Griffitts:Low-copy plasmid prep: Difference between revisions
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* Centrifuge for 8 min at 8000 rpm | * Centrifuge for 8 min at 8000 rpm | ||
* Resuspend in 2.5 mL of [[Griffitts:Common buffers#resuspension buffer|resuspension buffer]] | * Resuspend in 2.5 mL of [[Griffitts:Common buffers#resuspension buffer|resuspension buffer]] | ||
** Alternatively, you can use 2.5 mL old Buffer P1<sup><font color=red>*</font></sup> | |||
* Add 2.5 mL of [[Griffitts:Common buffers#lysis solution|lysis solution]] | * Add 2.5 mL of [[Griffitts:Common buffers#lysis solution|lysis solution]] | ||
** Alternatively, you can use 2.5 mL old Buffer P2<sup><font color=red>*</font></sup> | |||
===DNA Isolation=== | ===DNA Isolation=== | ||
* Add 2.5 mL of [[Griffitts:Common buffers#neutralization solution|neutralization solution]] | * Add 2.5 mL of [[Griffitts:Common buffers#neutralization solution|neutralization solution]] | ||
** Alternatively, you can use 2.5 mL old Buffer N3<sup><font color=red>*</font></sup> | |||
* Centrifuge at 13,000 rpm for 8 min | * Centrifuge at 13,000 rpm for 8 min | ||
* Transfer 6.5 mL of supernatant to 15-mL Falcon tube | * Transfer 6.5 mL of supernatant to 15-mL Falcon tube | ||
* Add 50 μL of [[Griffitts:Common buffers#RNAse A|RNAse A]] | * Add 50 μL of [[Griffitts:Common buffers#RNAse A|RNAse A]] | ||
** If you're using old buffers, you can just leave it on the bench top for 5–10 minutes to allow the native RNAses to work | |||
* Let sit at RT for 5 min | * Let sit at RT for 5 min | ||
* Add 6.5 mL of isopropanol | * Add 6.5 mL of isopropanol | ||
* Incubate at | * Incubate at –20°C for 30 min | ||
* Centrifuge in clinical (yellow) centrifuge for 10 min at max speed | * Centrifuge in clinical (yellow) centrifuge for 10 min at max speed | ||
* Pour off supernatant | * Pour off supernatant | ||
* Resuspend pellet in 1 mL 70% ethanol | * Resuspend pellet in 1 mL 70% ethanol | ||
* Centrifuge for 5 min in clinical centrifuge | * Centrifuge for 5 min in the clinical centrifuge at max speed | ||
** The clinical centrifuge is the yellow centrifuge by the lab autoclave | |||
* Discard supernatant | * Discard supernatant | ||
===Qiagen Miniprep=== | ===Qiagen Miniprep=== | ||
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* Centrifuge for another 60 seconds at full speed | * Centrifuge for another 60 seconds at full speed | ||
* Move column to a labeled 1.5 mL microcentrifuge tube | * Move column to a labeled 1.5 mL microcentrifuge tube | ||
* Add 70 μL [[Griffitts:Common buffers#TE buffer]] (preheated to 65°C) directly to disk | * Add 70 μL [[Griffitts:Common buffers#TE buffer|T<sub>3</sub>E<sub>0.3</sub>]] (preheated to 65°C) directly to disk | ||
** Don't touch the membrane with your tip | ** Don't touch the membrane with your tip | ||
**Note that [[Griffitts:Common buffers#TE buffer]] must be added to the column hot for efficient elution of large (20 kb) plasmids | **Note that [[Griffitts:Common buffers#TE buffer|T<sub>3</sub>E<sub>0.3</sub>]] must be added to the column hot for efficient elution of large (20 kb) plasmids | ||
* Let stand 1 | * Let stand 1–2 minutes | ||
* Centrifuge for 60 seconds at full speed to elute DNA | * Centrifuge for 60 seconds at full speed to elute DNA<br> | ||
<sup><font color=red>*</font></sup>The old buffers are kept in a Qiagen box on the upper shelf | |||
Latest revision as of 10:19, 12 October 2010
Miniprep procedure for large, low-copy plasmids
Procedure
Lysis
- Set up an overnight culture in 40 mL LB broth
- Centrifuge for 8 min at 8000 rpm
- Resuspend in 2.5 mL of resuspension buffer
- Alternatively, you can use 2.5 mL old Buffer P1*
- Add 2.5 mL of lysis solution
- Alternatively, you can use 2.5 mL old Buffer P2*
DNA Isolation
- Add 2.5 mL of neutralization solution
- Alternatively, you can use 2.5 mL old Buffer N3*
- Centrifuge at 13,000 rpm for 8 min
- Transfer 6.5 mL of supernatant to 15-mL Falcon tube
- Add 50 μL of RNAse A
- If you're using old buffers, you can just leave it on the bench top for 5–10 minutes to allow the native RNAses to work
- Let sit at RT for 5 min
- Add 6.5 mL of isopropanol
- Incubate at –20°C for 30 min
- Centrifuge in clinical (yellow) centrifuge for 10 min at max speed
- Pour off supernatant
- Resuspend pellet in 1 mL 70% ethanol
- Centrifuge for 5 min in the clinical centrifuge at max speed
- The clinical centrifuge is the yellow centrifuge by the lab autoclave
- Discard supernatant
Qiagen Miniprep
- Resuspend DNA pellet in 250 μL of Buffer P1
- The P1 is kept in the fridge
- Make sure to use P1 that has RNAse added
- Add 250 μL of Buffer P2
- Immediately invert 3 times
- Let stand for 2 minutes
- Add 350 μL of Buffer N3
- Immediately invert 8 times
- Keep on ice for 5 min
- Centrifuge at 13,000 rpm for 6 min in microfuge
- Carefully move the supernatant (~820 μL) to a spin column
- Centrifuge for 30 seconds at full speed
- Remove flowthrough
- Add 700 μL of wash buffer PE to column
- Centrifuge for 30 seconds at full speed
- Remove flowthrough
- Centrifuge for another 60 seconds at full speed
- Move column to a labeled 1.5 mL microcentrifuge tube
- Add 70 μL T3E0.3 (preheated to 65°C) directly to disk
- Don't touch the membrane with your tip
- Note that T3E0.3 must be added to the column hot for efficient elution of large (20 kb) plasmids
- Let stand 1–2 minutes
- Centrifuge for 60 seconds at full speed to elute DNA
*The old buffers are kept in a Qiagen box on the upper shelf
