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DNA Extraction and Quantitation for Forensic Analysts

Denaturation and Hydrolysis of Proteins

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Step Two: Denaturation and Hydrolysis of Proteins

Cells are lysed using a detergent, Proteinase K, and dithiothreitol (DTT). Extractions must use appropriate salt concentration and pH to ensure that proteins and other contaminants are separated into the organic phase and that DNA remains in the aqueous phase.

Detergents, which are included in the stain extraction buffer, have the following functions:

  • They lyse cell membranes.
  • They separate histone proteins from DNA.
  • They denature histone proteins.
  • They destroy secondary and tertiary structures of proteins, which decreases their solubility in aqueous solution.

Proteinase K is used to hydrolyze histone proteins and is well suited to the extraction process for the following reasons:

  • It is active over a wide pH range (4-12.5).
  • It is active in the presence of SDS.
  • It is not affected by EDTA.

Dithiothreitol (DTT) reduces disulfides to dithiols, allowing release of the DNA from its protective proteins and further degradation of the proteins by Proteinase K. DTT is an essential component for sperm cell lysis because the cell membrane contains a high concentration of disulfides.06

Diagram of Denaturation and Hydrolysis of Proteins
National Institute of Justice (NIJ) (see reuse policy).

Step Two Reagents

  • Detergents

Sarkosyl is generally used if a lysis procedure is conducted under refrigerated conditions (less than room temperature) because sodium dodecyl sulfate (SDS) precipitates out of solution at these temperatures. SDS is the detergent of choice when lysis procedures are conducted at room temperature.

  • Proteinase K

Proteinase K is produced by the fungus Tritirachium album Limber. It is an endolytic protease that cleaves peptide bonds at the carboxylic sides of aliphatic, aromatic, or hydrophobic amino acids. Proteinase K is classified as a serine protease. Proteinase K in the extraction buffer inactivates nucleases and aids in lysis of epithelial and white blood cells to free nuclear DNA. Nuclease inactivation is a very important step in DNA isolation. Nucleases naturally exist in the cell to break down the nucleic acids after they serve their functions in protein manufacture, thus allowing the individual building blocks of the DNA and RNA to be recycled by the cell. Inactivating these nucleases preserves the DNA so that it can be extracted and purified.06

Chemical makeup of Dithiothreitol
National Institute of Justice (NIJ) (see reuse policy).
  • DTT

DTT Construction. The DTT reduces disulfides to dithiols, allowing release of the DNA from its protective proteins and further degradation of the proteins by Proteinase K.

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