Difference between revisions of "Team:Potsdam/Protocols"

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4. Let the newly poured gel sit at room temperature for 20-30 mins, until it has completely solidified. <br>
 
4. Let the newly poured gel sit at room temperature for 20-30 mins, until it has completely solidified. <br>
 
if  you are in a hurry the gel can also be set more quickly if you place the gel tray at 4 °C  
 
if  you are in a hurry the gel can also be set more quickly if you place the gel tray at 4 °C  
earlier so that it is already cold when the gel is poured into it. </div> <br> <br>
+
earlier so that it is already cold when the gel is poured into it. </div> <br>
 
<b>5. Loading Samples and Running an Agarose Gel: </b>
 
<b>5. Loading Samples and Running an Agarose Gel: </b>
 
<br>
 
<br>
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little time as possible to minimize damage to the DNA.<br>
 
little time as possible to minimize damage to the DNA.<br>
 
Note:
 
Note:
The fragments of DNA are usually referred to as ‘bands’ due to their appearance on the gel.<br></div><br><br>
+
The fragments of DNA are usually referred to as ‘bands’ due to their appearance on the gel.<br></div><br>
 +
 
 
<b>6.Analyzing Your Gel</b>
 
<b>6.Analyzing Your Gel</b>
 
<div style="text-align: justify; margin-left:20px">
 
<div style="text-align: justify; margin-left:20px">

Revision as of 11:27, 31 October 2017

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Our research work

We are describing our research work. Below you can find the protocols we used.

Protocols