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Human Genomic DNA Isolation for Molecular Genetics Clinical Lab

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This comprehensive guide details the steps for isolating high-quality human genomic DNA, including methods such as phenol/chloroform extraction and spin-column DNA isolation. It covers cell lysis, protein removal, DNA precipitation, and quality assessment using techniques like gel electrophoresis. This document is essential for lab professionals engaged in genetic research and DNA analysis.

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Uploaded on
April 26, 2025
Number of pages
3
Written in
2024/2025
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Irene
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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:
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