Team:UPO-Sevilla/Notebook/08 02

From 2010.igem.org

(Difference between revisions)
Line 19: Line 19:
       <h2>Production Team</h2>
       <h2>Production Team</h2>
-
       <p><strong>Paola Gallardo.</strong> We started a new round of PCR for SDM, but this time we prepared five samples of each one. We run an electrophoresis to check the products and we have only get positive results for <i>fecI-fecR.</i></p>
+
       <p><strong>Paola Gallardo.</strong> We started a new round of PCR for SDM, but this time we prepared five samples of each one. We ran an electrophoresis to check the products and we had only get positive results for <i>fecI-fecR.</i></p>
       <p><strong>David Caballero.</strong> SDM is made by two PCR reactions. We performed the first PCR reactions for <i>fecA*,</i> <i>gltD**</i> and <i>fecI-fecR*</i> parts. <i>gltD**</i> had two restriction enzyme target. One of them was really near of start codon so we would get it out of there using a longer primer which overlapped the target site. After PCR reactions were performed, samples were running in electrophoresis gel. All samples were perfect. We purified samples from gel and performed the second SDM PCR reaction for each part. Results would be analyzed the next day.</p>
       <p><strong>David Caballero.</strong> SDM is made by two PCR reactions. We performed the first PCR reactions for <i>fecA*,</i> <i>gltD**</i> and <i>fecI-fecR*</i> parts. <i>gltD**</i> had two restriction enzyme target. One of them was really near of start codon so we would get it out of there using a longer primer which overlapped the target site. After PCR reactions were performed, samples were running in electrophoresis gel. All samples were perfect. We purified samples from gel and performed the second SDM PCR reaction for each part. Results would be analyzed the next day.</p>
Line 27: Line 27:
       <p>Mr Gene has come! YIPPEE!!.</p>
       <p>Mr Gene has come! YIPPEE!!.</p>
-
       <p>Today has been a hard day: On the one hand we have made colony PCR (candidates colonies: 12+2, 12+19, 18+3 and 1+19): unsuccessful results, our PCR are contaminated. On the other hand some biobriks are digested, ligated and transformated (2+4,2+5,2+6,2+7, 4+2,5+2,6+2,7+2,11+2,2+3 y 11+19).</p>
+
       <p>Today has been a hard day: On the one hand, we analyzed several devices using colony PCR (different candidates of the following plates: 12+2, 12+19, 18+3 and 1+19) and we had unsuccessful results. Probably, our PCRs were contaminated. On the other hand, some biobricks were digested, ligated and transformated (2+4,2+5,2+6,2+7, 4+2,5+2,6+2,7+2,11+2,2+3 and 11+19).</p>
       <h2>DryLab Team</h2>
       <h2>DryLab Team</h2>

Revision as of 23:19, 26 October 2010

August, 2nd

Production Team

Paola Gallardo. We started a new round of PCR for SDM, but this time we prepared five samples of each one. We ran an electrophoresis to check the products and we had only get positive results for fecI-fecR.

David Caballero. SDM is made by two PCR reactions. We performed the first PCR reactions for fecA*, gltD** and fecI-fecR* parts. gltD** had two restriction enzyme target. One of them was really near of start codon so we would get it out of there using a longer primer which overlapped the target site. After PCR reactions were performed, samples were running in electrophoresis gel. All samples were perfect. We purified samples from gel and performed the second SDM PCR reaction for each part. Results would be analyzed the next day.

Assembly Team

Mr Gene has come! YIPPEE!!.

Today has been a hard day: On the one hand, we analyzed several devices using colony PCR (different candidates of the following plates: 12+2, 12+19, 18+3 and 1+19) and we had unsuccessful results. Probably, our PCRs were contaminated. On the other hand, some biobricks were digested, ligated and transformated (2+4,2+5,2+6,2+7, 4+2,5+2,6+2,7+2,11+2,2+3 and 11+19).

DryLab Team

Wiki: Notebook calendar completed.

Go to 31th of July Go to 3rd of August
Return to Notebook

Footer