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HMW DNA Extraction (Monarch) critical

DNA Fragmentation and Size Reduction

Symptom
Extracted DNA shows reduced fragment size on gel electrophoresis or pulse-field gel analysis. UHMW DNA appears degraded with smaller molecular weight distribution than expected.
Common Causes
  1. 1 Extended heating of HMW samples: > 15–30 min at 56°C or > 1–3 hours at 37°C
  2. 2 UHMW DNA pipetted without wide-bore tips or vortexed, causing shearing
  3. 3 Blood samples thawed before adding RBC Lysis Buffer, activating nucleases
  4. 4 Fresh blood older than one week showing progressive degradation
  5. 5 Tissue samples not homogenized immediately or not placed in thermal mixer immediately after homogenization
  6. 6 Frozen tissue samples thawed before processing, allowing nuclease access to DNA
Solutions
  1. 1 Limit incubation times: maximum 15–30 min at 56°C, 1–3 hours at 37°C, or overnight at room temperature only
  2. 2 Always use wide-bore pipette tips for UHMW DNA; avoid vortexing
  3. 3 For frozen blood: keep frozen, add cold RBC Lysis Buffer directly to frozen sample
  4. 4 Process fresh blood within one week of collection
  5. 5 Place tissue samples in thermal mixer immediately after homogenization to inactivate nucleases rapidly
  6. 6 Keep frozen tissue samples frozen; work with smallest tissue pieces for rapid Proteinase K inactivation of nucleases; snap freeze in liquid nitrogen to minimize ice crystal damage
Related Video (2)
JoVE (YouTube) ★ 85
Extraction Of High Molecular Weight DNA From Microbial Mats l Protocol Preview
"Directly demonstrates HMW DNA extraction protocol with focus on preserving DNA integrity and avoiding degradation during handling and incubation steps"
JoVE (YouTube) ★ 82
Extraction: High Molecular Weight Genomic DNA From Soils & Sediments l Protocol Preview
"Shows HMW genomic DNA extraction technique from challenging samples with emphasis on proper temperature control and incubation time management to prevent fragmentation"
Source: neb.com ↗
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