Equisetum palustre (leaf)

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=Botanical Voucher Specimen=
 
=Botanical Voucher Specimen=
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| mainimage=Equisetum_palustre_Kew_imageBarcode=K001057681_650549.jpg
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| source=Royal Botanic Gardens, Kew.
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=Organoleptic Characteristics=
 
=Organoleptic Characteristics=
  

Latest revision as of 01:37, 19 August 2014

AHPA recognizes other valuable resources exist regarding the identity of Equisetum palustre.

To submit a suggestion or contribution, please contact Merle Zimmermann.

Contents

Nomenclature

Botanical Voucher Specimen

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Equisetum palustre Kew imageBarcode=K001057681 650549.jpg
Source: Royal Botanic Gardens, Kew.[1]


Organoleptic Characteristics

Macroscopic Characteristics

Microscopic Characteristics

High Performance Thin Layer Chromatographic Identification

HPTLC-assoc-Logo-farbig-Text-schwarz-300x47.png
(thumbnail)
Marsh horsetail herb (leaf) HPTLC ID - NP and PEG reagent, UV 366 nm

Marsh horsetail herb (leaf) (Equisetum palustre)

Lane Assignments Lanes, from left to right (Track, Volume, Sample):

  1. 2 µL Marsh horsetail herb 1
  2. 5 µL Marsh horsetail herb 1
  3. 8 µL Marsh horsetail herb 1
  4. 1 µL Rutin, hyperoside, caffeic acid (with increasing Rf)
  5. 2 µL Common horsetail herb 1
  6. 5 µL Common horsetail herb 1
  7. 8 µL Common horsetail herb 1
  8. 5 µL Common horsetail herb 2
  9. 5 µL Common horsetail herb 3
  10. 5 µL Common horsetail herb 4
  11. 5 µL Common horsetail herb 5
  12. 5 µL Common horsetail herb 6 (adulterated with Marsh horsetail herb)
  13. 5 µL Common horsetail herb 2 (adulterated with Marsh horsetail herb)
  14. 5 µL Common horsetail herb 3 (adulterated with Marsh horsetail herb) 

Reference Sample(s) Reference: Individually dissolve 1 mg of caffeic acid, 1 mg of rutin, and 1 mg of hyperoside each in 1 mL of methanol. 

Stationary Phase Stationary phase, i.e. Silica gel 60, F254 

Mobile Phase Ethyl acetate, water, acetic acid, formic acid 134:36:15:15 (v/v/v/v) 

Sample Preparation Method Sample: Mix 1 g of powdered sample with 10 mL of methanol and sonicate for 10 minutes, then centrifuge or filter the solutions and use the supernatants / filtrates as test solutions.

Derivatization reagent: NP reagent, Preparation: 1 g of natural products reagent in 200 mL of ethyl acetate; 2.) PEG reagent, Preparation: 10 g of polyethylene glycol 400 in 200 mL of methylene chloride, Use: Heat plate for 3 min at 100°C, dip (time 0, speed 5) in NP reagent, dry and dip (time 0, speed 5) in PEG reagent. 

Detection Method Saturated chamber; developing distance 70 mm from lower edge; relative humidity 33% 

Other Notes Images presented in this entry are examples and are not intended to be used as basis for setting specifications for quality control purposes.

System suitability test: Rutin: orange fluorescent zone at Rf ~ 0.34; Hyperoside: orange fluorescent zone at Rf ~ 0.50; Caffeic acid: light blue fluorescent zone at Rf ~ 0.88.

Identification: Compare result with reference images. The fingerprint of the test solution is similar to that of the corresponding botanical reference sample. Additional weak zones may be present. The chromatogram of the test solutions shows four green zones between the application position and the zone due to reference substance rutin (green arrows). Right above the zone due to rutin there is a faint blue zone. Just below the solvent front there are two red zones due to chlorophylls.

Test for adulteration: There is no yellow zone at or right above the position of hyperoside (pink arrow); between hyperoside and caffeic acid there are not two intense blue zones (white arrow, Common horsetail herb).


Source: HPTLC Association [2]

Supplementary Information

Sources

  1. Royal Botanic Gardens, Kew. http://specimens.kew.org/herbarium/K001057681
  2. HPTLC Association http://www.hptlc-association.org/
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