Southern blotting: Difference between revisions

From The School of Biomedical Sciences Wiki
Jump to navigation Jump to search
← Older editNewer edit →
mNo edit summary
No edit summary
Line 1: Line 1:
Southern blotting is when you isolate a particular [[Gene|gene]].  
Southern blotting, named after its inventor Edwin Southern, is a technique that is used to detect specific DNA sequences using gel-transfer hybridization.  


First you have to do [[Electrophoresis|electrophoresis]] on with the [[DNA|DNA]]. You use [[Restriction enzyme|restriction enzymes]] to break up the DNA and the run the gel using [[Agarose|agarose]]. The smallest fragments ith travel the furthest. Place [[Nitrocellulous|nitrocellulous]] filter on plate to pick up phages from each [[Plaque|plaque]]. Left with single stranded DNA. [[Hybridise|Hybridise]] with [[Labelled probe|labelled probe]]. Denature the DNA using [[NaOH|NaOH]].&nbsp;Left with single stranded DNA. Hybridise with labelled probe. Perform [[Autoradiography|autoradiography]]. Signal appears over [[Bacteriophage|phage]] DNA that is complementary to probe. Cut out signal area to obtain DNA <ref>http://askabiologist.asu.edu/southern-blotting</ref>.  
Firstly you have to cut the DNA into smaller strands, this is done using a restriction enzyme. Then you need to perform a gel electrophoresis on agrose gel,&nbsp;using the fragments obtained.The smallest DNA fragments travel the furthest, as they are able to&nbsp;move&nbsp;more easily between the gaps in the agrose gel. Once the gel electrophoresis is complete&nbsp;place a&nbsp;[[Nitrocellulous|nitrocellulous]]&nbsp;sheet over the gel, so the DNA fragments are transfered to the sheet. Wash&nbsp;the sheet in an alkaline solution,&nbsp;for example NaOH, this is to ensure that the double stranded DNA is separtaed before hybridization.&nbsp;Place the sheet in a sealed plastic bag thats contains a salt buffered solution and DNA nucleotides and leave in conditions that favour hybridization for a long period of time. Ensure the DNA nucleotides are labeled by a probe, either radioactive or fluroescent. Once hybridization is complete remove and wash the nitrocellulose sheet, so that only hybridised DNA molecules are left on the sheet. Perform autoradiography to obtain an image of the hybridised DNA. THis is image can be used to help create a detailed restriction map for this region of the genome.


=== References  ===
=== References  ===


<references /><br>
<references /><br>Molecular Biology of the Cell, 5th edition, 2008,&nbsp;B&nbsp;Alberts, p 539

Revision as of 14:29, 24 October 2012

Southern blotting, named after its inventor Edwin Southern, is a technique that is used to detect specific DNA sequences using gel-transfer hybridization.

Firstly you have to cut the DNA into smaller strands, this is done using a restriction enzyme. Then you need to perform a gel electrophoresis on agrose gel, using the fragments obtained.The smallest DNA fragments travel the furthest, as they are able to move more easily between the gaps in the agrose gel. Once the gel electrophoresis is complete place a nitrocellulous sheet over the gel, so the DNA fragments are transfered to the sheet. Wash the sheet in an alkaline solution, for example NaOH, this is to ensure that the double stranded DNA is separtaed before hybridization. Place the sheet in a sealed plastic bag thats contains a salt buffered solution and DNA nucleotides and leave in conditions that favour hybridization for a long period of time. Ensure the DNA nucleotides are labeled by a probe, either radioactive or fluroescent. Once hybridization is complete remove and wash the nitrocellulose sheet, so that only hybridised DNA molecules are left on the sheet. Perform autoradiography to obtain an image of the hybridised DNA. THis is image can be used to help create a detailed restriction map for this region of the genome.

References


Molecular Biology of the Cell, 5th edition, 2008, B Alberts, p 539

Retrieved from "https://teaching.ncl.ac.uk/bms/wiki//index.php?title=Southern_blotting&oldid=6761"