Team:HokkaidoU Japan/Notebook/Pre experiment/Plac-failed-experiment

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(Difference between revisions)

Revision as of 01:59, 18 October 2014

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Wrong Plac failed Experiment

Start
Get anti-sense vector
- Fri Jun 20
pHN1257 Great thanks to N. Nakashima
Transformation
- Thr Jul 3
R0010-B0034-E1010-B0015(on pSB6A1) from destribution kit 1µL to JM109
Liquid Culture
- Fri Jul 4
R0010-B0034-E1010-B0015(on pSB6A1)
Mini-prep
- Sat Jul 5
R0010-B0034-E1010-B0015(on pSB6A1)
PCR & PCR purification
- Fri Jul 25
R0040-B0034-E1010-B0015 as_RBS_XhoI_F Tm:68.2℃ & as_mRFP_NcoI_R Tm:76/0℃ KOD plus Neo
Ehanol precipetation
- Sat Jul 26
asmRFP
Digestion
- Sun Jul 27
Cut pHN1257 with NcoI, XhoI (using 10×Cut Smart) Cut asmRFP with NcoI, XhoI (using 10×Cut Smart)
Gel Extraction & Ethanol precipetation
- Sun Jul 27
pHN1257 & asmRFP
Ligation
- Sun Jul 27
Ligate asmRFP with pHN1257
Transformation
- Mon Jul 28
asmRFP(on pHN1257) 5µL DNA to DH5α Turbo
Colony PCR
- Tue Jul 29
asmRFP(on pHN1257) with as_RBS_XhoI_F Tm:68.2℃ & as_mRFP_NcoI_R Tm:76.0℃ Kapa-Taq
Liquid Culture
- Wed Jul 30
asmRFP(on pHN1257)
Mini-prep
- Thr Jul 31
asmRFP(on pHN1257)
DoubleTransformation
- Sun Aug 10
asmRFP(on pHN1257) & B0034-E1010-B0015(on pSB6A1) 2.5µL each to DH5α Turbo
Asssay(unsuccess)
- Wed Aug 13
Culture asmRFP(on pHN1257) & B0034-E1010-B0015(on pSB6A1)1. 2mL LB with 100µL 100mM IPTG 2. 2mL LB However, IPTG was too much to grow normally.
Assay(unsuccess)
- Thr Aug 14
Culture asmRFP(on pHN1257) & B0034-E1010-B0015(on pSB6A1) E. coli was early growth 1. 2mL LB with 20µL 100mM IPTG 2. 2mL LB However, pLac was inducible promoter that is promoted by IPTG. We decided to retry this examination.
Failure...

@@ Line 158: / Line 158: @@
 	      </ul>
 	      <div class="step-recipe">
-R0010-B0034-E1010-B0015(pSB6A1) from destribution kit 1&micro;L DNA to JM109
+R0010-B0034-E1010-B0015(on pSB6A1) from destribution kit 1&micro;L to JM109
 </div>
 	    </div>
@@ Line 179: / Line 179: @@
 	      </ul>
 	      <div class="step-recipe">
-pSB6A1
+R0010-B0034-E1010-B0015(on pSB6A1)
 </div>
 	    </div>
@@ Line 200: / Line 200: @@
 	      </ul>
 	      <div class="step-recipe">
-pSB6A1
+R0010-B0034-E1010-B0015(on pSB6A1)
 </div>
 	    </div>
@@ Line 221: / Line 221: @@
 	      </ul>
 	      <div class="step-recipe">
-R0040-B0034-E1010-B0015 as RBS XhoI, as mRFP NcoI
+R0040-B0034-E1010-B0015 as_RBS_XhoI_F Tm:68.2&#8451; & as_mRFP_NcoI_R Tm:76/0&#8451;
+        KOD plus Neo
 </div>
 	    </div>
@@ Line 242: / Line 244: @@
 	      </ul>
 	      <div class="step-recipe">
-anti-sense(mRFP)
+asmRFP
 </div>
 	    </div>
@@ Line 263: / Line 265: @@
 	      </ul>
 	      <div class="step-recipe">
-Cut pHN1257 with NcoI, XhoI (using 10&times;Cut Smart) Cut anti-sense(mRFP) with NcoI, XhoI (using 10&times;Cut Smart)
+Cut pHN1257 with NcoI, XhoI (using 10&times;Cut Smart)
+        Cut asmRFP with NcoI, XhoI (using 10&times;Cut Smart)
 </div>
 	    </div>
@@ Line 284: / Line 288: @@
 	      </ul>
 	      <div class="step-recipe">
-pHN1257 anti-sense(mRFP)
+pHN1257 & asmRFP
 </div>
 	    </div>
@@ Line 305: / Line 309: @@
 	      </ul>
 	      <div class="step-recipe">
-Ligate anti-sense(mFP) with pHN1257
+Ligate asmRFP with pHN1257
 </div>
 	    </div>
@@ Line 326: / Line 330: @@
 	      </ul>
 	      <div class="step-recipe">
-anti-sense(mRFP) on pHN1257 5&micro;L DNA to DH5&alpha; Turbo
+asmRFP(on pHN1257)
+&micro;L DNA to DH5&alpha; Turbo
 </div>
 	    </div>
@@ Line 347: / Line 353: @@
 	      </ul>
 	      <div class="step-recipe">
-anti-sense(mRFP) on pHN1257
+asmRFP(on pHN1257) with as_RBS_XhoI_F Tm:68.2&#8451; & as_mRFP_NcoI_R Tm:76.0&#8451;
+        Kapa-Taq
 </div>
 	    </div>
@@ Line 368: / Line 376: @@
 	      </ul>
 	      <div class="step-recipe">
-anti-sense(mRFP) on pHN1257
+	asmRFP(on pHN1257)
 </div>
 	    </div>
@@ Line 389: / Line 397: @@
 	      </ul>
 	      <div class="step-recipe">
-anti-sense(mRFP) on pHN1257
+asmRFP(on pHN1257)
 </div>
 	    </div>
@@ Line 397: / Line 405: @@
 	  <div class="step-tile">
 	  <h2 class="step-title">
-Transformation
+DoubleTransformation
 </h2>
 	  </div>
@@ Line 410: / Line 418: @@
 	      </ul>
 	      <div class="step-recipe">
-anti-sense(mRFP) on pHN1257 & pSB6A1 2.5&micro;L each DNA to DH5&alpha; Turbo
+asmRFP(on pHN1257) & B0034-E1010-B0015(on pSB6A1)
+.5&micro;L each to DH5&alpha; Turbo
 </div>
 	    </div>
@@ Line 431: / Line 441: @@
 	      </ul>
 	      <div class="step-recipe">
-Culture anti-sense(mRFP) on pHN1257 & pSB6A1 1. 2mL LB with 100&micro;L 100mM IPTG 2. 2mL LB However, IPTG was too much to grow normally.
+Culture asmRFP(on pHN1257) & B0034-E1010-B0015(on pSB6A1)1. 2mL LB with 100&micro;L 100mM IPTG 2. 2mL LB However, IPTG was too much to grow normally.
 </div>
 	    </div>
@@ Line 452: / Line 463: @@
 	      </ul>
 	      <div class="step-recipe">
-Culture anti-sense(mRFP) on pHN1257 & pSB6A1 E. coli was early growth 1. 2mL LB with 20&micro;L 100mM IPTG 2. 2mL LB However, pLac was inducible promoter that is promoted by IPTG. We decided to retry this examination.
+	Culture asmRFP(on pHN1257) & B0034-E1010-B0015(on pSB6A1) E. coli was early growth 1. 2mL LB with 20&micro;L 100mM IPTG 2. 2mL LB However, pLac was inducible promoter that is promoted by IPTG. We decided to retry this examination.
 </div>
 	    </div>

Team:HokkaidoU Japan/Notebook/Pre experiment/Plac-failed-experiment

From 2014.igem.org

Revision as of 01:59, 18 October 2014

Wrong Plac failed Experiment

Start

Get anti-sense vector

Transformation

Liquid Culture

Mini-prep

PCR & PCR purification

Ehanol precipetation

Digestion

Gel Extraction & Ethanol precipetation

Ligation

Transformation

Colony PCR

Liquid Culture

Mini-prep

DoubleTransformation

Asssay(unsuccess)

Assay(unsuccess)

Failure...