Echinacea angustifolia
» Echinacea angustifolia consists of the dried rhizome and roots of Echinacea angustifolia DC. (Fam. Asteraceae). It is harvested in the fall after 1 or more years of growth. It contains not less than 0.5 percent of total phenols, calculated on the dried basis as the sum of caftaric acid (C13H12O9), chicoric acid (C22H18O12), chlorogenic acid (C16H18O9), dicaffeoylquinic acids (C25H24O12), and echinacoside (C35H46O20). It contains not less than 0.075 percent of dodecatetraenoic acid isobutylamides (C16H25NO) on the dried basis.
Packaging and storage—
Store in well-closed, light-resistant containers.
Labeling—
The label states the Latin binomial and, following the official name, the parts of the plant contained in the article.
USP Reference standards 
11
—
USP Chlorogenic Acid RS.
USP Powdered Echinacea angustifolia Extract RS. USP 2E,4E-Hexadienoic Acid Isobutylamide RS.
11—
USP Chlorogenic Acid RS.
USP Powdered Echinacea angustifolia Extract RS. USP 2E,4E-Hexadienoic Acid Isobutylamide RS.
Botanic characteristics—
Macroscopic—
The outer surface of the rhizome is pale to yellowish brown, crowned with remains of the aerial stem, and sometimes showing surface annulations up to 15 mm in diameter. The roots are also pale to yellowish brown, cylindrical or slightly tapering, sometimes spirally twisted, longitudinally wrinkled and deeply furrowed, up to 4 to 10 mm in diameter, and passing imperceptibly into rhizome. The short fracture, when dry, becomes tough and pliable on exposure to air.
Microscopic—
The rhizomes and roots in transverse section show a thin outer bark separated from a wide xylem by a distinct cambial line. The cork is composed of several rows of thin-walled cells containing yellowish brown pigment. The rhizome has a small circular pith, occasional small groups of thick-walled, lignified fibers in the pericycle, and a parenchymatous cortex. The phloem and xylem are composed of narrow strands of vascular tissue separated by wide, non-lignified medullary rays. Xylem vessels are lignified, 25 to 75 µm in diameter, usually with reticulate thickening but occasionally with spiral or annular thickening. Sclereids occur singly or in small groups, varying considerably in size and shape from rounded to rectangular to elongated and fiber-like, up to 300 µm long and 20 to 40 µm wide, with intercellular spaces forming schizogenous oleoresin canals that are 80 to 150 µm in diameter and contain a dense black deposit. The canals are present outside of the central cylinder only (unlike Echinacea pallida, where they are present both inside and outside of the central cylinder). Spherocrystalline masses of inulin occur throughout the parenchymatous tissues. Lignified fibers, 300 to 800 µm long, are present in scattered groups, and are usually surrounded by phytomelanin (unlike fibers in Echinacea pallida, where they usually occur singly in the periphery of the cortex and are 100 to 300 µm long, with phytomelanin often absent).
Identification—
A:
Thin-Layer Chromatographic Identification Test 201—
201—
presence of echinacoside and dicaffeoylquinic acids (cynarin(e))—
Test solution—
Weigh and finely pulverize about 10 g of Echinacea angustifolia, and transfer 1 g of the powder to a suitable extraction thimble. Transfer the thimble to a continuous extraction apparatus, and extract with 50 mL of chloroform for 1 hour. Retain the chloroform extract for Identification test B. Continue the extraction with 50 mL of methanol, and concentrate to a small volume at 40
in vacuum. With the aid of methanol, transfer the extract to a 10-mL volumetric flask, and dilute with methanol to volume.
in vacuum. With the aid of methanol, transfer the extract to a 10-mL volumetric flask, and dilute with methanol to volume.
Standard solution 1—
Dissolve an accurately weighed quantity of USP Powdered Echinacea angustifolia Extract RS in methanol to obtain a solution having a concentration of about 20 mg per mL.
Standard solution 2—
Dissolve an accurately weighed quantity of 1,3-dicaffeoylquinic acid in methanol to obtain a solution having a concentration of about 1 mg per mL.
Developing solvent system—
Prepare a mixture of ethyl acetate, formic acid, and water (17:2:1).
Spray reagent 1—
Dissolve a suitable quantity of diphenylborinic acid, ethanolamine ester in methanol to obtain a solution having a concentration of about 10 mg per mL.
Spray reagent 2—
Dissolve a suitable quantity of polyethylene glycol 4000 in alcohol to obtain a solution having a concentration of about 50 mg per mL.
Procedure—
Proceed as directed in the chapter. Develop the chromatograms in Developing solvent system until the solvent front has moved not less than 12 cm, and dry the plate in a current of air. Spray the plate with Spray reagent 1 followed by Spray reagent 2, and examine the plate under UV light at 365 nm: the chromatogram obtained from the Test solution shows a yellowish zone at an RF value of 0.14 characteristic of echinacoside (absent or only traces present in Echinacea purpurea) that corresponds in color and RF value to that in the chromatogram of Standard solution 1, and another zone characteristic of 1,3-dicaffeoylquinic acid (absent in Echinacea pallida and Echinacea purpurea) corresponding in color and RF value to that in the chromatogram of Standard solution 2. Other colored zones of varying intensities may be observed in the chromatogram of the Test solution.
B: Thin-Layer Chromatographic Identification Test 201—
201—
presence of isobutylalkenylamides—
Test solution—
Evaporate the chloroform extract retained from preparation of the Test solution in Identification test A to dryness at 40 in vacuum. To the residue, add 1 mL of alcohol, and pass through a nylon membrane filter having a porosity of 0.45 µm.
in vacuum. To the residue, add 1 mL of alcohol, and pass through a nylon membrane filter having a porosity of 0.45 µm.
Standard solution 1—
Transfer an accurately weighed quantity of USP Powdered Echinacea angustifolia Extract RS to a centrifuge tube, and add chloroform to obtain a solution having a known concentration of about 100 mg per mL. Shake by hand to disperse, sonicate for 5 minutes, and centrifuge. Use the supernatant.
Standard solution 2—
Dissolve an accurately weighed quantity of 
-sitosterol in methanol to obtain a solution having a concentration of about 1 mg per mL.
-sitosterol in methanol to obtain a solution having a concentration of about 1 mg per mL.
Developing solvent system—
Prepare a mixture of hexane and ethyl acetate (2:1).
Spray reagent—
Prepare a mixture of glacial acetic acid, sulfuric acid, and p-anisaldehyde (10:5:0.5)in an ice bath.
Procedure—
Proceed as directed in the chapter. Develop the chromatograms in Developing solvent system until the solvent front has moved not less than 12 cm, and dry the plate in a current of air. Examine the plate under UV light at 254 nm: the chromatogram obtained from the Test solution shows one main zone at an RF value of about 0.25 due to 2E,4E,8Z,10E-dodecatetraenoic acid isobutylamide and dodeca-2E,4E,8Z,10Z-tetraenoic acid isobutylamide (absent in E. pallida) that corresponds in RF value to that in the chromatogram of Standard solution 1. Spray the plate with Spray reagent, and then heat the plate at 100 for 5 minutes: the chromatogram obtained from the Test solution shows a zone due to -sitosterol that corresponds in RF value to the principal spot in the chromatogram of Standard solution 2, below this spot, there is a zone due to dodeca-2E,4E,8Z,10E-tetraenoic acid isobutylamide and to dodeca-2E,4E,8Z,10Z-tetraenoic acid isobutylamide that corresponds in RF value to that in the chromatogram of Standard solution 1, and below this spot, there are several yellowish zones due to 
,-unsaturated isobutylamides (absent in Echinacea pallida and mostly violet in Echinacea purpurea due to the presence of ,,
,
-unsaturated isobutylamides) that are not visible or are very weak when viewed under UV light at 254 nm.
for 5 minutes: the chromatogram obtained from the Test solution shows a zone due to -sitosterol that corresponds in RF value to the principal spot in the chromatogram of Standard solution 2, below this spot, there is a zone due to dodeca-2E,4E,8Z,10E-tetraenoic acid isobutylamide and to dodeca-2E,4E,8Z,10Z-tetraenoic acid isobutylamide that corresponds in RF value to that in the chromatogram of Standard solution 1, and below this spot, there are several yellowish zones due to ,-unsaturated isobutylamides (absent in Echinacea pallida and mostly violet in Echinacea purpurea due to the presence of ,,,-unsaturated isobutylamides) that are not visible or are very weak when viewed under UV light at 254 nm.
C:
The retention time of the major peak in the chromatogram of the Test solution corresponds to that of the echinacoside peak in the chromatogram of Standard solution 1, as obtained in the test for Content of total phenols. The chromatogram of the Test solution shows a peak for 1,3-dicaffeoylquinic acid corresponding in retention time to that obtained with Standard solution 1.
Loss on drying 731:
Dry it at 105 for 2 hours: it loses not more than 10.0%.
731:
Dry it at 105 for 2 hours: it loses not more than 10.0%.
Foreign organic matter 561:
not more than 3.0%.
561:
not more than 3.0%.
Total ash 561:
not more than 7.0%.
561:
not more than 7.0%.
Acid-insoluble ash 561:
not more than 4.0%.
561:
not more than 4.0%.
Pesticide residues 561:
meets the requirements.
561:
meets the requirements.
Heavy metals, Method III 231:
0.001%.
231:
0.001%.
Content of total phenols—
Solvent—
Prepare a mixture of alcohol and water (7:3).
Solution A—
Prepare a filtered and degassed solution of phosphoric acid (0.1 in 100).
Solution B—
Use filtered and degassed acetonitrile.
Mobile phase—
Use variable mixtures of Solution A and Solution B as directed for Chromatographic system. Make adjustments if necessary (see System Suitability under Chromatography 621).
621).
Standard solution 1—
Dissolve an accurately weighed quantity of USP Powdered Echinacea angustifolia Extract RS in Solvent, shaking and heating in a water bath. Dilute with Solvent to obtain a solution having a known concentration of about 1 mg of per mL. Pass through a membrane filter having a 0.45-µm or finer porosity.
Standard solution 2—
Dissolve an accurately weighed quantity of USP Chlorogenic Acid RS in Solvent, shaking for 1 minute. Dilute quantitatively, and stepwise if necessary, with Solvent to obtain a solution having a known concentration of about 40 µg per mL. Pass through a membrane filter having a 0.45-µm or finer porosity.
Test solution—
Transfer about 125 mg of finely powdered Echinacea angustifolia (capable of passing through a 40-mesh sieve), accurately weighed, to a round bottom flask equipped with a condenser. Add 25.0 mL of Solvent, and heat under reflux, while shaking by mechanical means, for 15 minutes. Centrifuge, or pass through a membrane filter having a 0.45-µm or finer porosity.
Chromatographic system (see Chromatography 621)—
The liquid chromatograph is equipped with a 330-nm detector and a 4.6-mm × 25-cm column that contains 5-µm packing L1. The column temperature is maintained at 35. The flow rate is about 1.5 mL per minute. The chromatograph is programmed as follows.
Chromatograph Standard solution 1, and record the peak responses as directed for Procedure: the chromatogram obtained is similar to the Reference Chromatogram for total phenols provided with the USP Powdered Echinacea angustifolia Extract RS and the resolution, R, between the 1,3-dicaffeoylquinic acid isomer and echinacoside is not less than 1.0. Chromatograph Standard solution 2, and record the peak responses as directed for Procedure: the capacity factor, k¢, is not less than 3.0; the tailing factor is not more than 2.0; and the relative standard deviation for replicate injections is not more than 2.5%.
621)—
The liquid chromatograph is equipped with a 330-nm detector and a 4.6-mm × 25-cm column that contains 5-µm packing L1. The column temperature is maintained at 35. The flow rate is about 1.5 mL per minute. The chromatograph is programmed as follows.
| Time (minutes) |
Solution A
(%) |
Solution B
(%) |
Elution |
| 0–13 | 90®78 | 10®22 | linear gradient |
| 13–14 | 78®60 | 22®40 | linear gradient |
| 14–17 | 60 | 40 | isocratic |
| 17–17.5 | 60®90 | 40®10 | linear gradient |
| 17.5–22 | 90 | 10 | equilibration |
Procedure—
Separately inject equal volumes (about 5 µL) of Standard solution 1, Standard solution 2, and the Test solution into the chromatograph, record the chromatograms, and measure the areas for the relevant peaks. Identify the relevant analytes in the chromatogram obtained from the Test solution by comparison with the chromatogram obtained from Standard solution 1. Separately calculate the percentage of caftaric acid (C13H12O9), chicoric acid (C22H18O12), chlorogenic acid (C16H18O9), dicaffeoylquinic acids (C25H24O12), and echinacoside (C35H46O20) in the portion of Echinacea angustifolia taken by the formula:
2500F(C/W)(ri / rS)
in which F is the response factor and is equal to 0.695 for chicoric acid, 0.729 for dicaffeoylquinic acids, 0.881 for caftaric acid, 1.000 for chlorogenic acid, and 2.220 for echinacoside; C is the concentration, in mg per mL, of USP Chlorogenic Acid RS in Standard solution 2; W is the weight, in mg, of Echinacea angustifolia taken; and ri and rS are the peak responses for the relevant analyte obtained from the Test solution and Standard solution 2, respectively. Calculate the percentage of total phenols in the portion of Echinacea angustifolia taken by adding the individual percentages calculated.
Content of dodecatetraenoic acid isobutylamides—
Mobile phase—
Prepare a filtered and degassed mixture of acetonitrile and water (55:45).
Standard solution 1—
Dissolve, with sonication, an accurately weighed quantity of USP Powdered Echinacea angustifolia Extract RS in methanol, shaking for 10 minutes, and dilute with methanol to obtain a solution having a concentration of about 5 mg per mL. Pass through a membrane filter having a 0.45-µm or finer porosity.
Standard solution 2—
Dissolve an accurately weighed quantity of USP 2E,4E-Hexadienoic Acid Isobutylamide RS in methanol, shaking for 1 minute. Dilute quantitatively, and stepwise if necessary, with methanol to obtain a solution having a known concentration of about 10 µg per mL. Pass through a membrane filter having a 0.45-µm or finer porosity.
Test solution—
Transfer about 2.5 g of finely powdered Echinacea angustifolia (capable of passing through a 40-mesh sieve), accurately weighed, into a round-bottom flask. Add 80 mL of methanol, and reflux for 30 minutes. Cool to room temperature, and filter into a 100-mL volumetric flask, using small portions of methanol to rinse the flask and the filter. Dilute with methanol to volume, and mix. Pass through a membrane filter having a 0.45-µm or finer porosity.
Chromatographic system (see Chromatography 621)—
The liquid chromatograph is equipped with a 254-nm detector and a 4.6-mm × 25-cm column that contains 5-µm packing L1. The column temperature is maintained at 30. The flow rate is about 1.5 mL per minute. Chromatograph Standard solution 1, and record the peak responses as directed for Procedure: the chromatogram obtained is similar to the Reference Chromatogram for alkamides provided with USP Powdered Echinacea angustifolia Extract RS; and the resolution, R, between dodecatetraenoic acid isobutylamide peaks is not less than 1.0. Chromatograph Standard solution 2, and record the peak responses as directed for Procedure: the tailing factor is not more than 2.0; and the relative standard deviation for replicate injections is not more than 2.5%.
621)—
The liquid chromatograph is equipped with a 254-nm detector and a 4.6-mm × 25-cm column that contains 5-µm packing L1. The column temperature is maintained at 30. The flow rate is about 1.5 mL per minute. Chromatograph Standard solution 1, and record the peak responses as directed for Procedure: the chromatogram obtained is similar to the Reference Chromatogram for alkamides provided with USP Powdered Echinacea angustifolia Extract RS; and the resolution, R, between dodecatetraenoic acid isobutylamide peaks is not less than 1.0. Chromatograph Standard solution 2, and record the peak responses as directed for Procedure: the tailing factor is not more than 2.0; and the relative standard deviation for replicate injections is not more than 2.5%.
Procedure—
Separately inject equal volumes (about 25 µL) of Standard solution 1, Standard solution 2, and the Test solution into the chromatograph, record the chromatograms, and measure the areas for the relevant peaks. Identify the peaks due to 2E,4E,8Z,10E-dodecatetraenoic acid isobutylamide and 2E,4E,8Z,10Z-dodecatetraenoic acid isobutylamide in the chromatogram obtained from the Test solution by comparison with the chromatogram obtained from Standard solution 1. Calculate the percentage of dodecatetraenoic acid isobutylamides in the portion of Echinacea angustifolia taken by the formula:
10,000(1.353)(C/W)(ri / rs)
in which 1.353 is the response factor for 2E,4E-hexadienoic acid isobutylamide; C is the concentration, in mg per mL, of USP 2E,4E-Hexadienoic Acid Isobutylamide RS in Standard solution 2; W is the weight, in mg, of the portion of Echinacea angustifolia taken; ri is the sum of the peak responses of the relevant analytes obtained from the Test solution; and rS is the peak response obtained from Standard solution 2.
Auxiliary Information—
Please check for your question in the FAQs before contacting USP.
Chromatographic Column—
| Topic/Question | Contact | Expert Committee |
| Monograph | Maged H. Sharaf, Ph.D.
Senior Scientist 1-301-816-8318 |
(DSB05) Dietary Supplements - Botanicals |
| Reference Standards | Lili Wang, Technical Services Scientist 1-301-816-8129 RSTech@usp.org |
USP32–NF27 Page 993
Pharmacopeial Forum: Volume No. 30(2) Page 552
Chromatographic columns text is not derived from, and not part of, USP 32 or NF 27.