DNA pellet or eluate shows poor solubility with visible aggregates or turbidity. DNA remains undissolved after standard elution protocol, requiring extended incubation.
Common Causes
1Binding time exceeded recommendation (> 4 min standard or > 8 min high input), causing excessive DNA compacting
2Input amount exceeded limits: > 1 × 10⁷ cells at max agitation or > 5 × 10⁶ cells at low agitation or > 2 ml blood
3Incomplete resuspension of cell pellet during nuclei preparation, resulting in clumped cells and tangled DNA
4For blood: leukocyte pellets not completely resuspended (frozen or aged blood causes sticky leukocytes)
5For blood: erythrocyte lysis extended too long, reducing leukocyte viability and causing stickiness
Solutions
1Do not exceed binding time: 4 min in vertical rotating mixer (standard) or 8 min for high input samples
3Ensure complete resuspension during nuclei preparation: pipette thoroughly to break up cell clumps
4For sticky leukocytes in frozen/aged blood: ensure complete resuspension after all pelleting steps
5Proceed through erythrocyte lysis rapidly; do not extend RBC Lysis Buffer incubation time
6For poorly dissolved DNA: incubate 5–15 min at 56°C with 300 rpm agitation, pipette with wide-bore tip, then leave overnight at room temperature or 30 min at 37°C