| Literature DB >> 34281099 |
Shaeesta Khaleelahmed Bhavikatti1,2, Mohmed Isaqali Karobari3,4, Siti Lailatul Akmar Zainuddin1, Anand Marya5,6, Sameer J Nadaf7, Vijay J Sawant8, Sandeep B Patil9, Adith Venugopal6, Pietro Messina10, Giuseppe Alessandro Scardina10.
Abstract
Background-chlorhexidine (CHX) is most commonly used as a chemical plaque control agent. Nevertheless, its adverse effects, including teeth discoloration, taste alteration and calculus build-up, limit its use and divert us to medicinal herbs. The purpose of the study was to evaluate the phytochemical composition, antioxidant potential, and cytotoxic effects of Mimusops elengi Linn extract (ME) over normal human cultured adult gingival fibroblasts (HGFs). Methods-in vitro phytochemical screening, total flavonoid content, antioxidant potential by DPPH and Nitric Oxide (NO) radical scavenging activity, and cytotoxic effects of ME extracts over HGF were explored. The viability of HGF cells was determined using 3-(4,5-dimethylthiazol-2-yl)-2, 5-diphenyl tetrazolium bromide (MTT), neutral red uptake, and trypan blue assay after treatment with different concentrations of CHX and ME (0.3125 to 10 µg/mL). Results-ME showed some alkaloids, glycosides, saponins and flavonoids exhibited relatively moderate-to-good antioxidant potential. Increasing the concentration of CHX and ME from 0.3125 to 10 µg/mL reduced cell viability from 29.71% to 1.07% and 96.12% to 56.02%, respectively. At higher concentrations, CHX reduced the viability of cells by 52.36-fold compared to ME, revealed by MTT assay. At 10 µg/mL concentration, the mean cell viability of CHX and ME-treated cells was 2.24% and 57.45%, respectively, revealed by a neutral red assay. The viability of CHX- and ME-treated HGF cells estimated at higher concentrations (10 µg/mL) using trypan blue assay was found to be 2.18% and 47.36%, respectively. A paired t-test showed significance (p < 0.05), and one-way ANOVA difference between the mean cell viability of CHX- and ME-treated cells at different concentrations. One-way ANOVA confirmed the significant difference between the viability of CHX- and ME-treated cells. Conclusions-The cytoprotective and antioxidant effects of ME emphasize its potential benefits. Therefore, it could emerge as a herbal alternative and adjunct to conventional oral hygiene methods, that can diminish periodontal tissue destruction.Entities:
Keywords: chlorhexidine; cytotoxicity; fibroblast; gingival; herbs; medicinal
Year: 2021 PMID: 34281099 PMCID: PMC8297240 DOI: 10.3390/ijerph18137162
Source DB: PubMed Journal: Int J Environ Res Public Health ISSN: 1660-4601 Impact factor: 3.390
Active ingredients in the ME as evaluated.
| Chemical Constituents | Name of Test | Observed Changes | Result |
|---|---|---|---|
| Alkaloids | Mayer’s Reagent | White-colored turbidity | + |
| Wagner’s Reagent | Reddish Brown Precipitate | + | |
| Hager’s Reagent | Yellow Precipitate floating | + | |
| Ehrlich’s Reagent | Two separate yellow and brown colored layers | + | |
| Sterols &Triterpenoids | Salkowaski test | The lower layer turns red | + |
| Sulphur test | Sinks in it | + | |
| Glycosides | Baljet’s test | Yellow to orange color. | + |
| Keller killani test | No Separation between two layers, lower layer reddish-brown and upper layer turns bluish-green | + | |
| Anthraquinone glycosides | Borntrager’s test | The ammonical layer turns pink or red. | + |
| Saponins | Foam test | Formation of foam | + |
| Carbohydrates | Molisch’s test: | ND | |
| Barfoed’s test | ND | ||
| Benedict’s test | Reddish-brown precipitate | + | |
| Flavonoids | Shinoda test | Pink to magenta-red color | + |
| Alkaline reagent test | Yellow color becomes a color lesson | + | |
| Lead acetate solution test | Yellow precipitate | + | |
| Tannins | Ferric-chloride test | Dark color | + |
| Proteins | Millon’s test | ND | |
| Xanthoproteic test | No Yellow precipitate | _ | |
| Biuret test | No Blue color | _ | |
| Ninhydrin test | No Blue color. | _ |
Note: +, indicates the presence of phytoconstituents; _, indicates an absence of phytoconstituents; ND, indicates not determined.
Figure 1Calibration curve of Quercetin.
Antioxidant activities of Mimusops elengi Linn extract (DPPH and NO assays).
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| 0.34 | |
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| 0.04 | 88.23 |
| 200 µg/mL | 0.14 | 58.82 |
| 400 µg/mL | 0.10 | 70.58 |
| 600 µg/mL | 0.08 | 76.47 |
| 800 µg/mL | 0.07 | 79.41 |
| 1000 µg/mL | 0.05 | 85.29 |
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| 1.64 | |
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| 0.28 | 82.92 |
| 200 µg/mL | 1.49 | 08.87 |
| 400 µg/mL | 1.25 | 23.78 |
| 600 µg/mL | 1.00 | 39.02 |
| 800 µg/mL | 0.77 | 53.04 |
| 1000 µg/mL | 0.74 | 54.87 |
Figure 2Viability study of (A,D,G)—negative control; (B,E,H)—CHX treated; and (C,F,I)—ME-treated cells using MTT assay (A–C), Neutral red uptake assay (D–F) and Trypan blue assay (G–I), respectively.
Cell viability of Primary Gingival Fibroblasts determined using MTT, neutral red, and Trypan blue assay.
| Mean Cell Viability % (Primary Gingival Fibroblast) | ||||||
|---|---|---|---|---|---|---|
| Concentration (µg/mL) | MTT Assay | Neutral Red Assay | Trypan Blue Assay | |||
| CHX | ME | CHX | ME | CHX | ME | |
| 10 | 1.07 | 56.02 | 2.24 | 57.45 | 2.18 | 47.36 |
| 5 | 5.94 | 65.40 | 6.31 | 66.00 | 4.58 | 58.46 |
| 2.5 | 11.11 | 75.87 | 12.63 | 76.54 | 13.01 | 73.08 |
| 1.25 | 17.12 | 84.94 | 18.24 | 87.42 | 18.60 | 80.45 |
| 0.625 | 24.69 | 92.94 | 30.50 | 93.68 | 21.21 | 86.99 |
| 0.3125 | 29.71 | 96.12 | 33.64 | 97.46 | 25.58 | 92.64 |
| Negative Control | 100 | 100 | 100 | |||
Descriptive ANOVA statistics.
| Source | Sum of Squares ss | Degrees of Freedom | Mean Squarems | F Statistic | |
|---|---|---|---|---|---|
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| Treatment | 12,138.0602 | 1 | 12,138.0602 | 65.5995 | ** 0.000011 |
| Error | 1850.3285 | 10 | 185.0328 | ||
| Total | 13,988.3887 | 11 | |||
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| Treatment | 11,718.1250 | 1 | 11,718.1250 | 56.4817 | ** 0.00002 |
| Error | 2074.6763 | 10 | 207.4676 | ||
| Total | 13,792.8013 | 11 | |||
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| Treatment | 1941.7979 | 1 | 10,432.4244 | 53.7256 | ** 0.000025 |
| Error | 12,374.2223 | 10 | 194.1798 | ||
| Total | 1941.7979 | 11 | |||
** indicated statistical significance.
Descriptive statistics of multiple comparisons using a statistical test.
| Post-hoc Tukey HSD Test | ||||||
|---|---|---|---|---|---|---|
| Assay | Treatments | Tukey HSD | Tukey HSD | Tukey HSD inference | ||
| MTT | CHX vs. ME | 11.4542 | 0.0010053 | ** | ||
| NR | 10.6284 | 0.0010053 | ** | |||
| TB | 10.3659 | 0.0010053 | ** | |||
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| Assay | Treatments | Scheffé | Scheffé | Scheffé | ||
| MTT | CHX vs. ME | 8.0994 | 1.0567 × 10−5 | ** | ||
| NR | 7.5154 | 2.0266 × 10−5 | ** | |||
| TB | 7.3298 | 2.5123 × 10−5 | ** | |||
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| Assay | Treatments | Bonferroni | Bonferroni | Bonferroni | Holm | Holm |
| MTT | CHX vs. ME | 8.0994 | 1.0567 × 10−5 | ** | 1.0567 × 10−5 | ** |
| NR | 7.5154 | 2.0266 × 10−5 | ** | 2.0266 × 10−5 | ** | |
| TB | 7.3298 | 2.5123 × 10−5 | ** | 2.5123 × 10−5 | ** | |
NR: Neutral red; TB: Trypan Blue. ** indicate significant results.
Descriptive statistics of ANOVA considering the comparison of viability CHK- and PH-treated HGF cells estimated using a different assay.
| Description | Source | Sum of Squares ss | Degrees of Freedom | Mean Squarems | F Statistic | |
|---|---|---|---|---|---|---|
| ME treated cells | treatment | 147.9926 | 2 | 73.9963 | 0.2766 | * 0.7622 |
| error | 4013.1105 | 15 | 267.5407 | |||
| total | 4161.1030 | 17 | ||||
| CHX treated cells | treatment | 30.6475 | 2 | 15.3237 | 0.1240 | * 0.8843 |
| error | 1853.8300 | 15 | 123.5887 | |||
| total | 1884.4775 | 17 |
* indicates non-significant results.
Descriptive statistics demonstrating comparisons of viability results obtained using different assays.
| Post-hoc Tukey HSD Test | |||||
|---|---|---|---|---|---|
| Treatment pairs | Tukey HSD | Tukey HSD | Tukey HSD inference | ||
| ME treated cells | |||||
| A vs. B | 0.1812 | 0.8999947 | insignificant | ||
| A vs. C | 0.8067 | 0.8266214 | insignificant | ||
| B vs. C | 0.9879 | 0.7545422 | insignificant | ||
| CHX treated cells | |||||
| A vs. B | 0.5112 | 0.8999947 | insignificant | ||
| A vs. C | 0.1639 | 0.8999947 | insignificant | ||
| B vs. C | 0.6751 | 0.8789620 | insignificant | ||
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| Treatments pair | Scheffé TT-statistic | Scheffé | Scheffé inference | ||
| ME treated cells | |||||
| A vs. B | 0.1281 | 0.9918294 | insignificant | ||
| A vs. C | 0.5704 | 0.8513402 | insignificant | ||
| B vs. C | 0.6985 | 0.7865543 | insignificant | ||
| CHX treated cells | |||||
| A vs. B | 0.3615 | 0.9370267 | insignificant | ||
| A vs. C | 0.1159 | 0.9933079 | insignificant | ||
| B vs. C | 0.4774 | 0.8930757 | insignificant | ||
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| Treatments pair | Bonferroni and Holm TT-statistic | Bonferroni | Bonferroni inference | Holm | Holm inference |
| ME treated cells | |||||
| A vs. B | 0.1281 | 2.6992443 | insignificant | 0.8997481 | insignificant |
| A vs. C | 0.5704 | 1.7305385 | insignificant | 1.1536923 | insignificant |
| B vs. C | 0.6985 | 1.4865869 | insignificant | 1.4865869 | insignificant |
| CHK treated cells | |||||
| A vs. B | 0.3615 | 2.1683911 | insignificant | 1.4455941 | insignificant |
| A vs. C | 0.1159 | 2.7277837 | insignificant | 0.9092612 | insignificant |
| B vs. C | 0.4774 | 1.9199406 | insignificant | 1.9199406 | insignificant |
A: MTT assay; B; Neutral red assay; C: Trypan blue assay.