Team:Lyon-INSA-ENS/Realisation/Protocols/CaCl2 trans

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(Difference between revisions)

Latest revision as of 10:18, 10 January 2012

CaCl2 chemical transformation

This protocol aims at inserting plasmids notably into NM522 strains, or any other E.Coli strain

It has been found less efficient than the TSS transformation protocol, thus we do not recommend using it.

Procedure

1. Monitor the OD600 of a 50mL culture of NM522 cells ( or the strain you want to transform ) in LB medium at 37°C. Proceed to the next step when it reaches 0.2-0.4 ( not higher than 0.6 ), which takes approximately 3 hours.

2. Aliquot the culture into fractions of the desired volume V ( 10 or 15 mL usually ).

3. Incubate on ice for 10mn

4. Centrifuge at 4°C, 10mn, 5000rpm

5. Empty the supernatant

6. Add V/2 mL cold and sterile CaCl2 100mM

7. Incubate for 20mn on ice

8. Centrifuge at 4°C, 5mn, 5000rpm

9. Empty the supernatant and resuspend ( do not vortex ) in V/15 mL CaCl2 and V/30 mL glycerol 40%

10. Aliquot the bacteria in 200 µL fractions and keep on ice. These bacteria should be used within the day.

11. Add the desired quantity of DNA to the fractions. For positive control, we used Puc18 plasmid. For negative control, we used water.

12. Incubate for 30mn on ice

13. Heat shock at 42°C for 2mn

14. Incubate for 5mn on ice

15. Add 800µL of LB medium and incubate for 1h at 37°C

16.Optional Concentrate 10X by centrifuging for 2mn at 11000 rpm, eliminate the supernatant and resuspend in 100µL LB.

17. Plate 100µL of bacteria on LB medium with the appropriate antibiotic resistance and incubate at 37°C.

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      <p style="line-height : 1.5em">
+This protocol aims at inserting plasmids notably into NM522 strains, or any other E.Coli strain
      </p>
      <p style="line-height : 1.5em">
+It has been found less efficient than the TSS transformation protocol, thus we do not recommend using it.
      </p>
@@ Line 32: / Line 32: @@
      <p style="line-height : 1.5em">
-<b>1.</b>
+<b>1.</b> Monitor the OD600 of a 50mL culture of NM522 cells ( or the strain you want to transform ) in LB medium at 37°C. Proceed to the next step when it reaches 0.2-0.4 ( not higher than 0.6 ), which takes approximately 3 hours.
      <p/>
@@ Line 38: / Line 38: @@
      <p style="line-height : 1.5em">
-<b>2.</b>
+<b>2.</b> Aliquot the culture into fractions of the desired volume V ( 10 or 15 mL usually ).
      </p>
@@ Line 44: / Line 44: @@
      <p style="line-height : 1.5em">
-<b>3.</b>
+<b>3.</b> Incubate on ice for 10mn
      </p>
@@ Line 50: / Line 50: @@
      <p style="line-height : 1.5em">
-<b>4.</b>
+<b>4.</b> Centrifuge at 4°C, 10mn, 5000rpm
      </p>
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      <p style="line-height : 1.5em">
-<b>5.</b>
+<b>5.</b> Empty the supernatant
      </p>
@@ Line 62: / Line 62: @@
      <p style="line-height : 1.5em">
-<b>6.</b>
+<b>6.</b> Add V/2 mL cold and sterile CaCl2 100mM
      </p>
@@ Line 68: / Line 68: @@
      <p style="line-height : 1.5em">
-<b>7.</b>
+<b>7.</b> Incubate for 20mn on ice
      </p>
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      <p style="line-height : 1.5em">
-<b>8.</b>
+<b>8.</b> Centrifuge at 4°C, 5mn, 5000rpm
      </p>
@@ Line 80: / Line 80: @@
      <p style="line-height : 1.5em">
-<b>9.</b>
+<b>9.</b> Empty the supernatant and resuspend ( do not vortex ) in V/15 mL CaCl2 and V/30 mL glycerol 40%
      </p>
@@ Line 86: / Line 86: @@
      <p style="line-height : 1.5em">
-<b>10.</b>
+<b>10.</b> Aliquot the bacteria in 200 µL fractions and keep on ice. These bacteria should be used within the day.
      </p>
@@ Line 92: / Line 92: @@
      <p style="line-height : 1.5em">
-<b>11.</b>
+<b>11.</b> Add the desired quantity of DNA to the fractions. For positive control, we used Puc18 plasmid. For negative control, we used water.
      </p>
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      <p style="line-height : 1.5em">
-<b>12.</b>
+<b>12.</b> Incubate for 30mn on ice
      </p>
@@ Line 104: / Line 104: @@
      <p style="line-height : 1.5em">
-<b>13.</b>
+<b>13.</b> Heat shock at 42°C for 2mn
      </p>
@@ Line 110: / Line 110: @@
      <p style="line-height : 1.5em">
-<b>14.</b>
+<b>14.</b> Incubate for 5mn on ice
      </p>
@@ Line 116: / Line 116: @@
      <p style="line-height : 1.5em">
-<b>15.</b>
+<b>15.</b> Add 800µL of LB medium and incubate for 1h at 37°C
      </p>
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      <p style="line-height : 1.5em">
-<b>16.</b>
+<b>16.Optional</b> Concentrate 10X by centrifuging for 2mn at 11000 rpm, eliminate the supernatant and resuspend in 100µL LB.
      </p>
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      <p style="line-height : 1.5em">
-<b>17.</b>
+<b>17.</b> Plate 100µL of bacteria on LB medium with the appropriate antibiotic resistance and incubate at 37°C.
      </p>
- <br/>
-    <p style="line-height : 1.5em">
-<b>18.</b>
-    </p>
- <br/>
-    <p style="line-height : 1.5em">
-<b>19.</b>
-    </p>
- <br/>
-    <p style="line-height : 1.5em">
-<b>20.</b>
-    </p>
- <br/>
-    <p style="line-height : 1.5em">
-<b>21.</b>
-    </p>
- <br/>
      <p style="line-height : 1.5em">