Human Genomic DNA Isolation
Key steps:
o Cell lysis
Disruption of cell membrane
o Separation of DNA from macromolecules
Inactivation/Inhibition of endogenous nucleases/proteases
Removal of other proteins (histones, other DNA binding proteins)
o Separation of DNA from small molecules
Removal of detergents & salts
o Concentration of DNA into smaller volume
Precipitation of DNA
Gel Electrophoresis
o One lane of raw purified DNA
o One lane of raw purified DNA + all other ingredients except RE
o One lane of DNA + all ingredients with RE
Potential Sources of DNA
o Blood (buffy coat)
From peripheral vein
Use EDTA (purple) or ACD (yellow) tubes
Isolate DNA within 96 hrs of blood collection for regular prep
Do not freeze whole blood
o Tissue
From CVS sampling, pathology lab, POC
o Cultured Cells
Can use suspension/fibroblast cultures
Sourced from cytogenetics lab
Use trypsin to remove cells from flask/dish
Phenol/Chloroform Method
o Most common method to remove proteins & isolation of the DNA by precipitation with EtOH
o Cell lysis:
Proteinase K Degrades membrane proteins
o Separation of DNA from macromolecules:
Remove proteins by phenol extraction followed by chloroform extraction
Phenol denatures proteins
Approx. 10% of phenol is in aq. Layer
Chloroform also denatures proteins, remove water from phenol
Isoamyl alcohol Reduces foaming & stabilizes interface between organic/aq. Phases
o Conc. of DNA into smaller volume
Precipitate nucleic acids with -OH in presence of high salt, induces transition in DNA
o Notes:
Key steps:
o Cell lysis
Disruption of cell membrane
o Separation of DNA from macromolecules
Inactivation/Inhibition of endogenous nucleases/proteases
Removal of other proteins (histones, other DNA binding proteins)
o Separation of DNA from small molecules
Removal of detergents & salts
o Concentration of DNA into smaller volume
Precipitation of DNA
Gel Electrophoresis
o One lane of raw purified DNA
o One lane of raw purified DNA + all other ingredients except RE
o One lane of DNA + all ingredients with RE
Potential Sources of DNA
o Blood (buffy coat)
From peripheral vein
Use EDTA (purple) or ACD (yellow) tubes
Isolate DNA within 96 hrs of blood collection for regular prep
Do not freeze whole blood
o Tissue
From CVS sampling, pathology lab, POC
o Cultured Cells
Can use suspension/fibroblast cultures
Sourced from cytogenetics lab
Use trypsin to remove cells from flask/dish
Phenol/Chloroform Method
o Most common method to remove proteins & isolation of the DNA by precipitation with EtOH
o Cell lysis:
Proteinase K Degrades membrane proteins
o Separation of DNA from macromolecules:
Remove proteins by phenol extraction followed by chloroform extraction
Phenol denatures proteins
Approx. 10% of phenol is in aq. Layer
Chloroform also denatures proteins, remove water from phenol
Isoamyl alcohol Reduces foaming & stabilizes interface between organic/aq. Phases
o Conc. of DNA into smaller volume
Precipitate nucleic acids with -OH in presence of high salt, induces transition in DNA
o Notes:
