Team:Caltech/Week 3

From 2011.igem.org

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<p>
<p>
Redo PCR of [http://partsregistry.org/Part:BBa_R0010 R0010] and [http://partsregistry.org/Part:BBa_K123000 K123000]<br/>
Redo PCR of [http://partsregistry.org/Part:BBa_R0010 R0010] and [http://partsregistry.org/Part:BBa_K123000 K123000]<br/>
-
Gibson assemble pNT002, pNT001 if redo of PCR works<br/>
+
Analyze sequence of ER, design new primer for continued sequencing<br/>
-
Order primers and vectors for 16s sequencing<br/>
+
-
Analyze sequence of ER, design test plasmids if sequence of ER is correct, if not, plan repair <br/>
+
Plan experiments using pNT001 and pNT002</p>
Plan experiments using pNT001 and pNT002</p>
===Results===
===Results===
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==June 30==
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<p>Miniprep 5 K145001 cultures and send them off for sequencing before noon
 +
Make glycerol stocks of mCherry ([http://partsregistry.org/Part:BBa_J06702 J06702]), Lac Promoter ([http://partsregistry.org/Part:BBa_R0010 R0010]), double terminator ([http://partsregistry.org/Part:BBa_B0014 B0014] and [http://partsregistry.org/Part:BBa_B0015 B0015]) and Tet Promoter ([http://partsregistry.org/Part:BBa_R0040 R0040])<br/>
 +
Ask Joe if we need to PCR plasmid or if he has linear plasmid<br/>
 +
If we need to linearize: Borrow plasmid primers and plasmid, do PCR. Repeat failed PCR (Primers 9 and 10 and DNA B0014) along with it <br/>
 +
If we don't, then repeat failed PCR <br/>
 +
Get recipe from Joe for gibson mix and gibson protocol, make gibson mix, and run gibson reaction and transform<br/>
 +
For gels tomorrow: Use Joe's sybr safe.</p>
== This Week ==
== This Week ==
<p>
<p>

Revision as of 01:17, 30 June 2011


Caltech iGEM 2011



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June 26

Start overnight cultures of T7 polymerase (K145001), mCherry (J06702), Lac Promoter (R0010), double terminator (B0014 and B0015) and Tet Promoter (R0040)

June 27

Miniprep of T7 polymerase (K145001), mCherry (J06702), Lac Promoter (R0010), double terminator (B0014 and B0015) and Tet Promoter (R0040) and submit for sequencing
Transfer 0.5 mL aliquots of BPA and 5 mL aliquots 17a-ethynylestradiol cultures from June 23 to fresh minimal media
Checked DDT and nonylphenol cultures, will wait until tomorrow to transfer
Ethanol precipitation of DNA extractions from LA river samples following protocol
Streak out cells from fosmid kit
Prepare antibiotic stocks (Ampicillin, Chloramphenicol)

Results

Miniprep

Part Concentration(ng/ul)
B0014 230.5
B0015 254.1
J06702 301.3
K145001 205.6
R0010 117.3
R0040 156.8

We found growth in one of our BPA enrichment cultures, and slight growth in our ethinyl estradiol cultures. We transferred these vials today.

June 28

Send off continued forward sequencing for HER
PCR for Gibson assembly of PNT001 and PNT002
Gel and PCR purification of PCR products
Analysis of sequencing results from yesterday
Transfer DDT and nonylphenol cultures to new media
Transform mCherry (J06702), Lac Promoter (R0010), double terminator (B0014 and B0015) and Tet Promoter (R0040)for creation of glycerol stocks

Results

Sequencing: All biobricks showed correct sequence except T7 Polymerase

PCR of parts for pNT001 and pNT002(BioBricks + primers for Gibson): From left to right: 1 ladder; 2 blank; 3 R0010; 4 K123000; 5 B0014; 6 R0040; 7 K123001; 8 B0015

Ran a gel of the PCR products. Strangely, lanes 3 and 4 show no DNA. We will repeat the PCR of lanes 3-5 and Gibson assemble pNT001 (R0010, K123000, B0014) later in the week.

EtOH precipitation of Soil Extractions from June 21

Tube/Location Number Concentration(ng/ul)
1 13.6
2 15.2
4 8.3
5 11.4
6 25.5
7 23.5
9 261.3
10 74.0

June 29

Redo PCR of R0010 and K123000
Analyze sequence of ER, design new primer for continued sequencing
Plan experiments using pNT001 and pNT002

Results

Estrogen receptor (K123003) sequencing is back. Again, the translation is right, but the bases don't match. The stop codon is not in this read. We will keep sequencing.

Concentration of Purified PCR products from June 28 and June 29

Tube Number Concentration(ng/ul)
6/28 3 15.2
6/28 4 49.1
6/28 5 42.0
6/28 6 112.0
6/29 1 112.7
6/29 2 168.0

June 30

Miniprep 5 K145001 cultures and send them off for sequencing before noon Make glycerol stocks of mCherry (J06702), Lac Promoter (R0010), double terminator (B0014 and B0015) and Tet Promoter (R0040)
Ask Joe if we need to PCR plasmid or if he has linear plasmid
If we need to linearize: Borrow plasmid primers and plasmid, do PCR. Repeat failed PCR (Primers 9 and 10 and DNA B0014) along with it
If we don't, then repeat failed PCR
Get recipe from Joe for gibson mix and gibson protocol, make gibson mix, and run gibson reaction and transform
For gels tomorrow: Use Joe's sybr safe.

This Week

Email other teams
Use pNT001 and pNT002 to test degradation parts


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