2009 Mayıs | Turkish Chemistry - Part 3
May 14

Agarose gel electroporesis

Agarose electroporesis

Agarose electrophoresis separates DNA fragments according to their size. Typically, a DNA is digested with restriction enzymes, and the agarose electrophoresis is used as a diagnostic tool to visualize the fragments. An electric current is used to move the DNA across an agarose , which is a polysaccharide matrix that functions as a sort of sieve to help “catch” the as they are transported by the electric current.

This technique has lots of applications. Generally speaking you can analyze DNA fragments that result from an enzyme digestion of a larger piece of DNA to visualize the fragments and determine the sizes of the fragments. In addition to its usefulness in research techniques, agarose electrophoresis is a common forensic technique and is used in DNA fingerprinting.

The phosphate that make up the backbone of DNA have a high negative charge. When DNA is placed on a field with an electric current, these negatively charged DNA migrate toward the positive end of the field, whichin this case is an agarose immersed in a buffer bath. The agarose is a cross-linked matrix that is somewhat like a three-dimensional mesh or screen. The DNA are pulled to the positive end by the current, but they encounter resistance from this agarose mesh. The smaller are able to navigate the mesh faster than the larger one, so they make it further down the than the larger . This is how agarose electrophoresis separates different DNA according to their size. The is stained with ethidium bromide so you can visualize how these DNA resolved into bands along the .

Southern blotting may also be used as a visualization technique for agarose gels.


Unknown DNA samples are typically run on the same with a “ladder.” A ladder is a sample of DNA where the sizes of the bands are known. So after you run out your sample, you can compare the unknown fragments to the ladder fragments and determine the approximate size of the unknown DNA bands by how they match up to the known bands of the ladder.

May 12

SDS-PAGE

Where agarose gels are best for running larger molecules, like DNA, SDS-PAGE is better suited for running smaller ones, like proteins.

SDS-PAGE has a number of uses, which include:

  • Establishing
  • Protein identification
  • Determining sample purity
  • Identifying disulfide bonds
  • Quantifying proteins
  • Blotting applications

SDS-PAGE stands for sodium dodecyl (lauryl) sulfate-polyacrylamide electrophoresis. The SDS portion is a detergent. You may recognize it if you read the ingredients lists on your shampoo, soap, or toothpaste. The purpose of the SDS detergent is to take the protein from its native shape, which is basically a big glob, and open it up into a linear piece. It’s kind of like taking a wadded up ball of string and untangling it into one straight, long piece. This will allow it to run more efficiently down the and will get you better results, since it’s easier to compare two linear pieces of something rather than two of the same thing.

In more scientific terms, it is an that binds quantitatively to proteins, giving them linearity and uniform charge, so that they can be separated solely on the basis if their size. The SDS has a high negative charge that overwhelms any charge the protein may have, imparting all proteins with a relatively equal negative charge. The SDS has a hydrophobic tail that interacts strongly with protein (polypeptide) chains. The number of SDS molecules that bind to a protein is proportional to the number of amino acids that make up the protein. Each SDS contributes two negative charges, overwhelming any charge the protein may have. SDS also disrupts the forces that contribute to protein folding (tertiary structure), ensuring that the protein is not only uniformly negatively charged, but linear as well.

The polyacrylamide in a similar fashion to an agarose , separating protein molecules according to their size. In electrophoresis, an electric current is used to move the protein molecules across a polyacrylamide . The polyacrylamide is a cross-linked matrix that functions as a sort of sieve to help “catch” the molecules as they are transported by the electric current. The polyacrylamide acts somewhat like a three-dimensional mesh or screen. The negatively charged protein molecules are pulled to the positive end by the current, but they encounter from this polyacrylamide mesh. The smaller molecules are able to navigate the mesh faster than the larger one, so they make it further down the than the larger molecules. This is how SDS-PAGE separates different protein molecules according to their size.

Once an SDS-PAGE is run, you need to fix the proteins in the so they don’t come out when you stain the . Acetic acid 25% in water is a good fixative, as it keeps the proteins denatured. The is typically stained with Coomasie blue dye R250, and the fixative and dye can be prepared in the same solution using methanol as a solvent. The is then destained and dried.

May 12

Chromatography

Column chromatography is one of the most common methods of purification. Like many of the techniques on this site, it is as much an art form as a science. Proteins vary hugely in their properties, and the different types of column chromatography allow you to exploit those differences. Most of these methods do not require the denaturing of proteins.

To be very general, a is passed through a column that is designed to trap or slow up the passing of proteins based on a particular property (such as size, charge, or composition).

There are three main steps to purification:

    1. Capture. You need to get your into a concentrated form. If, for example, you are trying to isolate a you have synthesized in an E. coli cell, you could be looking at a to junk ratio of 1:1,000,000. For capture purification you need a high capacity method that is also fast. You need a speedy method because your crude solution is very likely to contain proteases in addition to your of interest that can quickly chew up your .

    2. Intermediate. Intermediate purification requires both speed and good resolution.

    3. Polishing. For the final step of purification you need a system that has both good resolution and speed. Capacity is usually irrelevant at this stage.

Some of the more common columns include:

  • IEX: Ion exchange chromatography. Good for capture, intermediate, and polish.
  • HIC: Hydrophobic interaction column. Good for intermediate purification.
  • AC: Affinity chromatography. Good for capture and intermediate purification.
  • GF: Gel filtration (size exclusion) chromatography. Good polishing step.

Let’s look at these types of columns in more detail.

Ion exchange chromatography

Ion exchange chromatography is based on the charge of the you are trying to isolate. If your has a high positive charge, you’ll want to pass it through a column with a negative charge. The negative charge on the column will bind the positively charged , and other proteins will pass through the column. You then use a procedure called “salting out” to release your positively charged from the negatively charged column. The column that does this is called a cation exchange column and often uses sulfonated residues. Likewise, you can bind a negatively charged to a positively charge column. The column that does this is called an anion exchange column and often uses quaternary ammonium residues.

Salting out will release, or elute, your from the column. This technique uses a high salt solution. The salt solution will out compete the in binding to the column. In other words, the column has a higher attraction for the charge of salts than for the charged , and it will release the in favor of binding the salts instead. Proteins with weaker ionic interactions will elute at a lower salt, so you will often want to elute with a salt gradient. Different proteins elute at different salt concentrations, so you will want to be sure you know the properties your well for best results.

Also be aware that changes in pH alter the charges in proteins. Be sure you know the isoelectric point of your (the isoelectric point is the pH at which the charge of a is zero) and make sure the pH of your system is adjusted and buffered accordingly.

The basic steps in using an ion exchange column are:

    1. Prep the column. Pour your buffer over the column to make sure it has equilibrated to the required pH.

    2. Load your solution. Some proteins in the solution don’t bind and will elute during this loading phase.

    3. Salt out. Increase the salt to elute the bound proteins. It is best to use a salt gradient to gradually elute proteins with different ionic strengths. At the end bump the system with a very high salt (2-3M) to make sure all proteins are off the column.

    4. Remove salts. Use dialysis to remove the salts from your solution.

Temperature doesn’t have a huge effect on column chemistry. However, it is better to work cold since proteins are more stable cold.

Hydrophobic interaction chromatography

Where ion exchange chromatography relies on the charges of proteins to isolate them, hydrophobic interaction chromatography uses the hydrophobic properties of some proteins. Hydrophobic groups on the bind to hydrophillic groups on the column. The more hydrophobic a is, the stronger it will bind to the column.

Load the proteins in the presence of a high of ammonium sulfate (not ammonium persulfate). Ammonium sulfate is a chaotropic agent. It increases the chaos (entropy) in water, and thereby increases hydrophobic interactions (the more disordered the water, the stronger the hydrophobic interactions). Ammonium sulfate also stabilizes proteins. So as a result of using an HIC column you can expect your to be in its most stable form.

The hydrophobic column is packed with a phenyl agarose matrix. In the presence of high salt concentrations the phenyl groups on this matrix binds hydrophobic portions of proteins. You can control elution of different column-bound proteins by reducing the salt or by adding solvents.

Affinity chromatography.

Affinity chromatography relies on the biological functions of a to bind it to a column. The most common type involves a ligand, a specific small biomolecule. This small molecule is immobilized and attached to a column matrix, such as cellulose or polyacrylamide. Your target is then passed through the column and bound to it by its ligand, while other proteins elute out. Elution of your target is usually done by passing through the column a solution that has in it a high of free ligand.  This is a very efficient purification method since it relies on the biological specificity of your target , such as the affinity of an enzyme for a substrate.

Gel filtration, or size exclusion, chromatography separates proteins on the basis of their size. The column is packed with a matrix of fine porous beads.

It works somewhat like a sieve, but in reverse. The beads have in them very small holes. As the solution is poured on the column, small molecules enter the pores in the beads. Larger molecules are excluded from the holes, and pass quickly between the beads.

These larger molecules are eluted first. The smaller molecules have a longer path to travel, as they get stuck over and over again in the maze of pores running from bead to bead. These smaller molecules, therefore, take longer to make their way through the column and are eluted last.

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