Table 1.
Differentiation of tested methods by variable
| Method 1 | Method 2 | Method 3 | Method 4 | Method 5 | Method 6 | Method 7 | |
|---|---|---|---|---|---|---|---|
| Early vs. Late bead-beatinga | Early | Late | Late | Early | Early | Early | Early |
| Bead Quantity | 150 mg | 150 mg | 150 mg | 75 mg | 150 mg | 150 mg | 150 mg |
| Phenol vs. No Phenolb | No phenol | No phenol | Phenol | No phenol | Phenol | No phenol | No phenol |
| Precipitation Temp/Reagentc | RT/2-Prop | RT/2-Prop | Cold ETOH | RT/2-Prop | RT/2-Prop | Cold ETOH | RT/2-Prop |
| Precipitation Saltd | NaOAc | NaOAc | NaOAc | NaOAc | NaCl | NaOAc | NaOAc |
| Number of washes | 3 | 3 | 3 | 3 | 3 | 3 | 5 |
a “Early” bead-beating refers to the timing prior to enzymatic digestion; “Late” bead-beating refers to timing after enzymatic digestion
All Early bead-beating was done in high SDS concentration, see Additional file 1
b DNA extractions in “no phenol” were extracted as described in Methods with chloroform:isoamyl alcohol (24:1, Tris-saturated)
Extractions in “phenol” were extracted using phenol:chloroform:isoamyl alcohol (25:24:1, Tris-saturated, pH 8.0)
c Precipitation reagent was either RT 2-Prop (room temperature isopropanol) or Cold ETOH (ethanol). See Additional file 4: Figure S1
d Precipitation salt was either 3 M sodium acetate (pH 5.2) or 5 M NaCl