Team:EPF Lausanne/Calendar/7 September 2013

From 2013.igem.org

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<font size = "4"> Sensing </font> <BR>
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Sensing <BR>
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''Purification of PCR products of the three sensing constructs'' <BR>
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-I purified the PCR products from the previous Day and the concentrations were within an acceptable range. Since I had not yet amplified the constitutive promoter from iGEM I put the purified Backbone for this promoter into the refridgarator for late use.
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'''Purification of PCR products of the three sensing constructs''' <BR>
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''DpnI digest of the two pH sensitive promoters and their backbones'' <BR>
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I purified the PCR products from the previous Day and the concentrations were within an acceptable range. Since I had not yet amplified the constitutive promoter from iGEM I put the purified Backbone for this promoter into the refridgarator for late use.
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'''DpnI digest of the two pH sensitive promoters and their backbones''' <BR>
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I did a DpnI digest and measured the concentrations again, they were all around 50ng/ul which is good.
I did a DpnI digest and measured the concentrations again, they were all around 50ng/ul which is good.
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'''Gibson assembly of the two constructs with the hya and the cad promoter (pH-sensors) '''<BR>
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''Gibson assembly of the two constructs with the hya and the cad promoter (pH-sensors)''<BR>
I did a Gibson assembly of both sensing construcst but it did not work for the one with the hya promoter, so I did another Restriction digest of the purified PCR products for this promoter.
I did a Gibson assembly of both sensing construcst but it did not work for the one with the hya promoter, so I did another Restriction digest of the purified PCR products for this promoter.
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'''PCR of the MMP2 insert and its Backbone and the MMP9 Backbone''' <BR>
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''PCR of the MMP2 insert and its Backbone and the MMP9 Backbone'' <BR>
We did a PCR of the backbones for both MMP2 and MMP9 as well as of the insertMMP2. The Gel showed that it worked.
We did a PCR of the backbones for both MMP2 and MMP9 as well as of the insertMMP2. The Gel showed that it worked.
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Revision as of 16:39, 3 October 2013

Taxi.Coli: Smart Drug Delivery iGEM EPFL

Header

Sensing

Purification of PCR products of the three sensing constructs
-I purified the PCR products from the previous Day and the concentrations were within an acceptable range. Since I had not yet amplified the constitutive promoter from iGEM I put the purified Backbone for this promoter into the refridgarator for late use.

DpnI digest of the two pH sensitive promoters and their backbones
I did a DpnI digest and measured the concentrations again, they were all around 50ng/ul which is good.

Gibson assembly of the two constructs with the hya and the cad promoter (pH-sensors)
I did a Gibson assembly of both sensing construcst but it did not work for the one with the hya promoter, so I did another Restriction digest of the purified PCR products for this promoter.

PCR of the MMP2 insert and its Backbone and the MMP9 Backbone
We did a PCR of the backbones for both MMP2 and MMP9 as well as of the insertMMP2. The Gel showed that it worked.