Difference between revisions of "Team:NAIT Edmonton/Modeling"
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− | <h3>As a quick overview, proteins are first denatured and linearized by SDS after being suspended in a protein sample loading buffer. Additionally, the SDS coats proteins with a negative charge. Immediately after denaturation, proteins are loaded into the wells of a polyacrylamide gel and an electric current is passed through it. The negatively charged proteins are pulled through the gel and migrate towards the electrode.</h3> | + | <h3>As a quick overview, proteins are first denatured and linearized by SDS after being suspended in a protein sample loading buffer. Additionally, the SDS coats proteins with a negative charge. Immediately after denaturation, proteins are loaded into the wells of a polyacrylamide gel and an electric current is passed through it. The negatively charged proteins are pulled through the gel and migrate towards the electrode. The model you see here is an example of a binding site for SDS in mammalian apoferritin. SDS binds to multiple sites such as these and along with a heat treatment, plays a role in linearizing the proteins. Often, heat treatment is skipped all together and proteins are completely denatured using only the detergent, SDS.</h3> |
Revision as of 01:02, 19 September 2015
Modeling