Abstract
AbstractSix flavonoid rhamnosides (1‐2, 4‐7) were separated from the water‐soluble non‐alkaloidal portion of the EtOH extract of the leaves of Neolitsea sericea var. aurata using various chromatographic techniques including Sephadex LH‐20, centrifugal partition chromatography, and RP‐18 Lobar. One additional compound (3) besides these six was identified by application of HPLC‐SPE‐NMR in a flavonoid rich fraction. The latter approach consumed only 1.5 mg of samples, theoretically equivalent to 0.2 g of dry leaves. This study demonstrates that HPLC‐SPE‐NMR has great advantage over the general methods on the aspects of manpower, research time, amounts of plant materials, and consumables in separation and characterization of natural products.
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