	5	6	7	8
sample	1 kb ladder	MP101 1 µL		D202 10 µL	D202 10 µL		D203 3 µL	100 bp ladder
expected size				2984 bp			1870 bp 1008 bp 105 bp
measured size				3 kb	3 kb		1,9 kb 1 kb

Purification

After purification
well n°2: D202 purified by gel
well n°3: D202 purified by column
well n°4: D203 purified by column
well n°5: MP101

D202 (EcoRI digestion) was purified in 2 ways:

by gel extraction
or by column

D203 (BspHI digestion) was purified:

by column

Elution in 30 µL of EB buffer

Ligation

3 ligases tested

ligase 1: our 250 µL (400 000 U/mL) tube
ligase 2: our 50 µL (400 000 U/mL) tube
ligase 3: 2nd floor 50 µL (400 000 U/mL) tube

Reaction mixture

For the samples for which the digestion products have not been purified, 1 µL of ligase and 1 µL of ATP (1 mM final concentration) have been added directly in the digestion products (in the digestion buffer 2). All the ligation were carried out overnight at 4°C.

ligation

1

2

3

4

5

6

7

8

9

10

11

12

13

digested DNA used

D202 (EcoRI digestion)

D203 (BspHI digestion)

type of purification
of the digestion products

gel extraction

column

no
purification