Analyzing Aloe vera and Avocado Seed Extracts for Antioxidants, Saponins, Tannins, Flavonoids, and Alkaloids Using the UV-VIS Spectrophotometric Method

Nur Ariska Nugrahani; Cecilya Nella Yuppy Anggraeni; Noor Hafida Widyastuti; Mahmud Kholifa

doi:10.12688/f1000research.157091.1

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Research Article

Analyzing Aloe vera and Avocado Seed Extracts for Antioxidants, Saponins, Tannins, Flavonoids, and Alkaloids Using the UV-VIS Spectrophotometric Method

[version 1; peer review: 2 approved with reservations]

Nur Ariska Nugrahani ¹, Cecilya Nella Yuppy Anggraeni², Noor Hafida Widyastuti³, Mahmud Kholifa¹

PUBLISHED 06 Jan 2025

Author details Author details

¹ Department Oral Biology, Faculty of Dentistry, Universitas Muhammadiyah Surakarta, Surakarta, Central Java, 57141, Indonesia
² Faculty of Dentistry, Universitas Muhammadiyah Surakarta, Surakarta, Central Java, 57141, Indonesia
³ Department of Conservative Dentistry, Universitas Muhammadiyah Surakarta, Surakarta, Central Java, 57141, Indonesia

Nur Ariska Nugrahani
Roles: Conceptualization, Formal Analysis, Investigation, Methodology, Resources, Supervision, Validation, Visualization, Writing – Original Draft Preparation, Writing – Review & Editing

Cecilya Nella Yuppy Anggraeni
Roles: Data Curation, Investigation, Methodology, Validation, Visualization, Writing – Original Draft Preparation

Noor Hafida Widyastuti
Roles: Validation, Visualization

Mahmud Kholifa
Roles: Validation, Visualization

OPEN PEER REVIEW

REVIEWER STATUS

Abstract

Background

This study sought to quantify the levels of saponins, alkaloids, flavonoids, and tannins, as well as the IC50 values of avocado seed and aloe vera extracts.

Methods

The materials included in the investigation consisted of 70% ethanol extracts derived from avocado seeds and Aloe vera. Both samples underwent quantitative phytochemical analyses to ascertain total component content and an antioxidant activity assessment utilizing the 2,2-Diphenyl-1-picrylhydrazyl (DPPH) technique to evaluate % inhibition and IC50 values. The absorbance of the samples was quantified using a UV-Vis spectrophotometer, which facilitated the calculation of total chemical content and antioxidant activity.

Results

The avocado seed extract comprised saponins, alkaloids, flavonoids, and tannins at concentrations of 0.21%, 0.0232%, 19.94%, and 10.66%, respectively, with an IC50 value of 135 μg/mL. The aloe vera extract comprises saponins, alkaloids, flavonoids, and tannins at concentrations of 0.74%, 0.0313%, 0.99%, and 4.68%, respectively, with an IC50 value of 4614 μg/mL.

Conclusion

Avocado seeds exhibited elevated levels of flavonoids and tannins, while aloe vera demonstrated increased concentrations of alkaloids and saponins. In the antioxidant activity assessment, avocado seeds demonstrated superior antioxidant efficacy.

Keywords

Antioxidant, Flavonoid, Aloe vera, Avocado seed, Quantitative phytochemistry

Corresponding author: Nur Ariska Nugrahani

Competing interests: No competing interests were disclosed.

Grant information: The author(s) declared that no grants were involved in supporting this work.

Copyright: © 2025 Nugrahani NA et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

How to cite: Nugrahani NA, Anggraeni CNY, Widyastuti NH and Kholifa M. Analyzing Aloe vera and Avocado Seed Extracts for Antioxidants, Saponins, Tannins, Flavonoids, and Alkaloids Using the UV-VIS Spectrophotometric Method [version 1; peer review: 2 approved with reservations]. F1000Research 2025, 14:36 (https://doi.org/10.12688/f1000research.157091.1) First published: 06 Jan 2025, 14:36 (https://doi.org/10.12688/f1000research.157091.1) Latest published: 06 Jan 2025, 14:36 (https://doi.org/10.12688/f1000research.157091.1)

Introduction

Indonesia is a tropical country with a diverse range of plants, particularly land plants. As many as 22,500 species have been recorded, around 1000 plants can be used as medicine,¹ such as avocado seeds and Aloe vera, which have long been known as plants believed to have high efficacy and lower side effects.^2,3 Avocado seeds and aloe vera have the potential to be raw materials for medicines without chemical content, food raw materials, beverage raw materials, cosmetics, and pharmaceutical industries. Avocado seeds can be analgesic and anti-inflammatory in dentistry and can be used as a gel for canker sores. In contrast, Aloe vera has been used in dentistry to help heal wounds, reduce inflammation, and relieve pain.³

Avocado seeds and Aloe vera have the same type of secondary metabolite compounds, namely tannins, Saponins, Flavonoids, and Alkaloids.^2,4 Tannins exhibit antioxidant, astringent, anti-diarrheal, and antibacterials.⁵ Flavonoids are the most abundant compounds found to have antioxidant and anti-inflammatory substances.⁶ The content of different compounds, namely saponins, has the potential to have antibacterial, antioxidant, anticancer, and anti-diabetics.⁷ The last compound is an alkaloid with antibacterial, anti-inflammatory, and antioxidants.⁸ Both materials’ secondary metabolite levels were determined using quantitative phytochemical tests.

Quantitative phytochemical analyses ascertain the quantities of secondary metabolites.⁹ The ethanol extract of avocado seeds has 0.435% alkaloids, 0.1084% flavonoids, 0.0309% phenols, and 0.2044% tannins, as determined using a spectrophotometer.¹⁰ A separate investigation employing UV-Vis spectrophotometry determined that avocado seed extract has 56.5063 μg/ml of alkaloids, 245.6875 μg/ml of flavonoids, 15.65 μg/ml of phenols, 27.03 μg/ml of tannins, and 22.73 μg/ml of saponins.¹¹ Aloe vera extract analyzed via UV-Vis spectrophotometry revealed concentrations of 4.65 ± 0.08 tannins, 1.43 ± 0.031 flavonoids, 60.85 ± 0.61 saponins, and 22.86 ± 0.15 alkaloids.¹² Aloe vera extract (100 g) had 31.067 g of alkaloids, 25.66 g of tannins, and 10.67 g of saponins. The ethanol extract of avocado seed showed a moderate antioxidant capacity (IC50 77.298 μg/mL). Still, the ethanol extract of Aloe vera displayed 70.7% antioxidant activity as assessed by the DPPH technique using a UV-Vis spectrophotometer.¹³ These compounds demonstrate considerable antioxidant capabilities, particularly tannins and flavonoids, which correlate with elevated antioxidant levels.¹⁴ The ethanol extract of avocado seeds had a moderate antioxidant capacity (IC50 77.298 μg/mL),¹⁵ but the ethanol extract of Aloe vera displayed 70.7% antioxidant activity as assessed by the DPPH technique.¹⁶

This study will investigate the extraction of avocado and aloe vera seeds by the maceration method utilizing 70% ethanol for 48 hours, distinguishing it from prior studies. This study compares quantitative phytochemical analyses using a UV-VIS spectrophotometer with antioxidant assessments employing the 2,2-Diphenyl-1-picrylhydrazyl (DPPH) method, also utilizing a UV-VIS spectrophotometer to ascertain the antioxidant activity and IC50 values in avocado seed extract and Aloe vera extract, thereby evaluating the compound levels and antioxidant activity in both extracts.

Methods

Ethics statement

Ethics clearance certificate number: 2.057/XI/HREC/2023. This in vitro study will be conducted at the Integrated Laboratory UPT Universitas Gadjah Mada Yogyakarta (Integrated Research and Testing Laboratory) for phytochemical and antioxidant testing and the Plant Systematics Laboratory of the Faculty of Biology UGM for determination purposes.

Plant determination (materials)

The avocado seeds used were taken from a resident garden in Kepurun Village, Manisrenggo, Klaten. The Aloe vera was taken from a resident’s garden on Kalimantan Street, Purwosari Sinduadi, Mlati District, Sleman. The determination was made at the Plant Systematics Laboratory, Faculty of Biology, UGM, using certificate number 00569/S. Tb.//II/2024 for Aloe vera, and 00568/S. Tb./II/2024 for the avocado seeds.

Extraction of Avocado seed and Aloe vera

Avocado and Aloe vera seeds were washed, cleaned, air-dried, ground into powdered simplicia by grinding, and then sieved. The simplicity of both ingredients was then extracted using the maceration technique. Maceration was performed by soaking the simplicia in 70% ethanol solvent (1:10) for 2 × 24 h with occasional stirring. The filtered filtrate was concentrated using a rotary evaporator.

Phytochemical quantitative test

1. Saponin test

A standard curve was established using a saponin scale of 10 mg of sample, specifically avocado seed extract and aloe vera extract, adding 5 ml of water to each extract. The mixture was vortexed for 5 minutes and added 50 μL of anisaldehyde. It was then shaken and allowed to stand for 10 minutes. Introduce 2 ml of 50% sulfuric acid and subject the mixture to heating in a water bath at 60 °C for 10 minutes. Water was added to a 10 ml volume in a measuring flask, with the standard concentrations beginning at 200, 100, 50, 25, 12.5, and 6.25 μl. Absorbance was measured at a wavelength of 435 nm.

To quantify total saponins, avocado seed extract and aloe vera extract samples were weighed to approximately 100 mg. Introduce 2 ml of 25% H₂SO₄, subject to autoclaving for 120 minutes at a temperature of 110 °C, followed by extraction with ether and subsequent drying of the filtrate. Add 1 ml of water and extract by vortexing for 5 minutes. Introduce 50 μL of anisaldehyde, mix thoroughly, and allow to stand for 10 minutes. Introduce 2 ml of 50% sulfuric acid and subject the mixture to heating in a water bath at 60 °C for 10 minutes. Ten milliliters of water were diluted using a volumetric flask, and the absorbance was measured at a wavelength of 435 nm.

2. Alkaloid test

A meticulous weighing of 10 milligrams of quinine standard and 5 milliliters of 2N hydrochloric acid produced the standard curve. The solution was passed through a separating funnel thrice with 10 mL of chloroform each time, and the chloroform phase was then discarded. 0.1 N NaOH was added to the mixture. Put in 5 ml of BCG Solution and 5 ml of Phosphate Buffer. Following 15 minutes of magnetic stirring at 500 rpm, 5 mL of chloroform was added to the solution for extraction. In two separate instances, chloroform was used for the extraction. The chloroform phase was removed by evaporation using nitrogen gas, and then 10 mL of chloroform was added. Dissolve and peruse The absorbance was assessed at a 470 nm wavelength.

The sample was measured to within ±100 mg to determine the total alkaloids. Then, 5 mL of 2N HCl was added and mixed with a shake. The mixture was then rinsed three times with 10 mL of Chloroform in a separating funnel. After removing the chloroform phase, the solution was acidified with 0.1 N NaOH. Put in 5 ml of BCG Solution and 5 ml of Phosphate Buffer. After 5 ml of chloroform was added to the solution, it was swirled magnetically at 500 revolutions per minute for 15 minutes. In two separate instances, chloroform was used for the extraction. A volume of 5 mL of chloroform was added after the chloroform phase had been recovered and evaporated using nitrogen gas. The absorbance was assessed at a 470 nm wavelength.

3. Flavonoid test

A quercetin standard (10.0 mg) and 0.3 ml of 5% sodium nitrite were utilized to construct the standard curve. Subsequently, 0.6 ml of 10% aluminum chloride was added after 5 minutes and allowed to stand for another 5 minutes. Subsequently, 2 ml of 1 M sodium hydroxide was introduced. About 10 ml of distilled water was introduced into the measuring flask. The solution was placed in a cuvette, and absorbance was measured at a wavelength of 510 nm.

Fifty milligrams of the sample were precisely measured to determine total flavonoids, followed by adding 0.3 milliliters of 5% sodium nitrite. After 5 minutes, 0.6 ml of 10% aluminum chloride was added and allowed to stand for another 5 minutes, followed by 2 ml of 1 M sodium hydroxide. Distilled water was added to a volume of up to 10 ml using the measuring flask and diluted as necessary. The solution was placed in a cuvette, and the absorbance was recorded at a wavelength of 510 nm.

4. Tannin test

The Tannic Acid standard was accurately weighed to construct the standard curve. Subsequently, 10 mL of Folin Ciocalteu reagent was added, vortexed, and allowed to stand for 5 minutes. Prepare a 20% Sodium Carbonate solution and adjust the final volume to 100 mL. Following a 30-minute incubation at room temperature, absorbance was assessed at 760 nm.

The sample was weighed to an accuracy of ±100 mg to assess the total tannin content. Perform extraction using 10 mL of diethyl ether for 20 hours, followed by filtration. The residual diethyl ether was evaporated, and distilled water was added to the sample to achieve a final volume of 10 mL. Measure 1 mL of the sample solution, incorporate 0.1 mL of Folin Ciocalteu reagent, vortex the mixture, and allow it to stand for 5 minutes. Introduce 2 mL of 20% Sodium Carbonate, vortex the solution, and allow it to stand for 5 minutes. Aquadest was introduced into a 10 ml volume and subsequently diluted by a factor of 10. Following a 30-minute incubation at room temperature, the absorbance was recorded at 760 nm.

5. To obtain a linear regression equation and correlation coefficient, The absorbance results were used to create a standard curve (flavonoids, tannins, alkaloids, and saponins). A regression equation was employed to compute the chemical content utilizing the subsequent formula:
$Total compound (% b / b) = \frac{Reading result (ppm) \times Solution Vol . add (ml) \times fp}{Sample Weight (g)} : 10000$
6. Antioxidant test

A stock solution was made by weighing 500 mg of the extract and diluting it in 20 mL of 70% ethanol. The mixture was transferred to a 50 mL volumetric flask, ethanol was poured to the mark, and subjected to ultrasonic treatment for 10 minutes. The solution was filtered until a transparent filtrate was acquired. The stock solution underwent dilution. Prepare a 0.4 mM DPPH solution using 15.7 mg of DPPH and ethanol (96%) to the mark in a 100 mL volumetric flask. The solution underwent ultrasonication for 5 minutes until DPPH was fully dissolved. A sample including 50 μL of extract, 1.0 mL of 0.4 mM DPPH, and 3,950 mL of ethanol was vortexed in a microplate and incubated for 30 minutes in a dark environment. Absorbance was quantified at a wavelength of 515 nm. Development of standard curves and linear regression formulae. The antioxidant activity was determined using the subsequent formula:

% Antioxidant : \frac{Abs . Control - Abs . Sample}{Abs . Control} \times 100 %

The IC50 value was determined utilizing the formula: (x) IC50 = (50 – b): a (a = intersep; b: koefisiensi beta).

Results

Quantitative measurement of saponins was conducted utilizing Quillaja bark standards at a wavelength of 435 nm, with the linear equation Y = 9.44528e-0.44x - 0.00332132 and a correlation coefficient (r²) of 0.99974 ( Figure 1). The subsequent equation was employed to ascertain the concentrations of saponin components, whereas the r-value indicates the correlation between the concentration of the standard solution and the absorbance. An r value around 1 is considered favorable as it implies a direct proportionality or linearity between the concentration of the standard solution and the absorbance. The overall saponin test findings indicated that the average saponin content in Aloe vera extract surpassed that of avocado seeds. The findings revealed that the mean saponin concentration in the Aloe vera extract sample was 0.74%, whereas that of the avocado seed extract was 0.21%.

Figure 1. Curve of Saponin.

The quantitative measurement of alkaloids was conducted utilizing the Quillaja bark standard at a wavelength of 470 nm, with the linear equation Y = 0.00154627x - 0.00434169 and a correlation coefficient (r²) of 0.99913 ( Figure 2). The overall alkaloid test findings indicated that the average alkaloid level in Aloe vera extract surpassed that of avocado seeds. The findings revealed that the mean concentration in avocado seeds was 0.0232%, whereas that in Aloe vera was 0.0313%.

Figure 2. Curve of Alkaloid.

The quantitative analysis of flavonoids was conducted utilizing the quercetin standard at a wavelength of 510 nm, resulting in a linear equation of Y = 0.00569497 x - 0.00473317, with a correlation coefficient (r²) of 0.99979 ( Figure 3). The total flavonoid test results indicated that the average flavonoid content in Aloe vera extract was lower than in avocado seeds. The observation results revealed that the average content of avocado seeds was 19.44%, while in Aloe vera, it was 0.99%.

Figure 3. Curve of Flavonoid.

The quantitative analysis of tannin was conducted utilizing the Tannin Acid standard at a wavelength of 760 nm, with a linear equation represented as Y = 0.019469x + 9.88071e-004, and a correlation coefficient (r²) of 0.99994 ( Figure 4). The total tannin test results on avocado and Aloe vera seeds indicated that the average tannin content in Aloe vera extract was less than that found in avocado seeds. The observation results revealed that the average content of avocado seed extract was 10.66%, while Aloe vera extract was measured at 4.68%.

Figure 4. Curve of Tanin.

The test results for Aloe vera extract samples ( Figure 5) indicated an IC50 value of 4614 μg/mL, categorizing it as inactive. Examinations of avocado seeds ( Figure 6) revealed an IC50 value of 135 μg/mL, categorizing it as moderate.

Figure 5. Antioxidant from Aloe vera.

Figure 6. Antioxidant from Avocado seed.

Discussion

The saponin concentration in A. vera surpasses that of avocado seeds, as the highest levels of saponin in plants are located in the fruit and leaves, particularly in mature leaves^17,18; this aligns with prior research indicating that saponin synthesis transpires in the leaves.¹⁹ Saponin demonstrates foaming properties upon interaction with water.¹⁹ The composition and concentration of saponins are significantly affected by environmental conditions and extraction methods.^20–22 Saponins work by exhibiting antibacterial action through the denaturation of proteins. The active compound saponin, akin to a detergent, can diminish the surface tension of bacterial cell walls, hence compromising the permeability of the bacterial membrane.²³

Aloe vera extract contained more alkaloid compounds. Plant type can also influence the difference, and environmental factors such as soil pH approaching neutral (5.79-6.97) can affect alkaloid production. The extraction process also affected the amount of alkaloid compound withdrawal.²⁴ The condition of the planting and maintenance soil is also thought to affect the quality of the avocado and Aloe vera plants used, so soil that uses nitrogen fertilizer can increase the production of Alkaloid.²⁵ Alkaloids have basic properties and contain one or more nitrogen atoms in a cyclic system combination. This compound is likely to be present in small quantities and must be separated from a complex mixture of compounds. The alkaloid compounds were the lowest compared to the other compounds.^26,27 Alkaloid compounds have non-polar properties; therefore, they are less suitable for extraction with polar compounds, such as 70% ethanol. Alkaloids play a role in plant metabolism and control plant development. Most Alkaloid compounds originate from plants, especially Angiospermae.²⁸

Flavonoid content is higher in plants grown in lowlands, which is closely related to temperature and soil nutrient availability.²⁹ The avocado and Aloe vera seeds used in this study were collected from different areas. The avocado seeds used in this study were obtained from lowland plantations with higher soil calcium content. This can affect flavonoid content. The significant difference in flavonoid content was also caused by the fact that the types and varieties of plants used were not uniform. Flavonoids are primary antioxidants that provide hydrogen atoms to the free radicals. The flavonoid levels in plants affect the plant’s antioxidant activity. Flavonoids are polar compounds that can dissolve in polar solvents, such as ethanol, methanol, butanol, acetone, and dimethylformamide. Water-soluble flavonoids are included in the polyphenol family. Flavonoids are also bound to glycosides. Hence, the mixture of the above solvents with water is a suitable solvent for flavonoid glycosides. In contrast, aglycones such as flavones, flavonols, and flavanones are more easily dissolved in chloroform and ether solvents.^30,31

The tannin content in avocado seeds was higher than in aloe vera seeds. Tannin compounds can be found in dicotyledonous plants’ stems, skin, flowers, seeds, leaves, and cell walls or vacuoles. Generally, tannin compounds are more commonly found in dicotyledonous plants or flowering plants with dicotyledonous seeds, especially in angiosperm plants, such as plants with closed seeds, such as avocado seeds. During the maturity phase, fruit seeds experience a significant increase in tannin levels.³² Avocado is a dicotyledonous angiosperm plant that is thought to have a high tannin content, especially in seeds. Simultaneously, Aloe vera is included in monocotyledonous angiospermae plants.^33,34 In addition, tannin has a molecular weight consisting of hydroxyl groups and several other groups, such as carboxyl and complex organic substances, which are difficult to separate and crystallize. Chemically, tannins are divided into condensed and hydrolyzed tannins. The type of tannin commonly found in plants is hydrolyzed tannin, usually marked by a color change from greyish-blue to blackish when given specific reagents. Tannins possess a sour and astringent flavor and create colloids upon dissolution in water. Tannin’s structure comprises two aromatic rings connected by three carbon atoms.^35,36

The antioxidant activity was evaluated utilizing the DPPH assay. rior to evaluating the sample concentrations by UV-Vis spectrophotometry, the DPPH solution was analyzed to ascertain the optimal wavelength, ensuring that the sample sensitivity was maximized at the highest absorbance value. A potent antioxidant possesses an IC50 value under 50 μg/mL, a powerful antioxidant has an IC50 value ranging from 50 to 100 μg/mL, a moderate antioxidant exhibits an IC50 value between 101 and 250 μg/mL, a weak antioxidant shows an IC50 value from 250 to 500 μg/mL, and an inactive antioxidant has an IC50 value exceeding 500 μg/mL.³⁷ The analysis of the DPPH solution indicated an optimal wavelength of 515.5 nm for DPPH. This wavelength was employed to assess the antioxidant activity of the samples. Sample testing was conducted by reacting the test solution with the DPPH solution, followed by a 30-minute incubation in a dark environment. The incubation period is ideal for the DPPH technique, facilitating effective binding between antioxidant molecules and DPPH radicals. The comparator employed in this investigation was Vitamin C. Vitamin C comprises powerful natural antioxidant molecules. Vitamin C serves as a reliable comparator with well-defined features; hence, the vitamin C antioxidant test findings can assist in assessing the quality and efficacy of antioxidant components in the extract under examination.³⁸

The avocado seed extract in this study was tested with three repetitions or taking from the mother liquor and obtained an average percentage inhibition result of 44.12% with an IC50 value of 135 μg/mL, classified as moderate. Aloe vera extract was tested with three repetitions or taken from the mother liquor and obtained an average percentage inhibition result of 40.17% with an IC50 value of 4614 μg/mL, classified as inactive but still has no potential as an antioxidant. The levels or concentrations used in Aloe vera were higher than those in avocado seeds, allowing the IC50 value to be obtained. The requirement for calculating the IC50 value is when there is an intersection between the inhibition value and a level above 50. If both levels are the same, the inhibition value obtained will not be more than 50%; therefore, the IC50 value in Aloe vera cannot be determined at.³⁹

IC50 denotes the concentration of antioxidant chemicals required to neutralize 50% of free radicals. A lower IC50 value indicates greater antioxidant activity.⁴⁰ The difference in results obtained in A. vera and avocado seed extracts can occur due to several factors, such as plant factors themselves, plant quality, planting methods, the environment around the planting, and contamination by other substances. The difference in results between avocado seeds and Aloe vera can be associated with tannins and flavonoids in both extracts. The levels of flavonoids and tannins obtained in avocado seed extract were much higher, at 10.66% and 19.44%, respectively, while in Aloe vera, the flavonoid and tannin contents were only 4.68% and 0.99%, respectively. The difference in the content of these two compounds can affect the antioxidant activity of a plant. Previous studies stated that the phenolic content, such as flavonoids and tannins, strongly influences a plant’s antioxidant activity.⁴¹ The comparison of flavonoid and tannin levels reveals that Aloe vera contains 4.68% tannins and 0.99% flavonoids, whereas avocado seeds exhibit significantly higher concentrations of 10.66% tannins and 19.44% flavonoids. Thus, the levels of both compounds are markedly greater in avocado seeds compared to Aloe vera. Both compounds are significant contributors to antioxidant activity.

Conclusion

The levels of flavonoids and tannins in the ethanol extract of avocado seeds were higher than those in A. vera. The levels of saponin and alkaloid compounds were higher in Aloe vera.

The antioxidant activity of the ethanol extract from avocado seeds exceeded that of Aloe vera. The inhibition percentage in avocado seeds was 44.12%, corresponding to an IC50 value of 135 μg/mL, indicating moderate activity. In contrast, Aloe vera exhibited an inhibition percentage of 40.17% with an IC50 value of 4164 μg/mL, suggesting inactivity.

Ethics and consent

Ethical approval and consent were not required.

Data availability

Extended data

Harvard Dataverse: “Analyzing Aloe vera and Avocado Seed Extracts for Antioxidants, Saponins, Tannins, Flavonoids, and Alkaloids Using the UV-VIS Spectrophotometric Method”, https://doi.org/10.7910/DVN/MQPRDT.

This project contains the following underlying data:

Figure 1 Curve Saponin, Figure 2 Curve of Alkaloid, Figure 3 Curve of Flavonoid, Figure 4 Curve of Tanin, Figure 5 Antioxidant Avocado Seed, Figure 6 Antioxidant Avocado Seed, Result of Antioxidant, Sample for Curve Saponin, Tanin, Flavonoid and Table flavonoid, alkaloid, tanin and saponin.

License: Data is available under the terms of the CC0 1.0 Universal.

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24. Karim A, Adnan J, Irmawati.: Determination of total alkaloid content of purple leaf ethanol extract (Graptophyllum pictum L.) by UV-Vis spectrophotometry method. J Pharm Pelamonia. 2022; 2(2): 42–47.
25. Wei W, Ye C, Huang HC, et al.: Appropriate nitrogen application enhances saponin synthesis and growth mediated by optimizing root nutrient uptake ability. J Ginseng Res. 2020; 44(4): 627–636. PubMed Abstract | Publisher Full Text | Free Full Text
26. Dymek A, Widelski J, Wojtanowski KK, et al.: Fractionation of Lycopodiaceae Alkaloids and Evaluation of Their Anticholinesterase and Cytotoxic Activities. Molecules. 2021; 26(21): 6379. PubMed Abstract | Publisher Full Text | Free Full Text
27. Heinrich M, Mah J, Amirkia V: Alkaloids Used as Medicines: Structural Phytochemistry Meets Biodiversity-An Update and Forward Look. Molecules. 2021; 26(7): 1836. PubMed Abstract | Publisher Full Text | Free Full Text
28. Debnath B, Singh WS, Das M, et al.: Role of plant alkaloids on human health: A review of biological activities. Mater Today Chem. 2018; 9: 56–72. Publisher Full Text
29. Mahfur M, Khasanah K, Anindhita MA, et al.: Comparison of the total phenolic and flavonoid contents of Amomum compactum Sol. Ex Maton from districts Linggo Asri and Paninggaran, Pekalongan Regency. Sasambo Journal of Pharmacy. 2023; 4(1): 8–13. Publisher Full Text
30. Yuliani RF, Dewi SK, Asri MT, et al.: Total phenolic and flavonoid contents of Elephantopus scaber and ageratum conyzoides (Asteraceae) leaves extracts from various altitude habitats. Ecol Environ Conserv. 2019; 25(7): S106–S113.
31. Kaur R, Dhanai R, Sharma J, et al.: Studies on the Diversity of Tannins and Dyes Yielding Plants of Kathua District of J and K, India. Environ Ecol. 2023; 41(3): 1425–1431. Publisher Full Text
32. Subba S, Gurung S, Mahato SK, et al.: Introduction of Avocado (Persia Americana) Fruits in Eastern Himalaya of India: A Review. Int J Econ Plants. 2023; 10(2): 127–131. Publisher Full Text
33. Jaiswal SK, Mahajan S, Chakraborty A, et al.: The genome sequence of Aloe vera reveals the adaptive evolution of drought tolerance mechanisms. iScience. 2021; 24(2): 102079. PubMed Abstract | Publisher Full Text | Free Full Text
34. Agustin AD, Purwasih R: Powder Drink of Permesia americana Mill. Seed with Adding Zingiber officinale Rosc. Var Rubrum and Stevia rebaudiana L. To Enhance Cardiovascular Health. Jurnal Ilmu Kefarmasian Indonesia. 2024; 1(2): 1–7.
35. Panche AN, Diwan AD, Chandra SR: Flavonoids: an overview. J Nutr Sci. 2016; 5: e47. PubMed Abstract | Publisher Full Text | Free Full Text
36. Soares S, Brandão E, Guerreiro C, et al.: Tannins in Food: Insights into the Molecular Perception of Astringency and Bitter Taste. Molecules. 2020; 25(11): 2590. PubMed Abstract | Publisher Full Text | Free Full Text
37. Itam A, Wati MS, Agustin V, et al.: Comparative Study of Phytochemical, Antioxidant, and Cytotoxic Activities and Phenolic Content of Syzygium aqueum (Burm. f. Alston f.) Extracts Growing in West Sumatera, Indonesia. Sci World J. 2021; 2021: 5537597.
38. Munteanu IG, Apetrei C: Analytical Methods Used in Determining Antioxidant Activity: A Review. Int J Mol Sci. 2021; 22(7): 3380. PubMed Abstract | Publisher Full Text | Free Full Text
39. Garcia-Molina P, Garcia-Molina F, Teruel-Puche JA, et al.: The Relationship between the IC₅₀ Values and the Apparent Inhibition Constant in the Study of Inhibitors of Tyrosinase Diphenolase Activity Helps Confirm the Mechanism of Inhibition. Molecules. 2022; 27(10): 3141. PubMed Abstract | Publisher Full Text | Free Full Text
40. Lee KJ, Oh YC, Cho WK, et al.: Antioxidant and Anti-Inflammatory Activity Determination of One Hundred Kinds of Pure Chemical Compounds Using Offline and Online Screening HPLC Assay. Evid Based Complement Alternat Med. 2015; 2015: 165457.
41. Savitri ES, Holil K, Resmisari RS: Phytochemistry Screening and Antioxidant Activities of Extract Pomegranate, Grape, Fig, and Olive in Various Solvents. J Biodjati. 2022; 7(1): 132–139. Publisher Full Text

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Author details Author details

¹ Department Oral Biology, Faculty of Dentistry, Universitas Muhammadiyah Surakarta, Surakarta, Central Java, 57141, Indonesia
² Faculty of Dentistry, Universitas Muhammadiyah Surakarta, Surakarta, Central Java, 57141, Indonesia
³ Department of Conservative Dentistry, Universitas Muhammadiyah Surakarta, Surakarta, Central Java, 57141, Indonesia

Nur Ariska Nugrahani
Roles: Conceptualization, Formal Analysis, Investigation, Methodology, Resources, Supervision, Validation, Visualization, Writing – Original Draft Preparation, Writing – Review & Editing

Cecilya Nella Yuppy Anggraeni
Roles: Data Curation, Investigation, Methodology, Validation, Visualization, Writing – Original Draft Preparation

Noor Hafida Widyastuti
Roles: Validation, Visualization

Mahmud Kholifa
Roles: Validation, Visualization

Competing interests

No competing interests were disclosed.

Grant information

The author(s) declared that no grants were involved in supporting this work.

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Nugrahani NA, Anggraeni CNY, Widyastuti NH and Kholifa M. Analyzing Aloe vera and Avocado Seed Extracts for Antioxidants, Saponins, Tannins, Flavonoids, and Alkaloids Using the UV-VIS Spectrophotometric Method [version 1; peer review: 2 approved with reservations]. F1000Research 2025, 14:36 (https://doi.org/10.12688/f1000research.157091.1)

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Reviewer Report 22 Jul 2025

Mona Luciana Gălăţanu, Titu Maiorescu University, Bucharest, Romania

Approved with Reservations

https://doi.org/10.5256/f1000research.172498.r391024

The paper presents a comparative study of phytochemical quantification of the predominant compounds between two plant species, as well as their antioxidant capacity. Few aspects must be clarified:
1. Which organ is used from Aloe vera, as it is ... Continue reading

The paper presents a comparative study of phytochemical quantification of the predominant compounds between two plant species, as well as their antioxidant capacity. Few aspects must be clarified:
1. Which organ is used from Aloe vera, as it is not specified in the text of Plant determination.
2. In the methods, at Saponin test, it is not written which standard substance was used to realize the standard curve.
3. Also, at the Alkaloid test, in Methods, quinine is mentioned as standard, while at Results, Quillaja bark appear to be the standard used. Which one was in fact used for obtaining the calibration curve?
4. In Discussion, it worth to be mentioned that both alkaloids and steroid saponins can determine a high risk of toxicity, that must be assessed through different studies.It is important also, to notice, that avocado seeds have these compounds in smaller doses, which make them safer for consumption.
5. Few typos in the text must be corrected.

Is the work clearly and accurately presented and does it cite the current literature?

Yes
Is the study design appropriate and is the work technically sound?

Partly
Are sufficient details of methods and analysis provided to allow replication by others?

Partly
If applicable, is the statistical analysis and its interpretation appropriate?

Yes
Are all the source data underlying the results available to ensure full reproducibility?

Yes
Are the conclusions drawn adequately supported by the results?

Yes

References

1. Gălăţanu M, Panţuroiu M, Sandulovici R: Flavonoids. 297-318 Publisher Full Text

Competing Interests: No competing interests were disclosed.

Reviewer Expertise: pharmacognosy, taxonomy, analytical chemistry

I confirm that I have read this submission and believe that I have an appropriate level of expertise to confirm that it is of an acceptable scientific standard, however I have significant reservations, as outlined above.

CITE

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5

Reviewer Report 28 Mar 2025

Didi Nurhadi Illian, Department of Pharmacy, Faculty of Mathematics and Natural Sciences, Universitas Syiah Kuala, Banda Aceh, Aceh, Indonesia

Approved with Reservations

https://doi.org/10.5256/f1000research.172498.r356891

This manuscript describes the quantification of the levels of saponins, alkaloids, flavonoids, and tannins from both extracts of avocado seed and aloe vera. In addition, the IC₅₀ values were determined. It is such an interesting manuscript to be reviewed. The ... Continue reading

This manuscript describes the quantification of the levels of saponins, alkaloids, flavonoids, and tannins from both extracts of avocado seed and aloe vera. In addition, the IC₅₀ values were determined. It is such an interesting manuscript to be reviewed. The paper presents some intriguing results, but it requires some modifications for publication acceptance.

Major Points

Please check again for grammatical errors and typos, or consult with a proofreader!

Introduction

Please mention more clear in this section the author's reason for using both samples of avocado seed and aloe vera for this study! The research gap is not so clear and difficult to recognize; please mention it to emphasize a sense of urgency to perform this investigation.

Methods

Please use a common format for all the chemicals and instruments. Also, mention the manufacturer and country in this section!
Sub-section Extraction of Avocado Seed and Aloe Vera:

Please check the sentence structure of "Avocado and aloe vera seeds were washed…" Did you really use aloe vera seeds? Please mention which part of the aloe vera was used in this study!

Sub-section Phytochemical Quantitative Test:

Please check the formula of Total Compound (%b/b); is that “:10000” or “×10000”?

Not a single reference was embedded for all the procedures of this study, from the extraction procedure and phytochemical analysis to the antioxidant activity test. Please mention the references for all methods that the authors used in each procedure!

Results

Figures 5 and 6 are not well presented; what values represent the x and y axes? Please complete and clarify! See Figures 1 to 4!

Discussion

Please add further discussion (in more detail or molecularly) on how the mechanism of action of the secondary metabolite compounds detected in both samples in facilitating the antioxidant activity obtained to strengthen your results! Simplifying, how can they become significant contributors to antioxidant activity?

Is the work clearly and accurately presented and does it cite the current literature?

Partly
Is the study design appropriate and is the work technically sound?

Yes
Are sufficient details of methods and analysis provided to allow replication by others?

Partly
If applicable, is the statistical analysis and its interpretation appropriate?

I cannot comment. A qualified statistician is required.
Are all the source data underlying the results available to ensure full reproducibility?

Partly
Are the conclusions drawn adequately supported by the results?

Yes

Competing Interests: No competing interests were disclosed.

Reviewer Expertise: Pharmacology, Toxicology, Immunology, Cancer Signaling

I confirm that I have read this submission and believe that I have an appropriate level of expertise to confirm that it is of an acceptable scientific standard, however I have significant reservations, as outlined above.

CITE

Report a concern

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Comments on this article Comments (0)

Version 1

VERSION 1 PUBLISHED 06 Jan 2025

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Version 1 06 Jan 25	read	read

Didi Nurhadi Illian, Universitas Syiah Kuala, Banda Aceh, Indonesia
Mona Luciana Gălăţanu, Titu Maiorescu University, Bucharest, Romania

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Reviewer Report

3 Views

22 Jul 2025 | for Version 1

Mona Luciana Gălăţanu, Titu Maiorescu University, Bucharest, Romania

3 Views Cite this report Responses(0)

Approved With Reservations

The paper presents a comparative study of phytochemical quantification of the predominant compounds between two plant species, as well as their antioxidant capacity. Few aspects must be clarified:
1. Which organ is used from Aloe vera, as it is not specified in the text of Plant determination.
2. In the methods, at Saponin test, it is not written which standard substance was used to realize the standard curve.
3. Also, at the Alkaloid test, in Methods, quinine is mentioned as standard, while at Results, Quillaja bark appear to be the standard used. Which one was in fact used for obtaining the calibration curve?
4. In Discussion, it worth to be mentioned that both alkaloids and steroid saponins can determine a high risk of toxicity, that must be assessed through different studies.It is important also, to notice, that avocado seeds have these compounds in smaller doses, which make them safer for consumption.
5. Few typos in the text must be corrected.

Is the work clearly and accurately presented and does it cite the current literature?

Yes
Is the study design appropriate and is the work technically sound?

Partly
Are sufficient details of methods and analysis provided to allow replication by others?

Partly
If applicable, is the statistical analysis and its interpretation appropriate?

Yes
Are all the source data underlying the results available to ensure full reproducibility?

Yes
Are the conclusions drawn adequately supported by the results?

Yes

References

1. Gălăţanu M, Panţuroiu M, Sandulovici R: Flavonoids. 297-318 Publisher Full Text

Competing Interests

No competing interests were disclosed.

Reviewer Expertise

pharmacognosy, taxonomy, analytical chemistry

I confirm that I have read this submission and believe that I have an appropriate level of expertise to confirm that it is of an acceptable scientific standard, however I have significant reservations, as outlined above.

Respond to this report

Responses (0)

Back to all reports

Reviewer Report

5 Views

28 Mar 2025 | for Version 1

Didi Nurhadi Illian, Department of Pharmacy, Faculty of Mathematics and Natural Sciences, Universitas Syiah Kuala, Banda Aceh, Aceh, Indonesia

5 Views Cite this report Responses(0)

Approved With Reservations

This manuscript describes the quantification of the levels of saponins, alkaloids, flavonoids, and tannins from both extracts of avocado seed and aloe vera. In addition, the IC₅₀ values were determined. It is such an interesting manuscript to be reviewed. The paper presents some intriguing results, but it requires some modifications for publication acceptance.

Major Points

Please check again for grammatical errors and typos, or consult with a proofreader!

Introduction

Please mention more clear in this section the author's reason for using both samples of avocado seed and aloe vera for this study! The research gap is not so clear and difficult to recognize; please mention it to emphasize a sense of urgency to perform this investigation.

Methods

Please use a common format for all the chemicals and instruments. Also, mention the manufacturer and country in this section!
Sub-section Extraction of Avocado Seed and Aloe Vera:

Please check the sentence structure of "Avocado and aloe vera seeds were washed…" Did you really use aloe vera seeds? Please mention which part of the aloe vera was used in this study!

Sub-section Phytochemical Quantitative Test:

Please check the formula of Total Compound (%b/b); is that “:10000” or “×10000”?

Not a single reference was embedded for all the procedures of this study, from the extraction procedure and phytochemical analysis to the antioxidant activity test. Please mention the references for all methods that the authors used in each procedure!

Results

Figures 5 and 6 are not well presented; what values represent the x and y axes? Please complete and clarify! See Figures 1 to 4!

Discussion

Please add further discussion (in more detail or molecularly) on how the mechanism of action of the secondary metabolite compounds detected in both samples in facilitating the antioxidant activity obtained to strengthen your results! Simplifying, how can they become significant contributors to antioxidant activity?

Is the work clearly and accurately presented and does it cite the current literature?

Partly
Is the study design appropriate and is the work technically sound?

Yes
Are sufficient details of methods and analysis provided to allow replication by others?

Partly
If applicable, is the statistical analysis and its interpretation appropriate?

I cannot comment. A qualified statistician is required.
Are all the source data underlying the results available to ensure full reproducibility?

Partly
Are the conclusions drawn adequately supported by the results?

Yes

Competing Interests

No competing interests were disclosed.

Reviewer Expertise

Pharmacology, Toxicology, Immunology, Cancer Signaling

I confirm that I have read this submission and believe that I have an appropriate level of expertise to confirm that it is of an acceptable scientific standard, however I have significant reservations, as outlined above.

Respond to this report

Responses (0)

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[2] 2. Yulistina Y, Suwondo A, Santoso B: Potential Nano Gel Avocado Seed Extract as an Alternative Relief in Wounds After Removal of White Rats Tooth. J Res Soc Sci Econ Manag. 2022; 2(1): 14–26.

[3] 3. Katubi KM, Amari A, Harharah HN, et al.: Aloe vera as a promising material for water treatment: A review. Processes. 2021; 9(5): 1–16. Publisher Full Text

[4] 4. Taukoorah U, Mahomoodally MF: Crude Aloe vera Gel Shows Antioxidant Propensities and Inhibits Pancreatic Lipase and Glucose Movement in Vitro. Adv Pharmacol Sci. 2016; 2016: 1–9. PubMed Abstract | Publisher Full Text | Free Full Text

[5] 5. Fraga-Corral M, Otero P, Cassani L, et al.: Traditional applications of tannin-rich extracts, supported by scientific data, include chemical composition, bioavailability, and bioaccessibility. Foods. 2021; 10(2). PubMed Abstract | Publisher Full Text | Free Full Text

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[7] 7. Ravi L, Manasvi V, Praveena Lakshmi B: Antibacterial and antioxidant activity of saponin from Abutilon indicum leaves. Asian J Pharm Clin Res. 2016; 9(1): 344–347. Publisher Full Text

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[9] 9. Mboneye A, Onchweri AN, Neeza T, et al.: Preliminary Phytochemical Screening and Quantitative Analysis of Methanol Leaf Extract of Erlangea tomentosa (Oliv. & Hiern) S. Moore (Asteraceae). J Trop Pharm Chem. 2021; 5(4): 396–405.

[10] 10. Rivai H, Putri YT, Rusdi R: Qualitative and Quantitative Analysis of the Chemical Content of Hexane, Acetone, Ethanol and Water Extract from Avocado Seeds (Persea americana Mill.). Sch Int J Tradit Complement Med Abbreviated Key Title. 2019; 8634: 25–31.

[11] 11. Sunday CU, Ndidiamaka HO, Ugochukwu DD, et al.: Phytochemical Analysis and Antioxidant Activity of Avocado Pear Peel (Persea americana) Extract. J Pharm Res Int. 2022; 34: 22–29. Publisher Full Text

[12] 12. Ibe C: Evaluation of the Antioxidant Activities of Psidium guajava and Aloe vera. Br J Pharm Res. 2014; 4(3): 397–406. Publisher Full Text

[13] 13. Nalado YA, Tijjani A: Qualitative and Quantitative Phytochemical Analysis of Aloe barbadensis Miller Leaf Extracts. UMYU Sci. 2023; 2(1): 24–30.

[14] 14. Antasionasti I, Datu OS, Lestari US, et al.: Correlation Analysis of Antioxidant Activities with Tannin, Total Flavonoid, and Total Phenolic Contents of Nutmeg (Myristica fragrans Houtt) Fruit Precipitated by Egg white. Borneo J Pharm. 2021; 4(4): 301–310. Publisher Full Text

[15] 15. Munthe WN, Riskianto R, Juvi D, et al.: Antioxidant, Total Phenolic, and Total Flavonoid of 70% Ethanol Extract of Avocado Seeds (Persea americana Mill.). Pharm J. 2023; 15(4): 599–605.

[16] 16. Hęś M, Dziedzic K, Górecka D, et al.: Aloe vera (L.) Webb.: Natural Sources of Antioxidants – A Review. Plant Foods Hum Nutr. 2019; 74(3): 255–265. PubMed Abstract | Publisher Full Text | Free Full Text

[17] 17. Ode Nanang Trisna Dewi W, Dewi F, Ardiansyah A, et al.: Analysis Of Saponin Content in Ruruhi Plant (Syzygium polycephalum Merr) in Kendari City, Southeast Sulawesi. Int J Sci Environ. 2023; 3(1): 21–24. Publisher Full Text

[18] 18. da Silva GG , Pimenta LPS, Melo JOF, et al.: Phytochemicals of Avocado Residues as Potential Acetylcholinesterase Inhibitors, Antioxidants, and Neuroprotective Agents. Molecules. 2022; 27(6): 1892. PubMed Abstract | Publisher Full Text | Free Full Text

[19] 19. Arsene MMJ, Viktorovna PI, Sergei GV, et al.: Phytochemical Analysis, Antibacterial and Antibiofilm Activities of Aloe vera Aqueous Extract against Selected Resistant Gram-Negative Bacteria Involved in Urinary Tract Infections. Fermentation. 2022; 8(11): 626. Publisher Full Text

[20] 20. Nolalita AH, Karyadi NP, Santoso SA, et al.: Effectiveness of Avocado Seed Extract on the Detergent Production Process. Journal of Vocational Studies on Applied Research. 2024; 6(1): 21–24.

[21] 21. Setyawan HY, Sukardi S, Puriwangi CA: Phytochemicals properties of avocado seed: A review. IOP Conf Ser Earth Environ Sci. 2021; 733(1): 012090. Publisher Full Text

[22] 22. Rai S, Acharya-Siwakoti E, Kafle A, et al.: Plant-Derived Saponins: A Review of Their Surfactant Properties and Applications. Sci. 2021; 3(4): 1–19. Publisher Full Text

[23] 23. Tatli Cankaya II, Somuncuoglu EI: Potential and Prophylactic Use of Plants Containing Saponin-Type Compounds as Antibiofilm Agents against Respiratory Tract Infections. Evid. Based Complement. Alternat. Med. 2021; 2021: 6814215.

[24] 24. Karim A, Adnan J, Irmawati.: Determination of total alkaloid content of purple leaf ethanol extract (Graptophyllum pictum L.) by UV-Vis spectrophotometry method. J Pharm Pelamonia. 2022; 2(2): 42–47.

[25] 25. Wei W, Ye C, Huang HC, et al.: Appropriate nitrogen application enhances saponin synthesis and growth mediated by optimizing root nutrient uptake ability. J Ginseng Res. 2020; 44(4): 627–636. PubMed Abstract | Publisher Full Text | Free Full Text

[26] 26. Dymek A, Widelski J, Wojtanowski KK, et al.: Fractionation of Lycopodiaceae Alkaloids and Evaluation of Their Anticholinesterase and Cytotoxic Activities. Molecules. 2021; 26(21): 6379. PubMed Abstract | Publisher Full Text | Free Full Text

[27] 27. Heinrich M, Mah J, Amirkia V: Alkaloids Used as Medicines: Structural Phytochemistry Meets Biodiversity-An Update and Forward Look. Molecules. 2021; 26(7): 1836. PubMed Abstract | Publisher Full Text | Free Full Text

[28] 28. Debnath B, Singh WS, Das M, et al.: Role of plant alkaloids on human health: A review of biological activities. Mater Today Chem. 2018; 9: 56–72. Publisher Full Text

[29] 29. Mahfur M, Khasanah K, Anindhita MA, et al.: Comparison of the total phenolic and flavonoid contents of Amomum compactum Sol. Ex Maton from districts Linggo Asri and Paninggaran, Pekalongan Regency. Sasambo Journal of Pharmacy. 2023; 4(1): 8–13. Publisher Full Text

[30] 30. Yuliani RF, Dewi SK, Asri MT, et al.: Total phenolic and flavonoid contents of Elephantopus scaber and ageratum conyzoides (Asteraceae) leaves extracts from various altitude habitats. Ecol Environ Conserv. 2019; 25(7): S106–S113.

[31] 31. Kaur R, Dhanai R, Sharma J, et al.: Studies on the Diversity of Tannins and Dyes Yielding Plants of Kathua District of J and K, India. Environ Ecol. 2023; 41(3): 1425–1431. Publisher Full Text

[32] 32. Subba S, Gurung S, Mahato SK, et al.: Introduction of Avocado (Persia Americana) Fruits in Eastern Himalaya of India: A Review. Int J Econ Plants. 2023; 10(2): 127–131. Publisher Full Text

[33] 33. Jaiswal SK, Mahajan S, Chakraborty A, et al.: The genome sequence of Aloe vera reveals the adaptive evolution of drought tolerance mechanisms. iScience. 2021; 24(2): 102079. PubMed Abstract | Publisher Full Text | Free Full Text

[34] 34. Agustin AD, Purwasih R: Powder Drink of Permesia americana Mill. Seed with Adding Zingiber officinale Rosc. Var Rubrum and Stevia rebaudiana L. To Enhance Cardiovascular Health. Jurnal Ilmu Kefarmasian Indonesia. 2024; 1(2): 1–7.

[35] 35. Panche AN, Diwan AD, Chandra SR: Flavonoids: an overview. J Nutr Sci. 2016; 5: e47. PubMed Abstract | Publisher Full Text | Free Full Text

[36] 36. Soares S, Brandão E, Guerreiro C, et al.: Tannins in Food: Insights into the Molecular Perception of Astringency and Bitter Taste. Molecules. 2020; 25(11): 2590. PubMed Abstract | Publisher Full Text | Free Full Text

[37] 37. Itam A, Wati MS, Agustin V, et al.: Comparative Study of Phytochemical, Antioxidant, and Cytotoxic Activities and Phenolic Content of Syzygium aqueum (Burm. f. Alston f.) Extracts Growing in West Sumatera, Indonesia. Sci World J. 2021; 2021: 5537597.

[38] 38. Munteanu IG, Apetrei C: Analytical Methods Used in Determining Antioxidant Activity: A Review. Int J Mol Sci. 2021; 22(7): 3380. PubMed Abstract | Publisher Full Text | Free Full Text

[39] 39. Garcia-Molina P, Garcia-Molina F, Teruel-Puche JA, et al.: The Relationship between the IC₅₀ Values and the Apparent Inhibition Constant in the Study of Inhibitors of Tyrosinase Diphenolase Activity Helps Confirm the Mechanism of Inhibition. Molecules. 2022; 27(10): 3141. PubMed Abstract | Publisher Full Text | Free Full Text

[40] 40. Lee KJ, Oh YC, Cho WK, et al.: Antioxidant and Anti-Inflammatory Activity Determination of One Hundred Kinds of Pure Chemical Compounds Using Offline and Online Screening HPLC Assay. Evid Based Complement Alternat Med. 2015; 2015: 165457.

[41] 41. Savitri ES, Holil K, Resmisari RS: Phytochemistry Screening and Antioxidant Activities of Extract Pomegranate, Grape, Fig, and Olive in Various Solvents. J Biodjati. 2022; 7(1): 132–139. Publisher Full Text

Analyzing Aloe vera and Avocado Seed Extracts for Antioxidants, Saponins, Tannins, Flavonoids, and Alkaloids Using the UV-VIS Spectrophotometric Method

Abstract

Background

Methods

Results

Conclusion

Keywords

Introduction

Methods

Ethics statement

Plant determination (materials)

Extraction of Avocado seed and Aloe vera

Phytochemical quantitative test

Results

Figure 1. Curve of Saponin.

Figure 2. Curve of Alkaloid.

Figure 3. Curve of Flavonoid.

Figure 4. Curve of Tanin.

Figure 5. Antioxidant from Aloe vera.

Figure 6. Antioxidant from Avocado seed.

Discussion

Conclusion

Ethics and consent

Data availability

Extended data

References

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