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Extraction Technologies For Medicinal And Aromatic Plants - Unido

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EXTRACTION TECHNOLOGIES FOR MEDICINAL AND AROMATIC PLANTS<br />

procedure, the stationary phase is more polar than the mobile phase. Lipophilic<br />

substances like oils, fats and lipids are separated by normal phase<br />

chromatography. Commonly used mobile solvents are n-hexane, heptane,<br />

chloroform, and alcohols. Most biomedical substances are separated by<br />

reverse phase chromatography using aqueous mixture with methanol, acetonitrile<br />

and additives (buffers, ion-pairs).<br />

11.2.2 Important Factors that Infl uence HPLC Separation<br />

HPLC separation is infl uenced by dead volume, capacity factor,<br />

theoretical plate count and selectivity:<br />

• Dead volume (V0) is the volume at which an un-retained component<br />

elutes.<br />

• Capacity factor (K ’ ) is a measurement of the retention time<br />

of a sample molecule, relative to column dead volume. It<br />

changes with variations in mobile phase composition, column<br />

surface chemistry or operating temperature. Capacity<br />

factor is calculated as follows:<br />

K ' = V1 – V0<br />

V0<br />

Ei<br />

V1 = Retention volume of peak 1<br />

• Theoretical plate count (N) is a measure of column effi ciency<br />

in terms of band-spreading of a peak. The smaller the bandspread,<br />

the higher the number of theoretical plates, which<br />

indicates good column and system performances.<br />

• Resolution (Rs) is the distance between the peak centres of<br />

two component peaks divided by the average base of the<br />

peaks, as follows:<br />

RS = V2 – V1<br />

√W1 + W2<br />

W1 = width of peak 1<br />

W2 = width of peak 2<br />

• Selectivity (α) is the relative retention of two peaks in a chromatogram.<br />

α = K' 2<br />

K ' 1<br />

= V2 – V0<br />

V1 – V0<br />

K 1 and K 2 = capacity factors for retention volume of peak 1<br />

and peak 2 respectively.<br />

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