Difference between revisions of "Team:Munich/purify1.html"

Revision as of 00:48, 18 October 2018

T7 DNA Extraction by Phenol Chloroform Precipitation

2018/05/17

Participants:	Keno Eilers
Protocol:	Phage T7 DNA Purification, Phenol Chloroform precipitation
Notes:	Still too much from E. coli
Results:	DNA concentration: 55,5 ng/µL

HIER FOTO

Cleanup of T7 DNA from 15.5.18 with NEB PCR Cleanup Kit

2018/05/19

Participants:	Nils O'Brien
Protocol:	NEB PCR Cleanup Kit, Agarose Gel electrophoresis
Notes:	Warming of columns on 40 °C for a few minutes before elution
Results:	No results, not possible with genome larger than 25kb

Second Try: Cleanup of T7 DNA from 15.5.18 with NEB PCR Cleanup Kit

2018/05/20

Participants:	Nils O'Brien
Protocol:	NEB PCR Cleanup Kit, Agarose Gel electrophoresis
Notes:	Warming of columns on 50 °C for a few minutes before elution
Results:	No visible bands on 0,3 Agarose gel, did not work out for large fragments. End of experiments with this method

T7 DNA Clean-Up T7 DNA

2018/05/22

Participants:	Keno Eilers
Protocol:	Phenol Chloroform precipitation

Generating MS2 RNA Genome

2018/05/23

Participants:	Keno Eilers
Protocol:	Phenol Chloroform precipitation, cDNA Synthesis
Notes:	1 µl DNAse I (NEB, 2.000 U/mL) added, incubate for 10 minutes at 37 °C
Results:	RNA concentration: 34900 ng/µl

Generating MS2 RNA Genome

2018/05/23

Participants:	Keno Eilers
Protocol:	Phenol Chloroform precipitation, cDNA Synthesis
Notes:	1 µl DNAse I (NEB, 2.000 U/mL) added, incubate for 10 minutes at 37 °C
Results:	RNA concentration: 34900 ng/µl

Optimization of DNA Precipitation out of T7 Phage

2018/05/23 - 2018/05/25

Participants:	Keno Eilers, Sophie Kurzbach, Nils O'Brien
Protocol:	Phage T7 DNA Purification, Agarose Gelelectrophoresis
Notes:	Step 11 of "T7 DNA purification" protocol: Optimization of PEG (63%) precipitation Incubation for 42 minutes, then proceeded with centrifugation
Results:	150 µl PEG: 302 ng/µl, 200 µl PEG: 164 ng/µl, 250 µl PEG: 278 ng/µl, 300 µl PEG: 113 ng/µl, 350 µl PEG: 279 ng/µl, 400 µl PEG: 216 ng/µl, 450 µl PEG: 530 ng/µl, 500 µl PEG: 422 ng/µl

T7 DNA Isolation with Different Infection Times

2018/05/29

Participants:	Sophie Kurzbach
Protocol:	Phage T7 DNA Purification, Phenol Chloroform precipitation
Notes:	Tested transfection times: 12 min (before supernatant), 22 min (after supernatant), 32 min (cell lysis)
Results:	12 min: 209 ng/µL, 22 min: 628 ng/µL, 32 min: 334 ng/µL

T7 DNA Isolation 10 min and 32 min after Super Transfection + RNAse

2018/06/05 -2018/06/06

Participants:	Sophie Kurzbach
Protocol:	Phage T7 DNA Purification, Phenol Chloroform precipitation, PEG percipitant
Notes:	Better results than DNA without RNAse treatment, still too much E. coli DNA
Results:	DNA concentration of 10 min: 633 ng/µL DNA concentration of 32 min: 200 ng/µL

HIER FOTO

T7 DNA Extraction by Phenol Chloroform Precipitation

2018/06/16-2018/06/18

Participants:	Keno Eilers
Protocol:	Phage T7 DNA Purification, Phenol Chloroform precipitation
Notes:	No notes
Results:	Good DNA: 10,37 nM

DNA Purification of T7 DNA with Qiagen Genomic Tips 100/G

2018/06/22

Participants:	Brigit Tunaj
Protocol:	Qiagen Genomic Tip Kit
Notes:	Preparation of buffers as descripted on their homepage
Results:	Did not work out

DNA Purification of T7 DNA with Qiagen Genomic Tips 100/G

2018/06/25

Participants:	Brigit Tunaj
Protocol:	Qiagen Genomic Tip Kit
Notes:	Increased DNA concentration 50 ug
Results:	Did not work out. Method not suitable for phage DNA.

@@ Line 3: / Line 3: @@
-<h4>T7 DNA extraction by phenol chloroform precipitation </h4>
+<h4>T7 DNA Extraction by Phenol Chloroform Precipitation </h4>
 <em>2018/05/17</em>
 <table class="table table-borderless">
@@ Line 64: / Line 64: @@
-<h4>second try: Cleanup of T7 DNA from 15.5.18 with NEB PCR Cleanup Kit </h4>
+<h4>Second Try: Cleanup of T7 DNA from 15.5.18 with NEB PCR Cleanup Kit </h4>
 <em>2018/05/20</em>
 <table class="table table-borderless">
@@ Line 93: / Line 93: @@
-<h4>T7 DNA clean up T7 DNA </h4>
+<h4>T7 DNA Clean-Up T7 DNA </h4>
 <em>2018/05/22</em>
 <table class="table table-borderless">
@@ Line 116: / Line 116: @@
-<h4> Generating MS2 RNA genome </h4>
+<h4> Generating MS2 RNA Genome </h4>
 <em>2018/05/23</em>
 <table class="table table-borderless">
@@ Line 147: / Line 147: @@
-<h4> Generating MS2 RNA genome </h4>
+<h4> Generating MS2 RNA Genome </h4>
 <em>2018/05/23</em>
 <table class="table table-borderless">
@@ Line 176: / Line 176: @@
 </table>
-<h4> Optimization of DNA precipitation out of T7 Phage </h4>
+<h4> Optimization of DNA Precipitation out of T7 Phage </h4>
 <em>2018/05/23 - 2018/05/25</em>
 <table class="table table-borderless">
@@ Line 205: / Line 205: @@
-<h4>T7 DNA Isolation with different infection times </h4>
+<h4>T7 DNA Isolation with Different Infection Times </h4>
 <em>2018/05/29</em>
 <table class="table table-borderless">
@@ Line 235: / Line 235: @@
-<h4> T7 DNA Isolation 10 min and 32 min after super transfection + RNAse </h4>
+<h4> T7 DNA Isolation 10 min and 32 min after Super Transfection + RNAse </h4>
 <em>2018/06/05 -2018/06/06</em>
 <table class="table table-borderless">
@@ Line 275: / Line 275: @@
      </figure> HIER FOTO
-<h4>T7 DNA extraction by phenol chloroform precipitation </h4>
+<h4>T7 DNA Extraction by Phenol Chloroform Precipitation </h4>
 <em>2018/06/16-2018/06/18</em>
 <table class="table table-borderless">
@@ Line 303: / Line 303: @@
 </table>
-<h4> DNA purification of T7 DNA with Qiagen Genomic Tips 100/G</h4>
+<h4> DNA Purification of T7 DNA with Qiagen Genomic Tips 100/G</h4>
 <em>2018/06/22</em>
 <table class="table table-borderless">
@@ Line 328: / Line 328: @@
 </table>
-<h4> DNA purification of T7 DNA with Qiagen Genomic Tips 100/G</h4>
+<h4> DNA Purification of T7 DNA with Qiagen Genomic Tips 100/G</h4>
 <em>2018/06/25</em>
 <table class="table table-borderless">