Separation of DNA Fragments Using PAGE Method

This method is able to separate DNA fragments with the size of as small as 10 bp and up to 1 kb with the resolution of as little as 1 bp. While agarose gel electrophoresis is only able to separate DNA fragments with the bigger size that PAGE does or in the size range of 100 nucleotides to around 10 – 15 kb.

Materials:

• Gel apparatus: Many designs of apparatus are commercially available. The gel is poured between two vertical plates held apart by spacers
  The plates should be cleaned thoroughly and then wiped with ethanol. To help ensure that the gel only sticks to one plate when the apparatus is disassembled, apply silicon to one of the gel plates. This is easily done by wiping the plate with a tissue soaked in dimethyl dichlorosilane solution and then washing the plate in distilled water followed by ethanol. If the plates are baked at 100^oC for 30 min, the siliconization will last four to five gel runs.
• Deionized H₂O: Autoclaved water is not necessary for the gel mix or running buffer, but it should be used for diluting samples and purification from gel slices.
• l0x TBE: 108 g of Trizma base (Tris), 55 g of boric acid, and 9.3 g of ethylenediaminetetraacetic acid (EDTA) (disodium salt). Make up to I L solution with deionized H₂O, which should be discarded when a precipitate forms.
• Acrylamide stock: 30% acrylamide, 1% N,N’-methylene bisacrylamide. Store at 4^oC. This is available commercially, or it can be made by dissolving acrylamide and bisacrylamide in water, which should be filtered. Acrylamide is a neurotoxin and therefore must be handled carefully. Gloves and a mask must be worn when weighing out.
• APS: 10% Ammonium persulphate (w/v). This can be stored at 4^oC for 1-2 months.
• TEMED: N,N,N’,N’-tetramethyl-l,2-diaminoethane. Store at 4^oC.
• 5X sample buffer: 15% Ficoll solution, 2.5X TBE, 0.25% (w/v) xylene cyanol and 0.025% (w/v) bromophenol blue.
• Ethidium bromide: A l0-mg/mL solution. Ethidium bromide is a potent mutagen and should be handled with care. Store at 4^oC in the dark.

Methods:

• For 50 mL, enough for a 18 x 14 x 0.15 cm gel, mix l0x TBE, acrylamide, H₂O, and APS as described in Table below.



• Just prior to pouring, add 50 microliters of TEMED and mix by swirling.
• Immediately pour the gel mix between the gel plates and insert the gel comb. Leave to set; this takes about 30 min.
• Fill the gel apparatus with 0.5X TBE and remove the comb. Use a syringe to wash out the wells, this may take multiple washes. It is important to remove as much unpolymerized acrylamide as possible because this impairs the running in of the samples
  If you are separating very small fragments, e.g., less than 50 bp, the gel should be prerun for 30 min, as this elevates the resolution problem experienced with fragments running close to the electrophoresis front..
• Add 0.2 volume of 5x sample buffer to each sample, usually in 10-20 microliters of TE, water, or enzyme buffer. Mix and spin the contents to the bottom of the tube
  High-salt buffers (above 50 mM NaCl) will affect sample mobility and tend to make bands collapse. In this case, salt should be removed by ethanol precipitation.
• Disassemble the gel apparatus and place the gel to stain in I mg/mL of ethidium bromide for approximately 30 min. View the stained gel on a transilluminator.

Hopefully the lab work on The Separation of DNA Fragments Using PAGE Method becomes doable for you and your lab partner.