Glasgow/Wetlab

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Revision as of 11:50, 26 October 2007 (view source) Scott.w.ramsay (Talk | contribs) ← Older edit		Latest revision as of 11:54, 26 October 2007 (view source) Scott.w.ramsay (Talk | contribs)
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-	*'''''First selection of biobricks transformed.'''	+	*'''First selection of biobricks transformed.'''
-	*'''''Preparation of stocks.'''	+	*'''Preparation of stocks.'''
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-	*'''''Researched DmpR, XylR and DntR sensor systems.'''	+	*'''Researched DmpR, XylR and DntR sensor systems.'''
-	*'''''Designed primers for DmpR, DntR, XylR and associated promoters.'''	+	*'''Designed primers for DmpR, DntR, XylR and associated promoters.'''
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	*'''phzD→phzG successfully cloned into TOPO vector.'''		*'''phzD→phzG successfully cloned into TOPO vector.'''
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-	*'''''Contains further work achieved.'''''	+	*'''Contains further work achieved.'''
		+	*'''XylR and Pr cloned into construction vectors.'''
		+	*'''XylR and Pr put next to responsive promoter and luciferase.'''
	|}		|}

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Latest revision as of 11:54, 26 October 2007

		Back To Glasgow's Main Page	Go To Glasgow's Modelling Page

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Protocols

References

Resources

Sequences

Biobricks Used

Gels

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Click on a week number for more detailed lab book...

Week 1	Week 2
First selection of biobricks transformed. Preparation of stocks.	Researched DmpR, XylR and DntR sensor systems. Designed primers for DmpR, DntR, XylR and associated promoters.
Week 3	Week 4
BioBricks tested by digestion and PCR. PCR with new primers associated with DntR and XylR.	phzM and phzS cloned into TOPO vectors. Primer design for 7 gene operon. DntR cloned into TOPO vector. Primer design for XylR and associated genes. Death gene cloned into TOPO vector. Primer design for death gene.
Week 5	Week 6
Suspected amplification of 7 gene operon. phzM and phzS confirmed as present in TOPO vectors. Confirmed presence of death gene plasmid in some vectors. Miller assay performed with DntR system. Yeast cells.	Biobricks made of phzM, phzS, and DntR.
Week 7	Week 8
Utilised new biobricks. Site directed mutagenesis of phzM completed.	Site directed mutagenesis of phzS completed.
Week 9	Week 10+
phzD→phzG successfully cloned into TOPO vector.	Contains further work achieved. XylR and Pr cloned into construction vectors. XylR and Pr put next to responsive promoter and luciferase.

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Protocols

References

Resources

Orders

Biobricks Used

Gels

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