Team:NU Kazakhstan/Notebook
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<td class="c1"><a href="https://2014.igem.org/Team:NU_Kazakhstan/Safety">Safety</a></td> | <td class="c1"><a href="https://2014.igem.org/Team:NU_Kazakhstan/Safety">Safety</a></td> | ||
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+ | <td class="c1"><a href="https://2014.igem.org/Team:NU_Kazakhstan/Human practices">Human practices</a></td> | ||
- | <td class="c1"><a href="https://2014.igem.org/Team:NU_Kazakhstan/ | + | <td class="c1"><a href="https://2014.igem.org/Team:NU_Kazakhstan/Interlab Study">Interlab Study</a></td> |
<td class="c1"> <a href="https://2014.igem.org/Main_Page"> <img src="https://static.igem.org/mediawiki/igem.org/6/60/Igemlogo_300px.png" | <td class="c1"> <a href="https://2014.igem.org/Main_Page"> <img src="https://static.igem.org/mediawiki/igem.org/6/60/Igemlogo_300px.png" | ||
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<td valign="top" class="body_txt"><h1></h1> | <td valign="top" class="body_txt"><h1></h1> | ||
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<li>Final extension: 72C, 5min</li></p> | <li>Final extension: 72C, 5min</li></p> | ||
<p>See agarose gel picture for the results.</p> | <p>See agarose gel picture for the results.</p> | ||
- | <img src="https:// | + | <img src="https://static.igem.org/mediawiki/2014/thumb/9/9a/June_19.jpg/800px-June_19.jpg" width="100" height="200"> |
<p>June 20: We did pcr of backbones and rfp part again, but using 3 best annealing temperatures. We have also used concentration of primers for the backbone twice as low as last time, and the bands are very clear. See the picture</p> | <p>June 20: We did pcr of backbones and rfp part again, but using 3 best annealing temperatures. We have also used concentration of primers for the backbone twice as low as last time, and the bands are very clear. See the picture</p> | ||
- | <img src="https:// | + | <img src="https://static.igem.org/mediawiki/2014/thumb/a/a3/June_20.jpg/800px-June_20.jpg" width="100" height="200"> |
<p>June 21-22: We did transformation of e.coli with 3 part+1 control. PelB and HlyA worked well, but LigA, which was planned to be used as 75kDa protein did not work. I found out, that it requires the special KRX strain of e.coli, which we do not have. So, I took another part (Salty_VrgP) from the kit which 79kDa protein and did the transformation; also I did transformation with NahR gene, which gives 34kDa protein, we will use it in constructing "rehearsal" part of the "competence project". In addition, we did miniprep of plasmids, that we've got from Madrid and of PelB and HlyA.</p> | <p>June 21-22: We did transformation of e.coli with 3 part+1 control. PelB and HlyA worked well, but LigA, which was planned to be used as 75kDa protein did not work. I found out, that it requires the special KRX strain of e.coli, which we do not have. So, I took another part (Salty_VrgP) from the kit which 79kDa protein and did the transformation; also I did transformation with NahR gene, which gives 34kDa protein, we will use it in constructing "rehearsal" part of the "competence project". In addition, we did miniprep of plasmids, that we've got from Madrid and of PelB and HlyA.</p> | ||
<p>June-23: we did the competent dh5a cells. The transformation was conducted The cells are competent.</p> | <p>June-23: we did the competent dh5a cells. The transformation was conducted The cells are competent.</p> | ||
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<li>We observed the bands of size 41kDa. See the picture for the results, but it is not seen clearly on the picture, probably, because of low concentration of the protein. | <li>We observed the bands of size 41kDa. See the picture for the results, but it is not seen clearly on the picture, probably, because of low concentration of the protein. | ||
Note: Size of 41kDa indicates the fact that secreted protein was not dimerized because dimerized protein was expected to have the size of 84 kDa</li></ol> | Note: Size of 41kDa indicates the fact that secreted protein was not dimerized because dimerized protein was expected to have the size of 84 kDa</li></ol> | ||
- | <img src="https:// | + | <img src="https://static.igem.org/mediawiki/2014/7/75/July_19.jpg" width="100" height="200"> |
<p>July 19: We did restriction digest of miniprep product (GFP in plasmid backbone) using EcoRI and SpeI: | <p>July 19: We did restriction digest of miniprep product (GFP in plasmid backbone) using EcoRI and SpeI: | ||
<p>1. Digestion with SpeI: DNA - 2ul (500ng), 10xTango buffer - 2ul, Water - 15.5ul, SpeI (Fermentas) - 0.5ul. We incubated the reaction at 37C for 1.5 hour</p> | <p>1. Digestion with SpeI: DNA - 2ul (500ng), 10xTango buffer - 2ul, Water - 15.5ul, SpeI (Fermentas) - 0.5ul. We incubated the reaction at 37C for 1.5 hour</p> | ||
<p>2. Then we added 2.5ul of EcoRI buffer and 0.5ul EcoRI (Fermentas) to the initial reaction.</p> | <p>2. Then we added 2.5ul of EcoRI buffer and 0.5ul EcoRI (Fermentas) to the initial reaction.</p> | ||
<p>3. We ran the reaction mixture on the gel and observed that the digestion worked (see the picture, third well): we have got band for the plasmid backbone (2070bp) and for GFP (~700bp)</p> | <p>3. We ran the reaction mixture on the gel and observed that the digestion worked (see the picture, third well): we have got band for the plasmid backbone (2070bp) and for GFP (~700bp)</p> | ||
- | <img src="https:// | + | <img src="https://static.igem.org/mediawiki/2014/d/db/July_19_restriction_digest.jpg" width="100" height="200"> |
<p>July 21: we decided to do the double digest of plasmid with EcoRI & PstI.</p> | <p>July 21: we decided to do the double digest of plasmid with EcoRI & PstI.</p> | ||
<p>Total reaction mixture - 20ul: DNA miniprep product (700ng) - 2.0ul,10xBuffer SH - 2ul,EcoRI (Invitrogen) - 1ul, PstI (Sigma) - 1ul. We incubated the reaction at 37C for 1hour, then inactivated the enzymes at 65C for 15 min. | <p>Total reaction mixture - 20ul: DNA miniprep product (700ng) - 2.0ul,10xBuffer SH - 2ul,EcoRI (Invitrogen) - 1ul, PstI (Sigma) - 1ul. We incubated the reaction at 37C for 1hour, then inactivated the enzymes at 65C for 15 min. | ||
The double digestion worked: we were able to see two distinct bands (for plasmid backbobe and for GFP). See the image.</p> | The double digestion worked: we were able to see two distinct bands (for plasmid backbobe and for GFP). See the image.</p> | ||
- | <img src="https:// | + | <img src="https://static.igem.org/mediawiki/2014/thumb/c/c0/July_21.jpg/210px-July_21.jpg" width="100" height="200"> |
- | + | <p>July 27: we tried a new method of assembling parts, which does not require the use of restriction enzymes and ligase. The method is Circular Polymerase Extension Cloning (CPEC).</p> | |
- | <img src="https:// | + | <b>Protocol:</b> |
- | <img src="https:// | + | <p>Reaction mixtures 25ul each:</p> |
- | <img src="https:// | + | <p>a) for incorporating NahR (34kDa) protein into backbone (3338bp total): Purified PCR product of backbone (100ng) - 4ul, Purified PCR product of NahR (100ng) - 4.2ul, HF master mix - 11.75ul, DMSO - 0.75ul, dWater - 4.3ul</p> |
- | </td> | + | <p> Thermocycler program: 30s - 98C, 10s - 98C, 30s - 55C, 50s (15s/kb) - 72C, 15 cycles, 10min - 72C</p> |
+ | <p>b) for incorporating INP into backbone (3000bp total), Not purified PCR product of backbone (700ng) - 1.02ul, Not purified PCR product of INP (700ng) - 1.81ul, HF master mix - 11.75ul, DMSO - 0.75ul, dWater - 9.67ul</p> | ||
+ | <p>Thermocycler program: 30s - 98C, 10s - 98C, 30s - 55C, 45s (15s/kb) - 72C, 15 cycles, 10min - 72C</p> | ||
+ | <p>Results: We observed the bands of the expected sizes on the gel, which means that the desired incorporation did occur. See the image for the results. We will transform the obtained products into E. coli tomorrow in order to confirm that the experiment worked.</p> | ||
+ | <img src="https://static.igem.org/mediawiki/2014/thumb/8/86/July_27_CPEC.jpg/543px-July_27_CPEC.jpg" width="100" height="200"> | ||
+ | <p>July 27: Another SDS PAGE for VHamylase. This time we did two types of samples: unheated and heated. We were able to observe the sizes of proteins for both dimerized proteins and monomers. See the picture.</p> | ||
+ | <img src="https://static.igem.org/mediawiki/2014/thumb/5/5b/July_27.jpg/695px-July_27.jpg" width="100" height="200"> | ||
+ | <p>July29: Today we combined 2 parts together and incorporated them into backbone with CPEC: INP+NahR(34kDa)+Backbone. | ||
+ | <p>1. We digested INP with SpeI and NahR with XbaI for 2 hours at 37C, then heat-killed the enzymes at 65c for 15min: DNA (directly from PCR) - 10ul, dWater - add up to 30ul, 10XRecomended Buffer - 2ul, Restriction Enzyme -1ul </p> | ||
+ | <p>2. We combined 3 genes with CPEC:</p> | ||
+ | <p>Reaction mixture (25ul):Backbone - 2ul, INP with digested SpeI site - 2ul, NahR with digested XbaI site - 2ul, High Fidelity Master - 11.75ul, DMSO - 0.75ul, dWater - 6.5ul </p> | ||
+ | <p>Program: the same as in my previous post, just the extension time was increased to 64s, due to the fact that we want to construct 4268bp long part. | ||
+ | See the picture of the gel.</p> | ||
+ | <img src="https://static.igem.org/mediawiki/2014/thumb/9/96/July_29_CPEC.jpg/602px-July_29_CPEC.jpg" width="100" height="200"> | ||
+ | <h4>October 13</h4> | ||
+ | <p>We have eventually received our genes (gp16 and Vhp53) in pUC57 vector backbone (http://www.genscript.com/app/product/downfile.html?from=1&file=filecenter/document/1400_20060331011034.JPG) and primers. We transformed Dh5alpha cells with these plasmids</p> | ||
+ | <h4>October 16</h4> | ||
+ | We did PCR of our parts and we got the following results: | ||
+ | <center><img src="https://static.igem.org/mediawiki/2014/thumb/e/e2/Super.jpg/800px-Super.jpg"></center> | ||
+ | <p>The size of amplified Gp16 gene was 1056bp, while the size of nanobody construct (Vh p53 + Ig hinge + his tag + HlyA) was 1995bp</p> | ||
+ | </td> | ||
</td> | </td> | ||
Latest revision as of 23:11, 16 October 2014
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