1. By Zainab sajjad (117114) Ayesha Rehman (117115)
Gel Electrophoresis By
Zainab sajjad (117114)
Ayesha Rehman (117115)

2. What is gel electrophoresis
Gel electrophoresis is a laboratory method used to separate mixtures of DNA, RNA, or proteins according to molecular size.
In gel electrophoresis, the molecules to be separated are pushed by an electrical field through a gel that contains small pores.

3. The molecules travel through the pores in the gel at a speed that is inversely related to their lengths.
This means that a small DNA molecule will travel a greater distance through the gel than will a larger DNA molecule.

4. History
The history of electrophoresis begins in earnest with the work of Arne Tiselius in the 1930s, and new separation processes and chemical analysis techniques based on electrophoresis continue to be developed into the 21st century.

5. gel electrophoresis used for?
Gel electrophoresis is used to test for genes related to specific illnesses, to identify DNA associated with crime scenes, to discover paternity and to track evolutionary relationships. 
This technique is important in medical, biological and criminal science.

6. Purpose of Gel Electrophoresis
A method for separating DNA
Can be used to separate the size of
DNA
RNA
Protein

7. DNA
We start with: A variety of different fragments of DNA all mixed together
We will use gel electrophoresis to separate/sort these fragments

8. How It Separates
The gel is a porous How It Separates matrix (like a sponge)
Separates DNA based on
Size
Charge

9. Separation by Size
As DNA is moved through the gel, smaller sized fragments move through faster than larger sized fragments
Ex. A 100 base pair fragment will move through the gel faster than a 500 bp fragment

11. Separation Using Charge
The charge on DNA is what makes it move through the gel
DNA is a charged molecule. What is the charge on DNA?
Negative charge
Why?
Phosphate group is negatively charged

12. Separation Using Charge
DNA is loaded into the gel on the cathode (-) end
Gel is placed in a buffer solution that will conduct electricity
Electric current is run through the gel
DNA is attracted to the + end (anode)

14. The Gel Wells are created to put the DNA into
We use agarose gels to separate DNA

15. Solution #1
Problem #1: How can we see the DNA sample as we load it into the gel
Problem #2: How can we make sure DNA won’t float away
Solution: Add loading dye to the initial DNA sample!

16. Loading Dye
Adds mass to the DNA sample so that it will go into the well
makes it sink to the bottom
Adds blue color so we can see what we are pipeting

17. Solution #2
Problem: DNA is colorless. Once the DNA has been run through the gel, how can we see where it is on the gel?
Solution: Add Ethidium Bromide (EtBr) or Gel Red to the gel

18. Ethidium Bromide The DNA intercalates with the Ethidium Bromide (EtBr)
Intercalates = inserts itself between bases
Gel Red also stains nucleic acids
EtBr and Gel Red will fluoresce under UV light

20. Relative Size vs. Absolute Size
In gel, we can determine which fragments of DNA are bigger than others
Relative Size
Which fragment is bigger, A or B
Fragment A (didn’t travel as far in a fixed amount of time)

22. Absolute Size
How can we determine the actual size of the DNA fragments (how many base pairs- bp)?
Use a size standard
Also called a DNA ladder
Consists of a series of fragments of known sizes
Use it to compare to our DNA fragments