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Phytochemical screening

Abhishek Gupta
Abhishek Gupta

This document summarizes various phytochemical screening tests that can be used to identify the presence of important plant constituents like carbohydrates, proteins, alkaloids, flavonoids, tannins, saponins, anthraquinones, and other metabolites. It provides details of common confirmatory tests used which involve visual observation of color changes or formation of precipitates when plant extracts are treated with specific detecting reagents. The results of these tests can help determine the major phytoconstituent classes present in a plant sample.

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Phytochemical Screening Abhishek Gupta Associate Professor Department of Pharmacognosy, Hygia Institute of pharmaceutical Education & Research, Lucknow, Uttar Pradesh, India Test for Carbohydrates: Molisch's reagent (a-NaphthoI): 15g of a-naphthol was dissolved in 100ml of alcohol. Molisch’s test To the Sample 2-3 drops of 1% alcoholic - napthol solution and 2 ml of conc. sulphuric acid was added along the sides of the test tube. Appearance of purple to violet ring at the junction of two liquids shows the presence of carbohydrates. Anthrone test: 2 ml of anthrone reagent was added to 500 μl of extract. Formation of green blue colour gives a positive anthrone test. *Anthrone is a tricyclic aromatic ketone. It is used for a common cellulose assay and in the colorometric determination of carbohydrates. ** Carbohydrate is first hydrolysed into simple sugars using dilute hydrochloric acid. In hot acidic medium glucose is dehydrated to hydroxmethyl furfural. This compound forms with anthrone a green coloured product with absorption maximum at 630 nm. Test for Reducing Sugars: Fehling test: 2ml solution of Fehling A and Fehling B were taken in a test tube then dropwise sample were added. The mixture was shaken well and kept in a water bath for 10-15 minutes at 100 0C. A rusty brown or brick red colour precipitate confirms the presence of carbohydrates in the sample. Fehling solution: a) Fehling's solution A (Copper sulfate solution): 3.46g of CUSO4. 5H2O was dissolved in 50ml of distilled water. b) Fehling's solution B (Alkaline tartrate solution): 17.3g of potassium sodium tartrate (Rochelle salts, KNaC4H406. 4H2O) and 5g of NaOH were dissolved in 50 ml of distilled water. Benedict test: 2ml of Benedict reagent was added to the 1 ml of plant extract. Then the mixture was shaken well and placed in a water bath for 10-15 minutes. Formation of reddish precipitate indicates the presence of sugars in the sample.
Benedict's solution (Fehling's solution) is used to test for simple sugars such as glucose. It is a clear blue solution which is a combination of copper sulfate, sodium citrate, and sodium carbonate. Test for Mono-saccharides Barfoed’s Test: This reagent was prepared by dissolving 13.3 g of crystalline neutral copper acetate in 200 ml of 1 % acetic acid solution. The test residue dissolved in water and heated with a little of the reagent. If a red precipitate of cuprous oxide is formed within two minutes, mono-saccharides are present. Test for Starch: 1 ml of iodine solution is mixed in 1ml of extract; formation of blue colour indicated the presence of starch in the extract. Test for mucilage and gums Small quantities of sample was added separately to 25 ml of absolute alcohol with constant stirring and filtered. The precipitates was dried in oil and examined for its swelling property for the presence of gum and mucilage. To the sample add ruthenium red solution, pink color shows presence of mucilage. Test for proteins and free amino acids: Biuret test: 1% of NaoH was added to 1 ml of extract and few drops of 1% CuSO4 were then added. Blue/ purple or violet/ pinkish colour indicates the presence of proteins. *The biuret test, also known as Piotrowski's test. **The Biuret reagent is made of sodium hydroxide (NaOH) and hydrated copper(II) sulfate, together with potassium sodium tartrate,[5] the latter of which is added to chelate and thus stabilize the cupric ions. The reaction of the cupric ions with the nitrogen atoms involved in peptide bonds leads to the displacement of the peptide hydrogen atoms under the alkaline conditions. A tri- or tetra-dentate chelation with the peptide nitrogen produces the characteristic color. Millon’s test: 1 ml of test extract was mixed with H2SO4 then Millon’s reagent was added dropwise. White/yellow precipitate appears which turns into brick red colour precipitate, after heating the mixture. This indicates the presence of proteins and free amino acids. *Millon's reagent is prepared by dissolving mercuric nitrate in nitric acid, and then adding water to dilute it. **Millon's reagent is an analytical reagent used to detect the presence of soluble proteins. A few drops of the reagent are added to the test solution, which is then heated gently. A reddish-brown coloration or precipitate indicates the presence of tyrosine residue which occur in nearly all proteins. Ninhydrin’s test: 2 drops of freshly prepared Ninhydrin reagent (0.1% in n- butanol) is added to 1ml of extract and heat and observed for blue or red orange colour. * Ninhydrin (2,2-dihydroxyindane-1,3-dione) is a chemical used to detect ammonia or primary and secondary amines. Ninhydrin is most commonly used to detect fingerprints, as the terminal amines of lysine residues in peptides and proteins sloughed off in fingerprints react with ninhydrin. It is a white solid which is soluble in ethanol and acetone at room temperature.
** Ninhydrin reacts with the α-amino group of primary amino acids producing 'Ruhemann's purple'. The chromophore formed is the same for all primary amino acids. The intensity of the colour formed depends on the number and chemical nature of the amino groups being analysed. The optimum pH for the overall reaction is 5.5. Test for Xanthoproteins: One ml of extracts is treated separately with few drops of conc. HNO3 and NH3 solution. Formation of reddish orange precipitate indicates the presence of xanthoproteins. Tests for fixed oils and fats: Spot test: A small quantity of sample was separately pressed between two filter papers. Appearance of oil stain on the paper indicates the presence of fixed oil. Saponification test: Few drops of 0.5 N alcoholic potassium hydroxide were added to a small quantity of sample along with a drop of phenolpthlein, the mixture was heated on a water bath for 1-2 hours, formation of soap or partial neutralization of alkali indicates the presence of fixed oils and fats. *Saponification is the process by which the fatty acids in the triglycerides or fat are hyrdrolysed by an alkali to give glycerol and potassium salts of fatty acids. A known quantity of fat or oil is refluxed with an excess amount of alcoholic KOH. The value obtained is used for the determination of saponification number. Test for Alkaloids: Mayer’s test: 1ml of sample was added to a few drops of Mayer’s reagent. Formation of white or pale yellow precipitate indicates the presence of alkaloids in the sample. * Mayer's reagent: 5g of KI was dissolved in 10ml of water and 1.35g of HgCl2 was dissolved in 60ml of water. Then both the solutions were mixed together and water was added to make the solution to 100ml. Wagner’s test: 1.5% of HCl was added in 1 ml of extract and a few drops of Wagner’s reagent were added to it. Appearance of yellow/ brown precipitate indicates the presence of alkaloids. Hager’s test: 1ml of extract was taken in a test tube, and few drops of Hagers reagent was added to it. Yellow precipitate confirms the presence of alkaloids in the sample. * Wagner's reagent (lodo-potasium iodide): 2g of iodine and 6g of KI was dissolved in 100ml of water Dragendorff test: 5ml of distilled water was added to the the 2 ml of sample, then 2M HCl and 1 ml of Dragondrof’s reagent (potassium bismuth iodide solution) was added. Orange / orange red precipitate indicates the presence of alkaloids. Hager’s Test: When the test filtrate was treated with this reagent, an orange yellow precipitate was formed indicating the presence of alkaloids. *Hager's reagent (Picric acid): 1g of picric acid was dissolve in 100ml of water to prepare Hager's reagent (saturated aqueous solution of picric acid). Valser’s test: A few drops of Valser’s reagent are added to a few mL of plant extract. A reddish- brown precipitate indicates a positive result.
*Valser’s reagent is Potassium iodide solution in Mercuric iodide. Tannic acid Test: A few drops of 10% Tannic acid solution are added to a few mL of plant extract. A Buff coloured precipitate indicates a positive result. Test for Glycosides Legal’s test: To the sample add 1 ml of pyridine and few drops of sodium nitropruside solutions and then it was made alkaline with sodium hydroxide solution. Appearance of pink to red colour shows the presence of glycosides. Borntrager’s test: Sample was treated with chloroform and then the chloroform layer was separated. To this equal quantity of dilute ammonia solution was added. Ammonia layer acquires pink color, showing the presence of glycosides. Baljet’s test: To the sample add Sodium picrate solution, orange color shows presence of glycosides. Test for cardiac glycosides: Keller-Killani test: Treat the extract with 2 ml of glacial acetic acid containing one drop of ferric chloride solution. Add 1ml of conc. sulphuric acid. Appearance of brown ring at the interface indicates the deoxysugar characteristic of cardenolides. Appearance of a violet ring below the brown ring & a greenish ring in the acetic acid layer confirmed the results. Test for tannins and phenolic compounds A small quantity of the sample was taken separately in water and test for the presence of phenol compounds and tannins was carried out with the following reagents: Lead acetate test: The extract (50 mg) is dissolved in distilled water. Then 3 mL of 10% lead acetate solution is added. A bulky white precipitate indicates the presence of phenolic compounds. Potassium Dichromate Test: If on an addition of a solution of potassium dichromate in test filtrate, dark color is developed, tannins are present. Test for Tannins: To 1 ml of the extract, 2ml of 5% FeCl3 is added which gives dark blue or greenish black colour and a positive tannin test. Test for Phlobatannins: 1ml of plant extract was treated with 1 ml of 1% HCl and heat. Red colour precipitate indicates the presence of Phlobatannins in the sample. Test for flavonoids: Alkaline reagent test To the test solution add few drops of magnesium hydroxide solution, intense yellow colour is formed which turns to colourless on addition of few drops of dilute acid indicates presence of flavonoids. Shinoda’s test Small quantities of the sample was dissolved in alcohol, to them piece of magnesium followed by conc. hydrochloric acid drop wise added and heated. Appearance of pink, crimson red, green to blue color shows the presence of flavonoids.
Bate–Smith and Metcalf test: 0.5 mL of concentrated hydrochloric acid is added to the extract. It is then warmed on a water bath for 15 minutes and is observed for an hour. A strong red or violet colour means a positive result. Lead acetate Test: Treat the extract with few drops of lead acetate solution. Formation of yellow precipitate indicated the presence of flavonoids. H2SO4 test: A fraction of the extract was taken and treated with concentrated H2SO4 and observed for the formation of orange colour. Ferric Chloride Test: Add a few drops of ferric chloride solution to the extract solution. Development of intense green colour indicates the presence of flavonoids. Test for Anthocyanin and Betacynin: 1 ml of plant extract was treated with 1 ml of 2N NaOH then heated. Formation of bluish –green colour indicated the presence of Anthocynin while yellow colour indicated the presence of betacynin. Tests for steroids and triterpenoids Libermann-burchard test Treat the sample with few drops of acetic anhydride, boil and cool. Then add conc. sulphuric acid from the side of test tube, brown ring is formed at the junction two layers and upper layer turns green which shows presence of steroids and formation of deep red colour indicates presence of phytosterols and triterpenoid. Salkowski test Mix 2 ml of chloroform to extract solution carefully added conc. Sulphuric acid (3 ml) to form a layer, red colour at lower layer indicates presence of steroids and formation of yellow coloured lower layer indicates presence of triterpenoids. Test for Terpinoids: To 1ml of plant extract, 2ml of chloroform and 3ml of conc. H2SO4 was added. A reddish brown precipitate at their interface, confirmed the presence of terpenoids. Test for waxes: To the test solution add alcoholic alkali solution, waxes get saponified. Test for Resins: 1ml of ethanolic extract was dissolved in acetone and then 1 ml of distilled water is added. Turbidity indicates the presence of resins. One ml of extract was treated with few drops of acetic anhydride solution followed by one ml of conc. H2SO4. Resins give colouration ranging from orange to yellow. Test for Carboxylic acid: One ml of the various extracts was separately treated with a few ml of sodium bicarbonate solution. Effervescence (due to liberation of carbon dioxide) indicates the presence of carboxylic acid. Test for Coumarins: 0.5 g of the moistened various extracts was taken in a test tube. The mouth of the tube was covered with filter paper treated with 1 N NaOH solution. Test tube was placed for few minutes in boiling water and then the filter paper was removed and examined under the UV light for yellow fluorescence indicated the presence of coumarins.
*Coumarins are a family of benzopyrones (1,2-benzopyrones or 2H-1-benzopyran-2-ones) widely distributed in the nature. They represent an important family of naturally occurring and/or synthetic oxygen-containing heterocycles, bearing a typical benzopyrone framework. Test for Quinones: One ml of each of the various extracts was treated separately with alcoholic potassium hydroxide solution. Quinines give coloration ranging from red to blue. * The quinones are a class of organic compounds that are formally "derived from aromatic compounds [such as benzene or naphthalene] by conversion of an even number of –CH= groups into –C(=O)– groups with any necessary rearrangement of double bonds", resulting in "a fully conjugated cyclic dione structure".
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Phytochemical screening

  • 1. Phytochemical Screening Abhishek Gupta Associate Professor Department of Pharmacognosy, Hygia Institute of pharmaceutical Education & Research, Lucknow, Uttar Pradesh, India Test for Carbohydrates: Molisch's reagent (a-NaphthoI): 15g of a-naphthol was dissolved in 100ml of alcohol. Molisch’s test To the Sample 2-3 drops of 1% alcoholic - napthol solution and 2 ml of conc. sulphuric acid was added along the sides of the test tube. Appearance of purple to violet ring at the junction of two liquids shows the presence of carbohydrates. Anthrone test: 2 ml of anthrone reagent was added to 500 μl of extract. Formation of green blue colour gives a positive anthrone test. *Anthrone is a tricyclic aromatic ketone. It is used for a common cellulose assay and in the colorometric determination of carbohydrates. ** Carbohydrate is first hydrolysed into simple sugars using dilute hydrochloric acid. In hot acidic medium glucose is dehydrated to hydroxmethyl furfural. This compound forms with anthrone a green coloured product with absorption maximum at 630 nm. Test for Reducing Sugars: Fehling test: 2ml solution of Fehling A and Fehling B were taken in a test tube then dropwise sample were added. The mixture was shaken well and kept in a water bath for 10-15 minutes at 100 0C. A rusty brown or brick red colour precipitate confirms the presence of carbohydrates in the sample. Fehling solution: a) Fehling's solution A (Copper sulfate solution): 3.46g of CUSO4. 5H2O was dissolved in 50ml of distilled water. b) Fehling's solution B (Alkaline tartrate solution): 17.3g of potassium sodium tartrate (Rochelle salts, KNaC4H406. 4H2O) and 5g of NaOH were dissolved in 50 ml of distilled water. Benedict test: 2ml of Benedict reagent was added to the 1 ml of plant extract. Then the mixture was shaken well and placed in a water bath for 10-15 minutes. Formation of reddish precipitate indicates the presence of sugars in the sample.
  • 2. Benedict's solution (Fehling's solution) is used to test for simple sugars such as glucose. It is a clear blue solution which is a combination of copper sulfate, sodium citrate, and sodium carbonate. Test for Mono-saccharides Barfoed’s Test: This reagent was prepared by dissolving 13.3 g of crystalline neutral copper acetate in 200 ml of 1 % acetic acid solution. The test residue dissolved in water and heated with a little of the reagent. If a red precipitate of cuprous oxide is formed within two minutes, mono-saccharides are present. Test for Starch: 1 ml of iodine solution is mixed in 1ml of extract; formation of blue colour indicated the presence of starch in the extract. Test for mucilage and gums Small quantities of sample was added separately to 25 ml of absolute alcohol with constant stirring and filtered. The precipitates was dried in oil and examined for its swelling property for the presence of gum and mucilage. To the sample add ruthenium red solution, pink color shows presence of mucilage. Test for proteins and free amino acids: Biuret test: 1% of NaoH was added to 1 ml of extract and few drops of 1% CuSO4 were then added. Blue/ purple or violet/ pinkish colour indicates the presence of proteins. *The biuret test, also known as Piotrowski's test. **The Biuret reagent is made of sodium hydroxide (NaOH) and hydrated copper(II) sulfate, together with potassium sodium tartrate,[5] the latter of which is added to chelate and thus stabilize the cupric ions. The reaction of the cupric ions with the nitrogen atoms involved in peptide bonds leads to the displacement of the peptide hydrogen atoms under the alkaline conditions. A tri- or tetra-dentate chelation with the peptide nitrogen produces the characteristic color. Millon’s test: 1 ml of test extract was mixed with H2SO4 then Millon’s reagent was added dropwise. White/yellow precipitate appears which turns into brick red colour precipitate, after heating the mixture. This indicates the presence of proteins and free amino acids. *Millon's reagent is prepared by dissolving mercuric nitrate in nitric acid, and then adding water to dilute it. **Millon's reagent is an analytical reagent used to detect the presence of soluble proteins. A few drops of the reagent are added to the test solution, which is then heated gently. A reddish-brown coloration or precipitate indicates the presence of tyrosine residue which occur in nearly all proteins. Ninhydrin’s test: 2 drops of freshly prepared Ninhydrin reagent (0.1% in n- butanol) is added to 1ml of extract and heat and observed for blue or red orange colour. * Ninhydrin (2,2-dihydroxyindane-1,3-dione) is a chemical used to detect ammonia or primary and secondary amines. Ninhydrin is most commonly used to detect fingerprints, as the terminal amines of lysine residues in peptides and proteins sloughed off in fingerprints react with ninhydrin. It is a white solid which is soluble in ethanol and acetone at room temperature.
  • 3. ** Ninhydrin reacts with the α-amino group of primary amino acids producing 'Ruhemann's purple'. The chromophore formed is the same for all primary amino acids. The intensity of the colour formed depends on the number and chemical nature of the amino groups being analysed. The optimum pH for the overall reaction is 5.5. Test for Xanthoproteins: One ml of extracts is treated separately with few drops of conc. HNO3 and NH3 solution. Formation of reddish orange precipitate indicates the presence of xanthoproteins. Tests for fixed oils and fats: Spot test: A small quantity of sample was separately pressed between two filter papers. Appearance of oil stain on the paper indicates the presence of fixed oil. Saponification test: Few drops of 0.5 N alcoholic potassium hydroxide were added to a small quantity of sample along with a drop of phenolpthlein, the mixture was heated on a water bath for 1-2 hours, formation of soap or partial neutralization of alkali indicates the presence of fixed oils and fats. *Saponification is the process by which the fatty acids in the triglycerides or fat are hyrdrolysed by an alkali to give glycerol and potassium salts of fatty acids. A known quantity of fat or oil is refluxed with an excess amount of alcoholic KOH. The value obtained is used for the determination of saponification number. Test for Alkaloids: Mayer’s test: 1ml of sample was added to a few drops of Mayer’s reagent. Formation of white or pale yellow precipitate indicates the presence of alkaloids in the sample. * Mayer's reagent: 5g of KI was dissolved in 10ml of water and 1.35g of HgCl2 was dissolved in 60ml of water. Then both the solutions were mixed together and water was added to make the solution to 100ml. Wagner’s test: 1.5% of HCl was added in 1 ml of extract and a few drops of Wagner’s reagent were added to it. Appearance of yellow/ brown precipitate indicates the presence of alkaloids. Hager’s test: 1ml of extract was taken in a test tube, and few drops of Hagers reagent was added to it. Yellow precipitate confirms the presence of alkaloids in the sample. * Wagner's reagent (lodo-potasium iodide): 2g of iodine and 6g of KI was dissolved in 100ml of water Dragendorff test: 5ml of distilled water was added to the the 2 ml of sample, then 2M HCl and 1 ml of Dragondrof’s reagent (potassium bismuth iodide solution) was added. Orange / orange red precipitate indicates the presence of alkaloids. Hager’s Test: When the test filtrate was treated with this reagent, an orange yellow precipitate was formed indicating the presence of alkaloids. *Hager's reagent (Picric acid): 1g of picric acid was dissolve in 100ml of water to prepare Hager's reagent (saturated aqueous solution of picric acid). Valser’s test: A few drops of Valser’s reagent are added to a few mL of plant extract. A reddish- brown precipitate indicates a positive result.
  • 4. *Valser’s reagent is Potassium iodide solution in Mercuric iodide. Tannic acid Test: A few drops of 10% Tannic acid solution are added to a few mL of plant extract. A Buff coloured precipitate indicates a positive result. Test for Glycosides Legal’s test: To the sample add 1 ml of pyridine and few drops of sodium nitropruside solutions and then it was made alkaline with sodium hydroxide solution. Appearance of pink to red colour shows the presence of glycosides. Borntrager’s test: Sample was treated with chloroform and then the chloroform layer was separated. To this equal quantity of dilute ammonia solution was added. Ammonia layer acquires pink color, showing the presence of glycosides. Baljet’s test: To the sample add Sodium picrate solution, orange color shows presence of glycosides. Test for cardiac glycosides: Keller-Killani test: Treat the extract with 2 ml of glacial acetic acid containing one drop of ferric chloride solution. Add 1ml of conc. sulphuric acid. Appearance of brown ring at the interface indicates the deoxysugar characteristic of cardenolides. Appearance of a violet ring below the brown ring & a greenish ring in the acetic acid layer confirmed the results. Test for tannins and phenolic compounds A small quantity of the sample was taken separately in water and test for the presence of phenol compounds and tannins was carried out with the following reagents: Lead acetate test: The extract (50 mg) is dissolved in distilled water. Then 3 mL of 10% lead acetate solution is added. A bulky white precipitate indicates the presence of phenolic compounds. Potassium Dichromate Test: If on an addition of a solution of potassium dichromate in test filtrate, dark color is developed, tannins are present. Test for Tannins: To 1 ml of the extract, 2ml of 5% FeCl3 is added which gives dark blue or greenish black colour and a positive tannin test. Test for Phlobatannins: 1ml of plant extract was treated with 1 ml of 1% HCl and heat. Red colour precipitate indicates the presence of Phlobatannins in the sample. Test for flavonoids: Alkaline reagent test To the test solution add few drops of magnesium hydroxide solution, intense yellow colour is formed which turns to colourless on addition of few drops of dilute acid indicates presence of flavonoids. Shinoda’s test Small quantities of the sample was dissolved in alcohol, to them piece of magnesium followed by conc. hydrochloric acid drop wise added and heated. Appearance of pink, crimson red, green to blue color shows the presence of flavonoids.
  • 5. Bate–Smith and Metcalf test: 0.5 mL of concentrated hydrochloric acid is added to the extract. It is then warmed on a water bath for 15 minutes and is observed for an hour. A strong red or violet colour means a positive result. Lead acetate Test: Treat the extract with few drops of lead acetate solution. Formation of yellow precipitate indicated the presence of flavonoids. H2SO4 test: A fraction of the extract was taken and treated with concentrated H2SO4 and observed for the formation of orange colour. Ferric Chloride Test: Add a few drops of ferric chloride solution to the extract solution. Development of intense green colour indicates the presence of flavonoids. Test for Anthocyanin and Betacynin: 1 ml of plant extract was treated with 1 ml of 2N NaOH then heated. Formation of bluish –green colour indicated the presence of Anthocynin while yellow colour indicated the presence of betacynin. Tests for steroids and triterpenoids Libermann-burchard test Treat the sample with few drops of acetic anhydride, boil and cool. Then add conc. sulphuric acid from the side of test tube, brown ring is formed at the junction two layers and upper layer turns green which shows presence of steroids and formation of deep red colour indicates presence of phytosterols and triterpenoid. Salkowski test Mix 2 ml of chloroform to extract solution carefully added conc. Sulphuric acid (3 ml) to form a layer, red colour at lower layer indicates presence of steroids and formation of yellow coloured lower layer indicates presence of triterpenoids. Test for Terpinoids: To 1ml of plant extract, 2ml of chloroform and 3ml of conc. H2SO4 was added. A reddish brown precipitate at their interface, confirmed the presence of terpenoids. Test for waxes: To the test solution add alcoholic alkali solution, waxes get saponified. Test for Resins: 1ml of ethanolic extract was dissolved in acetone and then 1 ml of distilled water is added. Turbidity indicates the presence of resins. One ml of extract was treated with few drops of acetic anhydride solution followed by one ml of conc. H2SO4. Resins give colouration ranging from orange to yellow. Test for Carboxylic acid: One ml of the various extracts was separately treated with a few ml of sodium bicarbonate solution. Effervescence (due to liberation of carbon dioxide) indicates the presence of carboxylic acid. Test for Coumarins: 0.5 g of the moistened various extracts was taken in a test tube. The mouth of the tube was covered with filter paper treated with 1 N NaOH solution. Test tube was placed for few minutes in boiling water and then the filter paper was removed and examined under the UV light for yellow fluorescence indicated the presence of coumarins.
  • 6. *Coumarins are a family of benzopyrones (1,2-benzopyrones or 2H-1-benzopyran-2-ones) widely distributed in the nature. They represent an important family of naturally occurring and/or synthetic oxygen-containing heterocycles, bearing a typical benzopyrone framework. Test for Quinones: One ml of each of the various extracts was treated separately with alcoholic potassium hydroxide solution. Quinines give coloration ranging from red to blue. * The quinones are a class of organic compounds that are formally "derived from aromatic compounds [such as benzene or naphthalene] by conversion of an even number of –CH= groups into –C(=O)– groups with any necessary rearrangement of double bonds", resulting in "a fully conjugated cyclic dione structure".