Team:Caltech/Week 4

From 2011.igem.org

(Difference between revisions)
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==July 5==
==July 5==
<p>Start overnight cultures of Gibson transformations<br/>
<p>Start overnight cultures of Gibson transformations<br/>
-
Begin dry run of fosmid kit</p>
+
Start gel to figure out length of purified river DNA (for fosmid kit)<br/>
 +
Confirm we have enough DNA for work with estrogen receptor<br/>
 +
Streak out new biobricks on chloramphenicol plates</p>
==July 6==
==July 6==
-
<p>Miniprep Gibson transformations and send off for sequencing</p>
+
<p>Miniprep Gibson transformations and send off for sequencing<br/>
 +
Redo gel for fosmid kit<br/>
 +
Continue sequencing of estrogen receptor (using new forward primer and old reverse primer)<br/>
 +
Start overnight cultures of new biobricks<br/>
 +
Plate enrichment cultures on LB
 +
</p>
==July 7==
==July 7==
 +
<p>Miniprep new biobricks and send off for sequencing<br/>
 +
Meet with Pedro about HPLC and p450s<br/>
 +
Image enrichment culture plates<br/>
 +
Image second fosmid kit gel<br/>
 +
Run river DNA on small gel to check size<br/>
 +
Start new minimal media cultures from plates</p>
 +
===Results===
===Results===
<gallery>
<gallery>

Revision as of 22:41, 7 July 2011


Caltech iGEM 2011



Home

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References

Support

July 3

Checked Gibson transformations
Plated remaining transformed cells
Made new dilutions of original enrichment cultures (BPA, nonylphenol, 17-alpha-ethinyl-estradiol, DDT)

Results

There was no growth on the transformed Gibson plates. Since we did a small reaction, we used all of the reaction in transforming competent cells. The Gibson assembly likely failed, as one of the negative control plates had a single colony. However, we have had trouble with our competent cells in the past and will try plating what we have left.

Gibson Transformations

Plate Number of Colonies
pNT001 + 0
pNT001 - 0
pNT002 + 0
pNT002 - 1

July 4

Results

After plating the remaining 450 ul of our transformed cells:

Plate Number of Colonies
pNT001 + 10
pNT001 - 0
pNT002 + 1
pNT002 - 0

This Week

Start enrichment cultures from a previous iteration, as the latest dilutions remain clear.
Design experiments to test for degradation of BPA by pNT001 and pNT002 using the HPLC
Get the BioBricks we ordered from the parts registry ([http://partsregistry.org/Part:BBA_K364309 K364309], [http://partsregistry.org/Part:BBA_K364329 K364329], [http://partsregistry.org/Part:BBA_K364327 K364327], [http://partsregistry.org/Part:BBA_K364307 K364307])
Transform these into cells, miniprep and sequence
Continue with enrichment cultures
Put LA River soil DNA into fosmids
Work on Project Description and Safety Proposal
Once we've sequenced ER ([http://partsregitry.org/Part:BBa_K123003 K123003]), start making test plasmids to see if it works.

July 5

Start overnight cultures of Gibson transformations
Start gel to figure out length of purified river DNA (for fosmid kit)
Confirm we have enough DNA for work with estrogen receptor
Streak out new biobricks on chloramphenicol plates

July 6

Miniprep Gibson transformations and send off for sequencing
Redo gel for fosmid kit
Continue sequencing of estrogen receptor (using new forward primer and old reverse primer)
Start overnight cultures of new biobricks
Plate enrichment cultures on LB

July 7

Miniprep new biobricks and send off for sequencing
Meet with Pedro about HPLC and p450s
Image enrichment culture plates
Image second fosmid kit gel
Run river DNA on small gel to check size
Start new minimal media cultures from plates

Results

Ddtv.png
Ddtnov.png
Ethynylestradiolv.png
Ethynylestradiolnov.png
Nonylphenolv.png
Nonlyphenolnov.png
Bpavroom12.png
Bpavroom34.png
Bpanovroom12.png
Bpanovroom34.png
Bpav3012.png
Bpav3034.png
Bpanov3012.png
Bpanov3034.png


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