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Team:SJTU-BioX-Shanghai/Notebook/Lab log/July
From 2013.igem.org
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(→Constitutive dCas9 and Ho1 pSB1C3 plasmid construction) |
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Extract the plasmid through miniprep. Identification by PCR. | Extract the plasmid through miniprep. Identification by PCR. | ||
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| + | ===Construct dCas9, pcyA and Ho1 plasmid=== | ||
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| + | PCR to connect dCas9, pcyA and Ho1 into pSB1C3. (Adding restriction enzyme cutting sites at both ends,Xba I and Sal I) | ||
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| + | Digest with Xba I and Sal I, and pSB1C3 backbone with Spe I and Sal I. 6 hours. | ||
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| + | Ligation and transformation (3 hours, DH5α). Culturing overnight. | ||
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| + | Picking colonies and culturing overnight. | ||
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| + | Identify by monocolonal colony PCR and send 2 copies of positive colony each of Ho1 and PcyA. | ||
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| + | No positive dCas9 colony identified. | ||
===Construct Red Sensor plasmid.=== | ===Construct Red Sensor plasmid.=== | ||
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===Construct luciferase plasmid.=== | ===Construct luciferase plasmid.=== | ||
Plasmid is confirmed by sequencing. | Plasmid is confirmed by sequencing. | ||
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| + | ===Construct dCas9, pcyA and Ho1 plasmid=== | ||
| + | Sequencing reseult showed that the plasmid we got was the model plasmid. The new backbone and original sequence model are both chlorampenicol resistant. | ||
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| + | Reconstruct constitutive pcyA and Ho1 plasmid using DpnI to digest plasmid model. | ||
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| + | Get 2 plasmids of pcyA to send sequencing. | ||
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| + | Again didn't get positive colony of dCas9 and Ho1. | ||
===Construct Red Sensor plasmid.=== | ===Construct Red Sensor plasmid.=== | ||
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Concentration of plasmid is low for sequencing. Culture colonies with positive results in large scale for 24 hours. | Concentration of plasmid is low for sequencing. Culture colonies with positive results in large scale for 24 hours. | ||
Plasmid extraction and identification by sequencing. | Plasmid extraction and identification by sequencing. | ||
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| + | ===Construct Blue Sensor plasmid onto another Backbone=== | ||
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| + | After we get the right sequencing result, we begin to use a pair of new primers doing PCR to add a new restriction enzyme site on the PCR pieces. | ||
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| + | Cut and Paste, trying to get another plasmid. | ||
=Week4= | =Week4= | ||
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| + | ===Construct dCas9, pcyA and Ho1 plasmid=== | ||
| + | ====Constitutive pcyA-pRSF plasmid construction==== | ||
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| + | PCR to add restriction enzyme cutting sites at both ends of consititutive pcyA operon, Xho1 and BamH1) | ||
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| + | Digest pRSF-duet1 plasmid and PCR product with Xho1 and BamH1. Use elecrophoresis and gel extraction to purify pcr product and backbone sequence. | ||
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| + | Ligation and transformation (3 hours, DH5α). | ||
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| + | Picking colonies and culturing overnight. | ||
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| + | Identify by monocolonal colony pcr. | ||
| + | |||
| + | |||
| + | ====Constitutive dCas9 and Ho1 pSB1C3 plasmid construction==== | ||
| + | |||
| + | Reconstruct Constitutive dCas9 and Ho1 pSB1C3 plasmid. | ||
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| + | Got 1 positive colony of Ho1 and sent sequencing. | ||
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| + | Again didn't get positive clone of dCas9. | ||
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===Construct Red Sensor plasmid.=== | ===Construct Red Sensor plasmid.=== | ||
PCR to connect cph8 into pSB1C3. | PCR to connect cph8 into pSB1C3. | ||
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Picking colonies and culturing 24 hours. | Picking colonies and culturing 24 hours. | ||
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| + | ===Blue Sensor Plasmid Faces with Challenge=== | ||
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| + | After several tests the result hasn't been got by us. | ||
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| + | Repeat and try to find the smallest mistakes. | ||
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Latest revision as of 03:17, 28 September 2013
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