User:Behzad Damadzadeh/Notebook/PcTF Subcloning in E-coli/2013/11/01: Difference between revisions
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Here we plan to mutate the BSMBI cut site: CGTCTC to CGTTTC | Here we plan to mutate the BSMBI cut site: CGTCTC to CGTTTC | ||
Design Primers: | |||
'''Design Primers:''' | |||
* '''Forward Primer''': 5' <span style="color:#A9A9A9">gca</span> <span style="color:#FF0000">GCTCTTC</span> '''G''' <span style="color:#228B22">'''T'''</span>TC + <span style="color:#800080">25 bps of top right strand</span> | * '''Forward Primer''': 5' <span style="color:#A9A9A9">gca</span> <span style="color:#FF0000">GCTCTTC</span> '''G''' <span style="color:#228B22">'''T'''</span>TC + <span style="color:#800080">25 bps of top right strand</span> | ||
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|{| DNA Template (ng)||200 || rowspan="6" | | |{| DNA Template (ng)||200 || rowspan="6" | | ||
* 95°C, 3 min. | * 95°C, 3 min. | ||
* [95°C, 30 sec.; '''45'''°C, 40 sec.; 72°C, * min (1 min/kb plasmid length) | * [95°C, 30 sec.; '''45'''°C, 40 sec.; 72°C, * min (1 min/kb plasmid length)] x35 | ||
* 72°C, 3 min. | * 72°C, 3 min. | ||
* 4°C, ∞ | * 4°C, ∞ | ||
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Run 5μL of each reaction on 1% agarose gel to confirm the plasmid linearization. | Run 5μL of each reaction on 1% agarose gel to confirm the plasmid linearization. | ||
DNA Purification Using the GenElute™ PCR Clean-Up Kit for rapid purification of double-stranded PCR amplification products. Measure the DNA concentration with plate reader. | DNA Purification Using the GenElute™ PCR Clean-Up Kit for rapid purification of double-stranded PCR amplification products. Measure the DNA concentration with plate reader. | ||
'''SapI Digestion''' | '''SapI Digestion''' | ||
Cutting the SAPI sites to make the sticky ends for ligation: | |||
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Restriction enzyme deactivation Incubate the tubes at 80°C for 10 minutes and place the tube and heat block out of the heater on the bench cool down the | '''Restriction enzyme deactivation''' | ||
Ligate the Sticky Ends to Make Circular DNA | |||
Incubate the tubes at 80°C for 10 minutes and place the tube and heat block out of the heater on the bench cool down the digested parts gradually in room temperature. | |||
'''Ligate the Sticky Ends to Make Circular DNA ''' | |||
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Revision as of 13:44, 4 November 2013
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PCR Based Mutagenesis Protocol
It is fast and efficient method using type IIs restriction enzymes. With designing a pair of mutagenesis primers that the mutated sequence is near and downstream of the recognition site of the type IIs restriction enzyme. PCR will linearize the plasmid with two blunt ends. Enzyme digestion will produce two sticky and complementary ends that will ligate together and generate the mutated plasmid. Here this method would be applied to mutate the BSMBI cut site within the hygromycine resistant gene of V0200 mammalian vector. Primers are designed for SapI restriction enzyme:
Here we plan to mutate the BSMBI cut site: CGTCTC to CGTTTC Design Primers:
PCR Reactions
Run 5μL of each reaction on 1% agarose gel to confirm the plasmid linearization. DNA Purification Using the GenElute™ PCR Clean-Up Kit for rapid purification of double-stranded PCR amplification products. Measure the DNA concentration with plate reader. SapI Digestion Cutting the SAPI sites to make the sticky ends for ligation:
Restriction enzyme deactivation Incubate the tubes at 80°C for 10 minutes and place the tube and heat block out of the heater on the bench cool down the digested parts gradually in room temperature. Ligate the Sticky Ends to Make Circular DNA
Bacterial transformation of each ligation reaction into DH5α-T , fast protocol: incubate DNA and cells on ice for 30 minutes and then spread on AMP agar plates and incubate in 37°C overnight.
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