Table 1.
Mean peak area ratio of trimethylsilyl ethers
| Sterolsa added | Sterolsa quantified | Saponification conditionsa | |||
|---|---|---|---|---|---|
| 1M18hr24°Cb | 1M18hr37°C | 1M3hr45°C | 3.6M3hr24°C | ||
| Cholesterol | Cholesterol tms ether | 0.7502 ± 0.28 (100) | 0.8730 ± 0.18 (116) | 0.5468 ± 0.18 (73) | 0.7855 ± 0.12 (105) |
| 7-Ketocholesterol | 7-Ketocholesterol tms ether | 0.5071 ± 0.16 (100) | 0.2684 ± 0.10 (53) | 0.2484 ± 0.27 (49) | 0.3623 ± 0.20 (71) |
| 3,5-7-Onec | 0.0580 ± 0.03 (100) | 0.2309 ± 0.08 (398) | 0.1994 ± 0.22 (344) | 0.0241 ± 0.01 (41) | |
| β-Sitosterol | β-Sitosterol tms ether | 0.5669 ± 0.29 (100) | 0.6995 ± 0.26 (123) | 0.3334 ± 0.21 (59) | 0.5240 ± 0.25 (92) |
aSamples of cholesterol, 7-keto and β-sitosterol were saponified under the following conditions: 1 M methanolic KOH for 18 h at 24 °C (1M18hr24°C, Control), 18 h at 37 °C (1M18hr37°C), 3 h at 45 °C (1M3hr45°C), and 3.6 M methanolic KOH for 3 h at 24 °C (3.6M3hr24°C). Trimethylsilyl ethers (tms ethers) were quantified. Means (6 samples) and standard deviations with different letters are statistically different at P ≤ 0.10. Cholest-5-ene-7-one (5-ene-7-one) was used as an internal standard
b1M18hr24°C (cold saponification) was used as the control and for comparison because it is regarded by many researchers as appropriate for generation of minimal artifacts during analysis
cArtifact of 7-ketocholesterol, values were corrected to account for 3,5-7-one initially present in the 7-ketocholesterol standard