Martínez-Escobedo, Vázquez-González, Valero-Galván, Álvarez-Parrilla, Garza-Ocañas, Najera-Medellin, and Quiñónez-Martínez: Antimicrobial activity, phenolic compounds content, and antioxidant capacity of four edible macromycete fungi from Chihuahua, Mexico

Journal Information

Journal ID (publisher-id): tip

Title: TIP. Revista especializada en ciencias químico-biológicas

Abbreviated Title: TIP

ISSN (print): 1405-888X

Publisher: Universidad Nacional Autónoma de México, Facultad de Estudios Superiores Zaragoza

Article Information

License (open-access, https://creativecommons.org/licenses/by-nc-nd/4.0/):

This is an open-access article distributed under the terms of the Creative Commons Attribution License

Date received: 05 November 2020

Date accepted: 04 June 2021

Publication date: 15 November 2021

Publication date: 2021

Volume: 24

Electronic Location Identifier: e318

DOI: 10.22201/fesz.23958723e.2021.318

Article Id (other): 00107

Antimicrobial activity, phenolic compounds content, and antioxidant capacity of four edible macromycete fungi from Chihuahua, Mexico

Translated Title (es): Actividad antimicrobiana, contenido de compuestos fenólicos y capacidad antioxidante de cuatro hongos macromicetos comestibles de Chihuahua, México

Neida Aurora Martínez-Escobedo[1]

Francisco Javier Vázquez-González[1]

José Valero-Galván[1]

Emilio Álvarez-Parrilla[1]

Fortunato Garza-Ocañas[2]

Jesús Alejandro Najera-Medellin[1]

Miroslava Quiñónez-Martínez[1][*]

[1] Instituto de Ciencias Biomédicas (ICB), Universidad Autónoma de Ciudad Juárez (UACJ), Av. Benjamín Franklin # 4650, Zona PRONAF, Ciudad Juárez 32310, Chihuahua, México. Universidad Autónoma de Ciudad Juárez Universidad Autónoma de Ciudad Juárez Instituto de Ciencias Biomédicas Ciudad Juárez 32310 Chihuahua Mexico

[2] Facultad de Ciencias Forestales, Universidad Autónoma de Nuevo León, Linares 67700, Nuevo León, México. Universidad Autónoma de Nuevo León Universidad Autónoma de Nuevo León Facultad de Ciencias Forestales Linares 67700 Nuevo León Mexico

Author notes:

Correspondence to: E-mail:*mquinone@uacj.mx

Abstract

In the present study, antimicrobial activity, phenolic compounds content and antioxidant capacity of four edible fungi (Amanita rubescens, Astraeus hygrometricus, Laccaria laccata and Lycoperdon perlatum) were determined.Antimicrobial activities were tested against Staphylococcus aureus, Streptococcus agalactiae and Candida albicans. Phenolic compounds and antioxidant activity were measured by spectrophotometric methods. All mushrooms present high activity against S. agalactiae. Phenolics compounds content ranked between 1.54 - 20.93 mg GAE/g DW and the antioxidant activity ranked between 0.0034 - 0.0854 mmol TE/g DW being A. rubescens the specie with the highest values. The results obtained for the antimicrobial activity using the disc diffusion method indicated that the extracts exhibited moderated antimicrobial activity. However, the MIC results with both solvents show that all the macromycete species registered inhibition of the microorganisms in different concentration. Generally, the ethanol extracts exerted stronger antimicrobial activity than methanol extracts. Similarly, S. agalactiae was the most susceptible microorganism, followed by C. albicans. S. aureus was the bacteria most resistant. The best antimicrobial activity was found in the ethanolic extracts of A. hygrometricus and L. perlatum against S. agalactiae, with a MIC value of 3.75 mg/mL. In conclusion, it is suggested that these species can be used as a natural source of antimicrobial and antioxidant components.

Resumen

En el presente estudio se determinó el contenido de compuestos fenólicos y la actividad antimicrobiana y antioxidante en cuatro especies de hongos comestibles (Amanita rubescens, Astraeus hygrometricus, Laccaria laccata y Lycoperdon perlatum). Las actividades antimicrobianas se probaron en Staphylococcus aureus, Streptococcus agalactiae y Candida albicans. Los compuestos fenólicos y la actividad antioxidante se midieron mediante métodos espectrofotométricos. Todos los hongos presentan una alta actividad en comparación con S. agalactiae. El contenido de compuestos fenólicos se ubicó entre 1.54 - 20.93 mg GAE/g DW y la actividad antioxidante entre 0.0034 - 0.0854 mmol TE / g DW, siendo A. rubescens la especie con el valor más alto encontrado. Los resultados obtenidos de la actividad antimicrobiana utilizando el método de difusión en disco indicaron que los extractos exhibieron una actividad moderada. Sin embargo, la Concentración Mínima Inhibitoria (CMI) con ambos disolventes muestra que todas las especies de macromicetos registraron inhibición de los microorganismos en diferentes concentraciones. En general, los extractos etanólicos ejercieron una actividad antimicrobiana mayor a los obtenidos con metanol. La bacteria S. agalactiae fue el microorganismo más susceptible y S. aureus la más resistente. La mejor actividad antimicrobiana se encontró en los extractos etanólicos de A. hygrometricus y L. perlatum, principalmente en S. agalactiae, con un valor de CMI de 3.75 mg/mL. En conclusión, se sugiere que estas especies de macromicetos se pueden utilizar como fuente natural de componentes antimicrobianos y antioxidantes.

Introduction

Infectious diseases represent one of the major threats worldwide due to the growing prevalence of drug resistance microorganisms (Wright, 2010). Within infectious diseases, the dermatologic infections are a public health problem, since it is estimated that between 30-70% of the world population is affected by at least one type of skin disease (Hay et al., 2014). Bacteria and fungus are considered responsible for dermatologic infections in humans, among the most frequents are Staphylococcus aureus, Streptococcus pyogenes and the species of the genus Candida (Riain, 2013). These microorganisms have been developed resistance to some commercial’s antibiotics. For this reason, it is necessary to continue the search for new compounds capable of their inhibition. Whereas the damage derived by the uncontrolled production of free radicals promotes the development of diseases like cancer, rheumatoid arthritis, cirrhosis, arteriosclerosis, and degenerative processes associated with aging (Elmastas, Isildak, Turkekul & Temur, 2007, Ren et al., 2014). Preliminary research has shown that macromycetes fungi produce a wide variety of bioactive compounds like phenolic compounds, which display an important role in the protection against oxidative damage, and the defense against bacteria, viruses, and insects (Leyva, Pérez- Carlón, González-Aguilar, Esqueda & Ayala-Zavala, 2013).

Macromycetes fungi have been recognized worldwide as sources of medicine and food (Quiñónez-Martínez et al., 2014). In Mexico, they have been incorporated into the diet of some ethnic groups and have been used for the treatment of different diseases since prehistoric times (Ruiz, Pérez-Moreno, Almaraz-Suárez &Torres-Aquino, 2013). Specifically, the Sierra Tarahumara of Chihuahua, Mexico has been known to have around 500 species of macromycete fungi (Gómez-Flores et al., 2019). Some of which have been reported to have medicinal and nutritional characteristics, like A. hygrometricus and L. perlatum, whose carpophores are used for acne problems as well as pain relievers, and burns cuts swelling (Quiñónez-Martínez et al., 2014). Likewise, L. laccata and A. rubescens show relevance due to their nutritive value, the last one is collected by the inhabitants for consumption and sale. Although there are many studies about the antimicrobial and antioxidant activities of macromycete fungi in the world, there is little information available about the traditional knowledge of mushrooms from the Sierra Tarahumara at Chihuahua, Mexico. The objective of this study was to evaluate the antimicrobial activities, the phenolics compounds and the antioxidant activity of four species of macromycete fungi from Chihuahua.

MATERIALS & METHODS

Samples and samples treatment

The fruiting body of A. rubescens, A. hygrometricus, L. laccata, and L. perlatum (Figure 1) were collected in the forest from the municipality of Bocoyna in the State of Chihuahua, Mexico, during August and September of 2017 and 2018. Samples were transported to the Laboratory of Biodiversity at the Institute of Biomedical Sciences (ICB) at the Universidad Autónoma de Ciudad Juárez (UACJ), where the identification and storage of the mushrooms were carried out. The samples were lyophilized (Labconco, Corp, Labconco, Kansas City, MO, EEUU) and grounded before analysis.

Figure 1

Carpophores of Amanita rubescens (a), Astraeus hygrometricus (b), Laccaria laccata (c) and Lycoperdon perlatum (d).

1405-888X-tip-24-e318-gf1.gif

Antimicrobial activity

Preparation of extracts

Powdered fruiting bodies (10 g) were extracted with 200 mL of absolute ethanol (Jalmek®) or absolute methanol (CTR scientific) respectively for 24 h. After that, the samples were sonicated (Bransonic® CPX5800H) for 30 min, then the extracts were centrifuged (IEC, HN-SII) for 10 min at 3,000 rpm and the supernatants were collected. The extracts were concentrated using a rotary evaporator (Büchi Rotavapor, R-114) and evaporated to dryness. Finally, the extracts were dissolved in the solvents at a concentration of 50 mg/mL and sterilized through a 0.22-micron membrane filter (Membrane Solutions) (Giri, Biswas, Pradhan, Mandal &Acharya, 2012). The extracts were stored at 4 °C for further use (Barros, Baptista, Estevinho & Ferreira, 2007).

Test microorganisms and growth conditions

For the antimicrobial activity, the microorganisms used were S. aureus, S. agalactiae, C. albicans (for the determination of the Minimum Inhibitory Concentration Test) and Candida sp. (for the determination of the diffusion disk test), which were obtained from the Microbiology Department at the university (UACJ).

Bacterial and fungal test organisms were grown in a different medium. S. aureus was cultured on Mueller Hilton agar (DIBICO®), S. agalactiae was cultured on Brain Heart Infusion Agar (BD Bioxon®). Both were incubated at 37 °C for 24 h. While fungal species were cultured on Potato DextroseAgar (BD Bioxon®) at 27 °C for 48 h. Then, S. aureus and Candida sp. were cultured in Trypticase Soy Broth (DIBICO®), while S. agalactiae was inoculated in Brain Heart Infusion Broth (DIBICO®) using the conditions before mentioned. Finally, the turbidity for each microorganism cultivated was adjusted to 0.5 McFarland standard which approximated to 1 x 106 CFU/mL.

Disk diffusion method

The antimicrobial activity was assessed by the disc diffusion method according to the modified procedure of Kalyoncu, Oskay, Sağlam, Erdoğan & Tamer (2010). Mueller Hinton agar, Brain Heart Infusion agar, and Potato Dextrose agar for S. aureus, S. agalactiae, and Candida sp., respectively. After 24 h, the turbidity of each microorganism cultivated was adjusted to 0.5 McFarland standard, which approximated to 1 x 106 CFU/mL. The surface of the plates was inoculated using 1 µL of the suspension, then was spread using a sterile cotton swab on Mueller Hinton agar for S. aureus, Brain Heart Infusion agar for S. agalactiae and Potato Dextrose Agar for Candida sp. Each test was carried out twice.

Smalls filter paper discs (6 mm diameter) were impregnated with 10 µL of the extracts and were air-dried until the excess of solvent was removed. After being dried, the discs were placed on the medium. Plates were incubated (at 37 °C for the bacterial and 27 °C for the fungi) and the zones of inhibition were measured after 24 h. Each test was done in duplicate. As positive control, erythromycin (2.5%) was used in case of bacteria and clotrimazole (2%) in case of fungi. As a negative control, methanol and ethanol (10 µL/disc) solvents were used.

Minimum Inhibitory Concentration (MIC)

The MIC of the extracts was determined according to the modified procedure of Padilla (2012). The extracts were incorporated into culture broth a concentration ranging from 1.25 mg/mL to 10 mg/mL, then 1 µL of each microorganism previously adjusted to equal that of 0.5 McFarland standard was inoculated and were incubated during 24 h (at 37 °C for the bacterial and 27 °C for the fungi). After the incubation time, 1 µL of each microorganism was used to inoculate the surface of the plates and were incubated for 24 h. The MIC of the extract for each test microorganism was considered the agar plate with the lower concentration without growth. A control without extract was prepared, and each assay was replicated three times.

Phenolic compounds and antioxidant activity

Preparation of extracts

The crude extracts for the determination of phenolics compounds and antioxidant activity were prepared according to Álvarez-Parrilla, de la Rosa, Martínez & González Aguilar, (2007). Dried samples (0.25 g) were mixed with 25 mL of 80% methanol and sonicated (Bransonic® CPX5800H) for 15 min. Then, the extracts were centrifugated (Eppendorf® 5804r) at 3,000 rpm and the supernatants were filtered using filter paper (Whatman No. 1). The extracting procedure was repeated, the supernatants were collected, and final volume was adjusted to 50 mL with 80% methanol.

Determination of total phenols

Total phenols were determined by the Folin-Ciocalteu method according to the modified procedure reported by Álvarez-Parrilla et al. (2007). Extract (250 µL) was mixed with 1,000 µLof 7.5% sodium carbonate (w/v) and 1250 µL of 10% Folin-Ciocalteu reagent (v/v). The mixture was incubated at 50 °C for 30 min, then, the absorbance was measured at 760 nm. A calibration curve was obtained using gallic acid as standard. Results are shown as mg of gallic acid equivalents (GAE) per gram of dry weight (mg GAE/g DW).

In vitro antioxidant assays (ABTS, DPPH and FRAP)

The antioxidant activity was evaluated using theABTS•+ radical (Álvarez-Parrilla, de la Rosa, Amarowicz & Shahidi, 2011). A 7 mM ABTS•+ reagent was prepared in a PBS solution (0.1 M, pH 7.4, KCl 0.15 M) mixed with sodium persulfate (2.45 mM) and incubated 16 h in darkness at room temperature. The absorbance of the ABTS•+ radical was adjusted to 0.7. Then, 285 µL of ABTS•+ solution was mixed with 12 µL of sample and the absorbance was measured at 734 nm for 30 min in a microplate reader (Bio Rad xMark). Inhibition percentage was determined according to equation 1:

(1)
1405-888X-tip-24-e318-g002.gifInhibition %=Ab-AsAbx100

WhereAb is the absorbance of the blank andAs is the absorbance in the presence of the extract. Trolox was used as standard and results were expressed as millimol Trolox equivalents (TE) per gram of dry weight (mmol TE/g DW).

The scavenging activity of the DPPH• radical was measured according to the procedure reported by Álvarez-Parrilla et al. (2011). Twenty-five µLof fungi extract was mixed with 200 µL of DPPH• reagent (190 µM in methanol). The absorbance was measured in a microplate reader at 517 nm for 30 min each 30 s at room temperature.

The inhibition percentage was determined using the equation (1). Trolox was used as standard and results were expressed as millimole Trolox equivalents (TE) per gram of dry weight (mmol TE/g DW).

The ferric reducing antioxidant power (FRAP) was measured using the modified methodology by Álvarez-Parrilla et al. (2011). The FRAP reagent was prepared by mixed 0.3 M acetate buffer (pH 3.6) with 10 mM TPTZ solution in 40 mM HCl and 20 mM FeCl3•H2O, at a 10:1:1 ratio. Then, FRAP reagent was incubated at 37 °C for 30 min. Afterwards, 180 µL of FRAP reagent was mixed with 24 µL of each extract, and the absorbance was measured at 595 for 60 min at 37 °C in a microplate reader. Trolox was used as standard and the results were expressed as millimol Trolox equivalents (TE) per gram of dry weight (mmol TE/g DW). All the experiments were done by triplicate.

Statistical analysis

Results of antimicrobial activity, total phenolic content, and antioxidant activity of the four species of macromycete fungi were expressed as mean values ± standard error (SE). The collected data was assumed to follow a normal distribution as determined by the Shapiro-Wilks test for normality (p > 0.05). A one-way ANOVA analysis of variance was performed to see if there were significant differences (p ≤ 0.05), afterwards a Tukey multiple mean comparison test was used. Lastly, a Pearson correlation test (r) was used to correlate the result of phenolic compounds and the antioxidant activity for all species together. Data was statistically analysed using SPSS (IBM, SPSS Statistics 20), Excel (Microsoft® Excel®, version 1903) and GraphPad Prism 8.1.2. software.

Results

Antimicrobial activity

Disk diffusion method

The results for the disk diffusion method are shown in Table I. The extracts obtained had an inhibitory response against S. agalactiae and Candida sp. to a concentration of 50 mg/mL, being S. agalactiae the microorganism most susceptible to the inhibitory action of macromicetes extracts. On the contrary, S. aureus was the most resistant microorganism due to the null activity of the extracts. The highest inhibitory activity was recorded by the ethanolic extract of L. perlatum against S. agalactiae (8.25 mm) and the ethanolic extract of A. hygrometricus showed the lowest activity against Candida sp. (4.5 mm). The range of extracts according to their inhibition zones against S. agalactiae was as follows: L. perlatum ethanol > A. hygrometricus methanol > L. laccata ethanol > L. laccata methanol > A. hygrometricus methanol > L. perlatum methanol. In general, the solvent with the best results was ethanol.

Table I

Antimicrobial activity of the ethanolic and methanolic extracts of four macromycete fungi from Chihuahua.

Macromycete fungi Mean inhibition zone (mm)
Ethanolic extracts Methanolic extracts
S. aureus S. agalactiae Candida sp. S. aureus S. agalactiae Candida sp.
Amanita rubescens - - - - - -
Astraeus hygrometricus - 5.79 ± 0.17de 4.5 ± 0.29e - 6.58 ± 0.31c -
Laccaria laccata - 6.43 ± 0.38cd - - 6.25 ± 0.47c -
Lycoperdon perlatum - 8.25 ± 0.25c - - 5.7 5 ± 0.25c -
Erythromycin (2.5%) 13.5 ± 0.20b 19.375 ± 0.47a - 13.5 ± 0.20b 19.375 ± 0.47a -
Clotrimazole (2%) - - 13.5 ± 0.28b - - 13.5 ± 0.28b
Solvent (Ethanol) - - - - - -

[i] Means value ± standard error. Different letters indicate significant differences, according to the Tukey HSD (p ≤ 0.05). - No inhibition. Extract concentration: 50 mg/mL. Fungal extracts/disc: 10 µL. Solvent/disc: 10 µL.

Minimum Inhibitory Concentration (MIC)

The minimum inhibitory concentration results showed that all the macromycete fungi species registered inhibition of the microorganisms at different concentration (Table II). The ethanol and methanol extracts of the tested mushrooms showed stronger antimicrobial activity when compared with the disc diffusion method. Generally, the ethanol extracts exerted stronger antimicrobial activity than methanol extracts. Similarly, S. agalactiae was the most susceptible microorganism, followed by C. albicans, and again S. aureus was the most resistant bacteria.

The best antimicrobial activity was found in the ethanolic extracts of A. hygrometricus and L. perlatum against S. agalactiae, with a MIC value of 3.75 mg/mL (Table II).

Table II

Minimum inhibitory concentration of the ethanolic and methanolic extracts of four macromycete fungi from Chihuahua.

Macromycete fungi Minimum inhibitory concentration (mg/mL)
Ethanolic extracts Methanolic extracts
S. aureus S. agalactiae C. albicans S. aureus S. agalactiae C. albicans
Amanita rubescens 8.75 5 7.5 10 6.25 7.50
Astraeus hygrometricus 7.5 3.75 6.25 8.75 5 6.25
Laccaria laccata 8.75 5 6.25 10 5 8.75
Lycoperdon perlatum 7.5 3.75 7.5 10 5 7.5

[i] Data are presented as the mean of three replicate.

The methanolic extracts of the macromycete fungi evaluated in this study showed complete inhibition of the pathogens at concentrations of 5 to 10 mg/mL (Table II). The lower MIC against the three microorganisms tested was exhibited by A. hygrometricus followed by the extracts of L. perlatum, and L. laccata, which presented similar MIC values. Finally, A. rubecens showed slightly weaker activity.

Phenolic compounds and antioxidant activity

The results of the quantification of total phenolic compounds and antioxidant capacity indicated variations in the averages depending on the species and the method used (Table III).

Table III

Content of phenolic compounds and antioxidant capacity of four macromycete fungi from Chihuahua.

Macromycete fungi Total phenols (mg GAE/g) ABTS (mmol TE/g) DPPH (mmol TE/g) FRAP (mmol TE/g)
Amanita rubescens 20.93 ± 0.90a 0.0854 ± 0.0024a 0.0437 ± 0.0004a 0.0254 ± 0.0006b
Astraeus hygrometricus 1.54 ± 0.07c 0.0074 ± 0.0002c 0.0135 ± 0.0010d 0.0034 ± 0.0002d
Laccaria laccata 8.75 ± 0.54b 0.0293 ± 0.0034b 0.0368 ± 0.0004b 0.0078 ± 0.0009c
Lycoperdon perlatum 6.05 ± 0.29b 0.0240 ± 0.0004b 0.0244 ± 0.0003c 0.0298 ± 0.0013a

[i] Values are presented as the mean of three replicates of analysis performed in triplicate ± standard error. Averages with different letters indicate a significant difference between fungal species due to antioxidant activity, according to the Tukey HSD test (p ≤ 0.05).

The total phenols content varied between 1.54 and 20.93 mg EAG/g DW. A. rubescens showed the highest content, followed by L. laccata, L. perlatum, and finally A. hygrometricus (Table III).

The antioxidant capacity of the four species were evaluated through the FRAP, DPPH and ABTS assays. The results indicate an antioxidant potential ranging from 0.0074 to 0.0854 mmol TE/g DW. The antioxidant capacity varied in a similar pattern to the total phenols content, thus the species with the highest antioxidant activity was A. rubescens (0.0854 mmol ET/g DW), while A. hygrometricus obtained the lowest activity (0.0034 mmol TE/g DW). In agreement with previously published results, antioxidant capacity methods showed different behaviour (Álvarez-Parrilla et al., 2014). In the case of A. rubescens and L. laccata, the highest averages were observed using the ABTS method, for A. hygrometricus it was by the DPPH method and for L. perlatum the best averages were found employing the FRAP assay.

Table IV shows the correlation between total phenols content and antioxidant capacity. These results indicate a highly significant correlation between the ABTS•+ radical and total phenols (r = 0.9951), there is also a significant correlation between total phenols and DPPH• radical (r = 0.9070), unlike for antioxidant capacity reducing FRAP, no significant correlation with total phenols content was found.

Table IV

Correlation between phenolic compounds (Ft) and antioxidant capacity (ABTS, DPPH, FRAP) of four species of macromycete fungi from Chihuahua.

Ft ABTS DPPH FRAP
Ft 1
ABTS 0.9951** 1
DPPH 0.9070* 0.8612 1
FRAP 0.5171 0.5415 0.3913 1

[i] *Significant ** Highly significant.

Discussion

Macromycete fungi represent a source of bioactive compounds that can be beneficial to humans (González-Barranco et al., 2009), it is known that their compounds could present different pharmacological activities like antimicrobial and antioxidant activities (Ren et al., 2014). In our study, we found that the four studied mushrooms species presented both activities. The antimicrobial activity of the mushrooms was tested using two different methods, disk diffusion assay and minimum inhibitory concentration (MIC). Only three macromycete fungi (A. hygrometricus, L. laccata and L. perlatum) presented inhibitory action against S. agalactiae and Candida sp. in the disk diffusion method. Nonetheless, employing the MIC method, all the mushroom extracts shown antimicrobial activity against the three-microorganism tested, which coincides with other studies that report greater effectiveness of the broth dilution method compared to the disk diffusion method when evaluating the antimicrobial activity of fungal extracts (Ren et al., 2014, Hleba et al., 2016). The disk diffusion method, as its name implies, depends primarily on the diffusion capacity of the substance present in the extracts (Ren et al., 2014), resulting in little mobility of the compounds in the agar due to its low solubility or high molecular mass.

The solvent with the best results was ethanol. This may be due to the differences in polarity with methanol and dielectric constant, which allows increasing the solubility of compounds with antimicrobial activity, such as polyphenols (Adhikari, Pandey, Agnihotri & Pande, 2018; Do et al., 2014).

The best antimicrobial activity was presented byA. hygrometricus and L. perlatum, due to the similarity of recorded values. For the disk diffusion method, the high inhibition zones were obtained by the ethanolic extract of L. perlatum against S. agalactiae (8.25 mm). These results accord with those found by Dulger (2005) who reports the antimicrobial activity of the ethanolic extract of L. perlatum, but against S. pyogenes. There are several compounds to which antimicrobial activity in L. perlatum can be attributed, such as those found in ethanolic and methanolic extracts, mainly phenolic compounds, alkaloids, carbohydrates, tannins, saponins, glycosides, and proteins (Akpi, Odoh, Ideh & Adobu, 2017).

Astraeus hygrometricus obtained the best inhibition values against Candida sp. since it was the only one capable of developing inhibition zones (4.5 mm) and the one that reported lower concentrations of the yeast by the MIC method. The antimicrobial activity of A. hygrometricus has been demonstrated in previous studies, Giri et al. (2012) reported positive zones of inhibition when extracting carpophores with methanol at a concentration of 10 mg/mL. Also, according to Lai et al. (2012), the constituents responsible for the inhibition against C. albicans in A. hygrometricus are two triterpenes known as astrakurkurol and astrakurkurone.

In the case of L. laccata, its extracts exhibited similar inhibition actions, this could be attributed to the phenolic compounds found in the carpophores (8.75 mg GAE/g DW), and in addition to the fatty acids found in the petroleum ether and ethyl acetate fractions from the ethanolic extract of L. laccata carpophores, such palmitic acid, linoleic acid, and oleic acid (Nieto & Cucaita, 2007), which have been previously reported as compounds with antimicrobial activity.

The extracts of A. rubescens did not show inhibition of the microorganisms through the disk diffusion method since this method is not appropriate to test partially or completely hydrophobic compounds (Ren et al., 2014), this specie is rich in compounds with such nature (Kalač, 2013). Among the majority compounds in the species of the Amanita genus are some peptides (Li & Oberlies, 2005), which have low solubility in a solid medium such as agar, but they manage to diffuse properly into a liquid (dilution in broth). Although A. rubescens was the specie with the highest content of total phenols (20.93 mg GAE/g DW), the low antimicrobial activity may be due to the existence of compounds linked to phenols that make them more hydrophilic, such as sugars, polysaccharides, lignins, amines, long-chainalcohols, and glycerol, as well as long-chain omega fatty acids (Naczk & Shahidi, 2006), making it difficult to diffuse during tests of antimicrobial activity. A. rubescens is the species with the least inhibitory effect using the MIC assay, along with other species of the same genus such as A. muscaria and A. phalloides which also exhibit a moderate MIC of 6.25 mg/mL against S. pyogenes (Chelela, Chacha & Matemu, 2014). S. agalactiae was the microorganism most susceptible to the inhibitory action of macromycetes, these results agree with several reports (Canli, Akata & Altuner, 2016; Alves et al., 2013). In general, some studies indicate that fungal extracts have a greater growth inhibitory effect on species belonging to the genus Streptococcus than other microorganisms, mainly in the species of S. pyogenes, S. mutans and S. sobrinus with MIC values ranging from 2.4 to 87.4 µg/mL(Doǧan, Duman, Özkalp & Aydin, 2013; Lund et al., 2009). Therefore, it is considered the microorganism more susceptible to most antibiotics, since there are few strains with characteristics of resistance to penicillin, ampicillin, and cefotaxime (Torres & Cercenado, 2010), making possible the action of the evaluated extracts against the microorganism in the present study.

Staphylococcus aureus did not show susceptibility since it is considered a microorganism with phenotypes resistant to different antibiotics such as beta-lactams and methicillin (Torres & Cercenado, 2010). However, the phenotype used in these tests of antimicrobial activity is unknown. There are studies about the null activity of fungal extracts against S. aureus such as that of Canli et al. (2016), who found no inhibition by the ethanolic extracts of Lycoperdon lividum; Barros, Venturini, Baptista, Estevinho & Ferreira (2008), whose extracts did not show antimicrobial activity using L. perlatum, and Giri et al. (2012), reporting no inhibition of the bacteria with methanolic extracts of A. hygrometricus.

Phenols compounds are widely distributed in plants and fungal species. Some studies mention that the total phenol content in fungi ranges between 6.08 and 24.85 mg GAE/g (Prasad, Varshney, Harsh & Kumar, 2015), although in the present investigation results are found in a range of 1.54 - 20.93 mg GAE/g DW. According to Mujić, Zeković, Lepojević,Vidović & Živković (2010), the range obtained of total phenolics compounds for mushrooms are in a range of 7.8 - 23.07 mg GAE/g, and for edible mushrooms it goes from 4.94 to 35.56 mg GAE/g (Alispahić et al., 2015). Even though our results are similar and are within the range reported, it is difficult to compare the results due to differences in the mode of expression of the results, extraction methods of the phenolic compounds in the fungi, and environmental conditions from the collection site.

Amanita rubescens (20.93 mg GAE/g DW) presented a high content of total phenols, which differs from that found by Keleş, Koca & Gençcelep (2011), who reported a content of 5.7 mg GAE/g DW. However, there are reports for other species of the genus Amanita with similar values than those found in the study, like A. patherina (5.27 mg GAE/g), A. muscaria (7.59 mg GAE/g), A. porphyria (14.53 mg GAE/g) and A. citrina (38.44 GAE/g) (Nowacka et al., 2015).

L. laccata and L. perlatum presented phenolic content in the range of those reported for this specie (8.75 and 6.05 mg GAE/g DW, respectively). Nowacka et al. (2014), found records like those of the study for L. laccata (9.38 mg GAE/g dry extract) and different for L. perlatum (13.59 mg GAE/g dry extract).According to Heleno, Barros, Sousa, Martins & Ferreira (2010), the variations found are mainly due to the substrate where the macromycetes grow, which causes modifications in the secondary metabolism of the species (shikimic acid and acetate pathway) affecting the production of phenolic compounds. In addition, the area and collection time also causes changes in the composition of total phenols (Smolskaite, Venskutonis & Talou, 2015). Astraeus hygrometricus was the species with the lowest content of total phenols (1.54 mg GAE/g DW) compared to the other species analyzed. These differences are mainly attributed to the extraction methods, due to the treatment of the carpophores with boiled water before quantification, maximizing the extraction of the compounds, since cooking results in an increase in total phenols (Pavithra, Sridhar, Greeshma & Tomita-Yokotani, 2016).

In general, fungi have great antioxidant activity (Álvarez- Parrilla et al., 2007; Elmastas et al., 2007), which is in a range that goes from 0.0741 to 7.61 mmol TE /100 g (Srikram & Supapvanich, 2016; Özyürek, Bener, Güçlü & Apak, 2014). However, in the present study lower values were found. The differences in the results of the antioxidant capacity are due to factors such as the analysis of different species, the area in which they are collected or the substrate where they grow (Heleno et al., 2010). As well as differences in extraction methods (since that there is still no standardization or consensus on the treatment of the sample before the analysis), among which are the extraction temperature and the relation of the solute with the solvent (Dai & Mumper, 2010). In the present investigation, the extraction temperature to assess antioxidant capacity was 24 °C and according to Özyürek et al. (2014), the optimal extraction temperature that improves the performance of antioxidant capacity in mushroom extracts is 80 °C, since an increase in temperature can accelerate cell rupture, generating a raise in internal pressure within the cells of fungi and promoting a higher solubility of the analyte (Dai & Mumper, 2010). Likewise, the use of solvents other than methanol may also show better results, since depending on the polarity of the solvents they will be able to extract various compounds that may have a high antioxidant capacity (Kosanić, Ranković, Rančić & Stanojković, 2016). Kaewnarin, Suwannarach, Kumla & Lumyong (2016), extracting the antioxidant compounds using ethanol, methanol, and water, with water shows highest antioxidant activity efficiency for the same methods evaluated (ABTS, DPPH, and FRAP).

ABTS assay measures the ability of the radical to donate a proton to an unstable cationic radical (ABTS•+), it is used to evaluate antioxidant capacity, making possible theanalysis ofhydrophilic and lipophilic compounds (Kaewnarin et al., 2016). The results obtained by this test showed that A. rubescens presents the highest averages of antioxidant capacity (0.0854 mmol TE/g DW), followed by L. laccata (0.0293 mmol TE/g DW), L. perlatum (0.0240 mmol TE/g DW) and A. hygrometricus (0.0074 mmol TE/g DW). This differs from that reported by Iwalokun, Usen, Otunba & Olukoya (2007), whose antioxidant activity (ABTS•+ radical) of Pleurotus ostreatus extracts was 4.4 millimol. However, they used acetone as a solvent, which can extract another class of antioxidant compound such as carotenoids and tocopherols (Liu, Jia, Kan & Jin, 2013), also the species was different.

DPPH test is considered one of the most widely used methods to evaluate antioxidant capacity because radicals are very stable and easy to use (Acharya, Khatua & Ray, 2017). The antioxidant activity of the extracts showed very similar averages among the species, with A. rubescens (0.043 mmol TE/g DW) being the species with the highest radical uptake, followed by L. laccata (0.0368 mmol TE/g DW), L. perlatum (0.0244 mmol TE/g DW) and A. hygrometricus (0.0135 mmol TE/g DW). The same behavior was observed with total phenols content, which coincides with that reported by Alothman, Bhat & Karim (2009), who mentioned that the higher the phenolic content, the higher the DPPH values. Recently Smolskaite et al. (2015), evaluated the antioxidant properties of eight macromycete species through different tests (ABTS, DPPH, and FRAP) using sequential extractions with solvents of different polarities (among which was methanol), whose valuesrangedfrom 0.12 to 9.62 µM TE/g DW for the DPPH assay is similar to the results obtained by the same method.

FRAP assay is based on measuring the ability of antioxidants to reduce ferric iron to its ferrous form (Kaewnarin et al., 2016). In this case, the highest value was presenting in L. perlatum (0.0298 mmol TE/g DW), followed by A. rubescens (0.0254 mmol TE/g DW), L. laccata (0.0078 mmol TE/g DW) and A. hygrometicus (0.0034 mmol TE/g DW). This differs from that reported by Srikram & Supapvanich, (2016), who obtained higher results in the species A. calyptroderma (1.98 mmol TE/100 g), A. princeps (1.14 mmol TE/100 g) and A. odoratus (07.61 mmol TE/100 g). In the same way, Yahia, Gutiérrez-Orozco & Moreno-Pérez (2017), reports higher reducing power averages for L. perlatum (17 mmol TE/100 g wet weight), A. flavoconia (7 mmol TE/100 g), A. pantherina (13 mmol TE/100 g) and A. virosa (6 mmol TE/100 g), which can be attributed to the same factors previously mentioned (different species, collection site, and extraction methods) (Kosanić et al., 2016; Nowacka et al., 2014). In our results, L. perlatum and A. rubescens were the species with the greatest reducing power, so it is believed that the phenolic compounds present in the species could have more hydroxyl-functional residues in the phenol rings than the other species, which act as electron donors in the reduction reaction (Liu et al., 2013).

Antioxidant capacity varied in a pattern like the phenolic compounds, thus the species with the highest antioxidant activity was A. rubescens, while A. hygrometricus obtained the lowest activity. According to Ferreira, Barros & Abreu (2009), the antioxidant activity of different species of macromycetes is mainly related to their phenolic content, since these compounds are known to be capable of donating hydrogen to free radicals to stop the lipid chain reaction in the initial stage (due to the presence of their hydroxyl groups) (Kosanić et al., 2016).

Some studies demonstrate a significant correlation between total phenols and antioxidant capacity using the radicals ABTS•+ and DPPH•, as well as those reported by different authors who mentioned correlation coefficients of 0.8 and 0.95 in several species of fungi (Kaewnarin et al., 2016; Smolskaite et al., 2015); confirming that phenolic compounds are important contributors to the antioxidant characteristics in fungal extracts. In the case of the ferric ion reducing ability (FRAP), there is no significant correlation, which indicates that not only are phenolic compoundsresponsible for theantioxidantactivityofthe species but also that other types of compounds with reducing power could be acting as antioxidants such as tocopherols, ascorbic acid, and carotenoids, which after phenolic compounds, are the main antioxidant compounds in macromycetes (Liu et al., 2013; Özyürek et al., 2014).

Finally, there is nodirectrelationbetween antimicrobialactivity with phenolic compounds and antioxidant activity. Since A. hygrometricus and L. perlatum showed to be the species with the best antimicrobial capacity, while A. rubescens turned out to be the species with the highest total phenol content and antioxidant capacity. These results are similar with some authors reporting that species with high phenol content and antioxidant capacity exhibit better results in tests of antimicrobial activity (Liu et al., 2013; Smolskaite et al., 2015). However, these differences may be due to the extraction methods used for each test, since in most of the studies they used the same extracts for the evaluation of the antimicrobial and antioxidant activity.

Conclusions

The evaluated macromycete fungal species presented antimicrobial activity, which varied depending on the solvent, the method used, and the microorganism tested, highlighting A. hygrometricus and L. perlatum. This finding promotes these species as an important source for obtaining compounds with pharmacological activities.

The optimal method to evaluate antimicrobial activity was through the minimum inhibitory concentration (MIC) technique since it allowed the correct diffusion of the extracted compounds.

The minimum concentration reached with the ethanolic extracts was of 8.75 mg/mL in A. hygrometricus and L. perlatum for S. aureus; 3.75 mg/mL for S. agalactiae with the same fungi previously mentioned, and 6.25 mg/mL for C. albicans using A. hygrometricus and L. laccata. On the other hand, for methanolic extracts the growth of S. aureus was inhibited at 8.75 mg/mL using A. hygrometricus; for S. agalactiae the MIC was 5mg/mL using A. hygrometricus, L. laccata and L. perlatum, finally, A. hygrometricus had the best response inhibiting C.albicans at a concentration of 6.25 mg/mL. Generally, the ethanol extracts exerted stronger antimicrobial activity than methanol extracts, making it possible to identify the inhibitory capacity of the mushroom species.

On the other hand, it was shown that the four fungi have phenolic compounds and antioxidant properties as measured by several tests, emphasizing A. rubescens, which, being an edible species, has the potential to be a source of natural antioxidants and other bioactive compounds for nutrition.Yet, it is important to identify the bioactive compounds responsible for the antimicrobial and antioxidant activities in these species, since they can participate in the production of new antibiotics and cope with diseases caused by oxidative stress.

Acknowledgements

The authors thank CONACYT for the scholarships awarded (#485096) to Neida Aurora Martínez Escobedo to carry out her master’s studies.

References

1 

Acharya, K., Khatua, S. & Ray, S. (2017). Quality assessment and antioxidant study of Pleurotus djamor (Rumph. ex Fr.) Boedijn. Journal of Applied Pharmaceutical Science, 7(6), 105-110. https://doi.org/10.7324/JAPS.2017.70614

K. Acharya S. Khatua S. Ray 2017Quality assessment and antioxidant study of Pleurotus djamor (Rumph. ex Fr.) BoedijnJournal of Applied Pharmaceutical Science7(6)10511010.7324/JAPS.2017.70614

2 

Adhikari, P., Pandey, A., Agnihotri, V. & Pande, V. (2018). Selection of solvent and extraction method for determination of antimicrobial potential of Taxus wallichiana Zucc. Research in Pharmacy, 8, 1-9.

P. Adhikari A. Pandey V. Agnihotri V. Pande 2018Selection of solvent and extraction method for determination of antimicrobial potential of Taxus wallichiana ZuccResearch in Pharmacy819

3 

Akpi, U., Odoh, C., Ideh, E. & Adobu, U. (2017). Antimicrobial Activity of Lycoperdon perlatum Whole Fruit Body on Common Pathogenic Bacteria and Fungi. Journal of Clinical and Experimental Microbiology, 18(2), 79-85. https://dx.doi.org/10.4314/ajcem.v18i2.4

U. Akpi C. Odoh E. Ideh U. Adobu 2017Antimicrobial Activity of Lycoperdon perlatum Whole Fruit Body on Common Pathogenic Bacteria and FungiJournal of Clinical and Experimental Microbiology18(2)798510.4314/ajcem.v18i2.4

4 

Alispahić, A., Šapčanin, A., Salihović, M., Ramić, E., Dedić, A. & Pazalja, M. (2015). Phenolic content and antioxidant activity of mushroom extracts from Bosnian market. Bulletin of the Chemists and Technologists of Bosnia and Herzegovina, 44, 5-8.

A. Alispahić A. Šapčanin M. Salihović E. Ramić A. Dedić M. Pazalja 2015Phenolic content and antioxidant activity of mushroom extracts from Bosnian marketBulletin of the Chemists and Technologists of Bosnia and Herzegovina4458

5 

Alothman, M., Bhat, R. & Karim, A. A. (2009). Antioxidant capacity and phenolic content of selected tropical fruits from Malaysia, extracted with different solvents. Food Chemistry, 115(3), 785-788. https://doi.org/10.1016/j. foodchem.2008.12.005

M. Alothman R. Bhat A. A. Karim 2009Antioxidant capacity and phenolic content of selected tropical fruits from Malaysia, extracted with different solventsFood Chemistry115(3)78578810.1016/j. foodchem.2008.12.005

6 

Álvarez-Parrilla, E., de La Rosa, L. A., Martínez, N. R. & González Aguilar, G. A. (2007). Total phenols and antioxidant activity of commercial and wild mush rooms from Chihuahua, Mexico. Ciencia y Tecnologia Alimentaria, 5(5), 329-334. https://doi.org/10.1080/11358120709487708

E. Álvarez-Parrilla L. A. de La Rosa N. R. Martínez G. A. González Aguilar 2007Total phenols and antioxidant activity of commercial and wild mush rooms from Chihuahua, MexicoCiencia y Tecnologia Alimentaria5(5)32933410.1080/11358120709487708

7 

Álvarez-Parrilla, E., de la Rosa, L., Amarowicz, R. & Shahidi, F. (2011). Antioxidant Activity of Fresh and Processed Jalapen Serrano Peppers. Journal of Agricultural and Food Chemistry, 59, 163-173. https://doi.org/10.1021/jf103434u

E. Álvarez-Parrilla L. de la Rosa R. Amarowicz F. Shahidi 2011Antioxidant Activity of Fresh and Processed Jalapen Serrano PeppersJournal of Agricultural and Food Chemistry59163173

8 

Álvarez-Parrilla, E., Mercado-Mercado, G., de la Rosa, L. A., López.Díaz, J..A., Wall-Medrano, A. & González-Aguilar, F. (2014), Antioxidant activity and prevention of pork meat lipid oxidation using traditional Mexican condiments (pasilla dry pepper, achiote, and mole sauce). Food Science and Technology Campinas, 34(2), 371-378. http://dx.doi.org/10.1590/fst.2014.0052

E. Álvarez-Parrilla G. Mercado-Mercado L. A. de la Rosa J..A. López.Díaz A. Wall-Medrano F. González-Aguilar 2014Antioxidant activity and prevention of pork meat lipid oxidation using traditional Mexican condiments (pasilla dry pepper, achiote, and mole sauce)Food Science and Technology Campinas34(2)37137810.1590/fst.2014.0052

9 

Alves, M. J., Ferreira, I. C. F. R., Dias, J., Teixeira, V., Martins, A. & Pintado, M. (2013). A Review on antifungal activity of mushroom (basidiomycetes) extracts and isolated compounds. Current Topics in Medicinal Chemistry, 13(21), 2648-2659. https://doi.org/10.2174/15680266113136660191

M. J. Alves I. C. F. R. Ferreira J. Dias V. Teixeira A. Martins M. Pintado 2013A Review on antifungal activity of mushroom (basidiomycetes) extracts and isolated compoundsCurrent Topics in Medicinal Chemistry13(21)2648265910.2174/15680266113136660191

10 

Barros, L., Baptista, P., Estevinho, L. M. & Ferreira, I. C. F. R. (2007). Effect of fruiting body maturity stage on chemical composition and antimicrobial activity of Lactarius sp. mushrooms. Journal of Agricultural and Food Chemistry, 55(21), 8766-8771. https://doi.org/10.1021/jf071435

L. Barros P. Baptista L. M. Estevinho I. C. F. R. Ferreira 2007Effect of fruiting body maturity stage on chemical composition and antimicrobial activity of Lactarius sp. mushroomsJournal of Agricultural and Food Chemistry55(21)8766877110.1021/jf071435

11 

Barros, L., Venturini, B. A., Baptista, P., Estevinho, L. M. & Ferreira, I. C. F. R. (2008). Chemical composition and biological properties of Portuguese wild mushrooms: A comprehensive study. Journal of Agricultural and Food Chemistry, 56(10), 3856-3862. https://doi.org/10.1021/ jf8003114

L. Barros B. A. Venturini P. Baptista L. M. Estevinho I. C. F. R. Ferreira 2008Chemical composition and biological properties of Portuguese wild mushrooms: A comprehensive studyJournal of Agricultural and Food Chemistry56(10)3856386210.1021/ jf8003114

12 

Canli, K.,Akata, I. & Altuner, E. M. (2016). In VitroAntimicrobial Activity Screening of Xylaria hypoxylon. African Journal of Traditional, Complementary and Alternative Medicines, 13(4), 42-46. https://doi.org/10.21010/ajtcam.v13i4.7

K. Canli I. Akata E. M. Altuner 2016In VitroAntimicrobial Activity Screening of Xylaria hypoxylonAfrican Journal of Traditional, Complementary and Alternative Medicines13(4)424610.21010/ajtcam.v13i4.7

13 

Chelela, B. L., Chacha, M. & Matemu, A. (2014). Antibacterial and antifungal activities of selected wild mushrooms from Southern Highlands of Tanzania. American Journal of Research Communication, 2(9), 58-68.

B. L. Chelela M. Chacha A. Matemu 2014Antibacterial and antifungal activities of selected wild mushrooms from Southern Highlands of TanzaniaAmerican Journal of Research Communication2(9)5868

14 

Dai, J. & Mumper, R. J. (2010). Plant phenolics: Extraction, analysis and their antioxidant and anticancer properties. Molecules, 15(10), 7313-7352. https://doi.org/10.3390/molecules15107313

J. Dai R. J. Mumper 2010Plant phenolics: Extraction, analysis and their antioxidant and anticancer propertiesMolecules15(10)7313735210.3390/molecules15107313

15 

Do, Q. D., Angkawijaya, E., Tran-Nguyen, P., Huynh, L., Soetaredjo, F., Ismadji, S. & Ju, Y.-H. (2014). Effect of extraction solvent on total phenol content , total flavonoid content , and antioxidant activity of Limnophila aromatica. Journal of Food and Drug Analysis, 22, 296-302. https://doi.org/10.1016/j.jfda.2013.11.001

Q. D. Do E. Angkawijaya P. Tran-Nguyen L. Huynh F. Soetaredjo S. Ismadji Y.-H. Ju 2014Effect of extraction solvent on total phenol content , total flavonoid content , and antioxidant activityLimnophila aromatica. Journal of Food and Drug Analysis2229630210.1016/j.jfda.2013.11.001

16 

Doǧan, H. H., Duman, R., Özkalp, B. & Aydin, S. (2013). Antimicrobial activities of some mushrooms in Turkey. Pharmaceutical Biology, 51(6), 707-711. https://doi.org/10.3109/13880209.2013.764327

H. H. Doǧan R. Duman B. Özkalp S. Aydin 2013Antimicrobial activities of some mushrooms in TurkeyPharmaceutical Biology51(6)70771110.3109/13880209.2013.764327

17 

Dulger, B. (2005). Antimicrobial activity of ten Lycoperdaceae. Fitoterapia, 76(3-4), 352-354. https://doi.org/10.1016/j. fitote.2005.02.004

B. Dulger 2005Antimicrobial activity of ten LycoperdaceaeFitoterapia76(3-4)35235410.1016/j. fitote.2005.02.004

18 

Elmastas, M., Isildak, O., Turkekul, I. & Temur, N. (2007). Determination of antioxidant activity and antioxidant compounds in wild edible mushrooms. Journal of Food Composition and Analysis, 20(3-4), 337-345. https://doi.org/10.1016/j.jfca.2006.07.003

M. Elmastas O. Isildak I. Turkekul N. Temur 2007Determination of antioxidant activity and antioxidant compounds in wild edible mushroomsJournal of Food Composition and Analysis20(3-4)33734510.1016/j.jfca.2006.07.003

19 

Ferreira, I., Barros, L. & Abreu, R. (2009). Antioxidants in Wild Mushrooms. Current Medicinal Chemistry, 16(12), 1543-1560. https://doi.org/10.2174/092986709787909587

I. Ferreira L. Barros 2009Antioxidants in Wild MushroomsCurrent Medicinal Chemistry16(12)1543156010.2174/092986709787909587

20 

Giri, S., Biswas, G., Pradhan, P., Mandal, S. C. & Acharya, K. (2012). Antimicrobial activities of basidiocarps of wild edible mushrooms of West Bengal, India. International Journal of PharmTech Research, 4(4), 1554-1560.

S. Giri G. Biswas P. Pradhan S. C. Mandal K. Acharya 2012Antimicrobial activities of basidiocarps of wild edible mushrooms of West Bengal, IndiaInternational Journal of PharmTech Research4(4)15541560

21 

Gómez-Flores, L. D. J., Martínez-Ruiz, N. D. R., Enríquez- Anchondo, I. D., Garza-Ocañas, F., Nájera-Medellín, J. A. & Quiñónez-Martínez, M. (2019). Análisis proximal y de composición mineral de cuatro especies de hongos ectomicorrízicos silvestres de la Sierra Tarahumara de Chihuahua. TIP Revista Especializada En Ciencias Químico-Biológicas, Vol. 22, 1-10. https://doi.org/10.22201/fesz.23958723e.2019.0.184

L. D. J. Gómez-Flores N. D. R. Martínez-Ruiz I. D. Enríquez- Anchondo F. Garza-Ocañas J. A. Nájera-Medellín M. Quiñónez-Martínez 2019Análisis proximal y de composición mineral de cuatro especies de hongos ectomicorrízicos silvestres de la Sierra Tarahumara de ChihuahuaTIP Revista Especializada En Ciencias Químico-Biológicas2211010.22201/fesz.23958723e.2019.0.184

22 

González Barranco, P., Garza Ocañas, L., Salinas Carmona, M., Vera Cabrera, L., Garza Ocañas, F., Ramírez Gómez, X. & Torres Alanis, O. (2009). Actividad antioxidadnte, antimicrobiana y citotoxicidad de dos espcies mexicanas de Suillus spp. CIENCIA UANL, XII(1), 62-70.

P. González Barranco L. Garza Ocañas M. Salinas Carmona L. Vera Cabrera F. Garza Ocañas X. Ramírez Gómez O. Torres Alanis 2009Actividad antioxidadnte, antimicrobiana y citotoxicidad de dos espcies mexicanas de Suillus sppCIENCIA UANLXII(1)6270

23 

Hay, R. J., Johns, N. E., Williams, H. C., Bolliger, I. W., Dellavalle, R. P., Margolis, D. J., Marks, R., Naldi, L., Weinstock, M. A., Wulf, S. K., Michaud, C., Murray, C. & Naghavi, M. (2014). The Global Burden of Skin Disease in 2010: An Analysis of the Prevalence and Impact of Skin Conditions. Journal of Investigative Dermatology, 134(6), 1527-1534. https://doi.org/10.1038/jid.2013.446

R. J. Hay N. E. Johns H. C. Williams I. W. Bolliger R. P. Dellavalle D. J. Margolis R. Marks L. Naldi M. A. Weinstock S. K. Wulf C. Michaud C. Murray M. Naghavi 2014The Global Burden of Skin Disease in 2010: An Analysis of the Prevalence and Impact of Skin ConditionsJournal of Investigative Dermatology134(6)1527153410.1038/jid.2013.446

24 

Heleno, S. A., Barros, L., Sousa, M. J., Martins, A. & Ferreira, I. C. F. R. (2010). Tocopherols composition of Portuguese wild mushrooms with antioxidant capacity. Food Chemistry, 119(4), 1443-1450. https://doi.org/10.1016/j.foodchem.2009.09.025

S. A. Heleno L. Barros M. J. Sousa A. Martins I. C. F. R. Ferreira 2010Tocopherols composition of Portuguese wild mushrooms with antioxidant capacityFood Chemistry119(4)1443145010.1016/j.foodchem.2009.09.025

25 

Hleba, L., Kompas, M., Hutková, J., Rajtar, M., Petrová, J., Čuboň, J., Kántor, A. & Kačániová, M. (2016). Antimicrobial activity of crude ethanolic extracts from some medicinal mushrooms. Journal of Microbiology, Biotechnology and Food Sciences, 05(Speciall), 60-63. https://doi.org/10.15414/jmbfs.2016.5.speciall.60-63

L. Hleba M. Kompas J. Hutková M. Rajtar J. Petrová J. Čuboň A. Kántor M. Kačániová 2016Antimicrobial activity of crude ethanolic extracts from some medicinal mushroomsJournal of Microbiology, Biotechnology and Food Sciences05(Speciall)606310.15414/jmbfs.2016.5.speciall.60-63

26 

Iwalokun, B.A., Usen, U.A., Otunba,A.A. & Olukoya, K. (2007). Comparative phytochemical evaluation, antimicrobial and antioxidant properties of Pleurotus ostreatus. African Journal of Biotechnology, 6(15), 1732-1739. https://doi.org/10.5897/ajb2007.000-2254

B.A. Iwalokun U.A. Usen A.A. Otunba K. Olukoya 2007Comparative phytochemical evaluation, antimicrobial and antioxidant properties of Pleurotus ostreatusAfrican Journal of Biotechnology6(15)1732173910.5897/ajb2007.000-2254

27 

Kalač, P. (2013). A review of chemical composition and nutritional value of wild-growing and cultivated mushrooms. Journal of the Science of Food and Agriculture, 93(2), 209-218.

P. Kalač 2013A review of chemical composition and nutritional value of wild-growing and cultivated mushroomsJournal of the Science of Food and Agriculture93(2)209218

28 

Kalyoncu, F., Oskay, M., Sağlam, H., Erdoğan, T. F. & Tamer, A. Ü. (2010). Antimicrobial and Antioxidant Activities of Mycelia of 10 Wild Mushroom Species. Journal of Medicinal Food, 13(2), 415-419.

F. Kalyoncu M. Oskay H. Sağlam T. F. Erdoğan A. Ü. Tamer 2010Antimicrobial and Antioxidant Activities of Mycelia of 10 Wild Mushroom SpeciesJournal of Medicinal Food13(2)415419

29 

Kaewnarin, K., Suwannarach, N., Kumla, J. & Lumyong, S. (2016). Phenolic profile of various wild edible mushroom extracts from Thailand and their antioxidant properties, anti-tyrosinase and hyperglycaemic inhibitory activities. Journal of Functional Foods, 27, 352-364. https://doi.org/10.1016/j.jff.2016.09.008

K. Kaewnarin N. Suwannarach J. Kumla S. Lumyong 2016Phenolic profile of various wild edible mushroom extracts from Thailand and their antioxidant properties, anti-tyrosinase and hyperglycaemic inhibitory activitiesJournal of Functional Foods2735236410.1016/j.jff.2016.09.008

30 

Keleş, A., Koca, İ. & Gençcelep, H. (2011). Antioxidant Properties of Wild Edible Mushrooms. Journal of Food Processing & Technology, 2(6), 1-6. https://doi.org/10.4172/2157-7110.1000130

A. Keleş İ. Koca H. Gençcelep 2011Antioxidant Properties of Wild Edible MushroomsJournal of Food Processing & Technology2(6)1610.4172/2157-7110.1000130

31 

Kosanić, M., Ranković, B., Rančić, A. & Stanojković, T. (2016). Evaluation of metal concentration and antioxidant, antimicrobial, and anticancer potentials of two edible mushrooms Lactarius deliciosus and Macrolepiota procera. Journal of Food and Drug Analysis, 24(3), 477-484. https://doi.org/10.1016/j.jfda.2016.01.008

M. Kosanić B. Ranković A. Rančić T. Stanojković 2016Evaluation of metal concentration and antioxidant, antimicrobial, and anticancer potentials of two edible mushrooms Lactarius deliciosus and Macrolepiota proceraJournal of Food and Drug Analysis24(3)47748410.1016/j.jfda.2016.01.008

32 

Lai, T., Biswas, G., Chatterjee, S., Dutta, A., Pal, C., Banerji, J., Bhuvanesh, N., Reibenspies, J. & Acharya, K. (2012). Leishmanicidal and anticandidal activity of constituents of Indian edible mushroom Astraeus hygrometricus. Chemistry and Biodiversity, 9(April), 1517-1524.

T. Lai G. Biswas S. Chatterjee A. Dutta C. Pal J. Banerji N. Bhuvanesh J. Reibenspies K. Acharya 2012Leishmanicidal and anticandidal activity of constituents of Indian edible mushroom Astraeus hygrometricusChemistry and Biodiversity9(April)15171524

33 

Leyva, J. M., Pérez-Carlón, J. J., González-Aguilar, G. A., Esqueda, M. & Ayala-Zavala, J. F. (2013). Funcionalidad antibacteriana y antioxidante de extractos hidroalcohólicos de Phellinus merrillii. Revista Mexicana de Micología, 37, 11-17. Retrieved from http://revistamexicanademicologia.org/wp-content/uploads/2013/06/RMM-Tr-273-version-paginada-11-17.pdf

J. M. Leyva J. J. Pérez-Carlón G. A. González-Aguilar M. Esqueda J. F. Ayala-Zavala 2013Funcionalidad antibacteriana y antioxidante de extractos hidroalcohólicos de Phellinus merrilliiRevista Mexicana de Micología371117http://revistamexicanademicologia.org/wp-content/uploads/2013/06/RMM-Tr-273-version-paginada-11-17.pdf

34 

Li, C., & Oberlies, N. H. (2005). The most widely recognized mushroom: Chemistry of the genus Amanita. Life Sciences, 78, 532-538. https://doi.org/10.1016/j.lfs.2005.09.003

C. Li N. H. Oberlies 2005The most widely recognized mushroom: Chemistry of the genus AmanitaLife Sciences7853253810.1016/j.lfs.2005.09.003

35 

Liu, J., Jia, L., Kan, J. & Jin, C. (2013). In vitro and in vivo antioxidant activity of ethanolic extract of white button mushroom (Agaricus bisporus). Food and Chemical Toxicology, 51(1), 310-316. https://doi.org/10.1016/j.fct.2012.10.014

J. Liu L. Jia J. Kan C. Jin 2013In vitro and in vivo antioxidant activity of ethanolic extract of white button mushroom (Agaricus bisporus)Food and Chemical Toxicology51(1)31031610.1016/j.fct.2012.10.014

36 

Lund, R. G., Del Pino, F. A. B., Serpa, R., do Nascimento, J. S., Da Silva, V. M. I., Ribeiro, G. A. & Rosalen, P. L. (2009). Antimicrobial activity of ethanol extracts of Agaricus brasiliensis against mutans streptococci. Pharmaceutical Biology, 47(9), 910-915. https://doi.org/10.1080/13880200902950801

R. G. Lund F. A. B. Del Pino R. Serpa J. S. do Nascimento V. M. I. Da Silva G. A. Ribeiro P. L. Rosalen 2009Antimicrobial activity of ethanol extracts of Agaricus brasiliensis against mutans streptococciPharmaceutical Biology47(9)91091510.1080/13880200902950801

37 

Mujić, I., Zeković, Z., Lepojević, Ž., Vidović, S. & Živković, J. (2010).Antioxidant properties of selected edible mushroom species. Journal of Central European Agriculture, 11(4), 387-391.

I. Mujić Z. Zeković Ž. Lepojević S. Vidović J. Živković 2010Antioxidant properties of selected edible mushroom speciesJournal of Central European Agriculture11(4)387391

38 

Naczk, M. & Shahidi, F. (2006). Phenolics in cereals , fruits and vegetables: Occurrence, extraction and analysis. Journal of Pharmaceutical and Biomedical Analysis, 41, 1523-1542. https://doi.org/10.1016/j.jpba.2006.04.002

M. Naczk F. Shahidi 2006Phenolics in cereals , fruits and vegetables: Occurrence, extraction and analysisJournal of Pharmaceutical and Biomedical Analysis411523154210.1016/j.jpba.2006.04.002

39 

Nieto, I. J. & Cucaita, E. del P. (2007). Ácidos grasos, ésteres y esteroles del cuerpo fructífero del hongo Laccaria laccata. Revista Colombiana de Química, 36(3), 277-284. Retrieved from http://revistas.unal.edu.co/index.php/rcolquim/article/view/1290

I. J. Nieto E. del P. Cucaita 2007Ácidos grasos, ésteres y esteroles del cuerpo fructífero del hongo Laccaria laccataRevista Colombiana de Química36(3)277284http://revistas.unal.edu.co/index.php/rcolquim/article/view/1290

40 

Nowacka, N., Nowak, R., Drozd, M., Olech, M., Los, R. & Malm, A. (2015). Antibacterial, antiradical potential and phenolic compounds of thirty-one polish mushrooms. PLoS ONE, 10(10), 1-13. https://doi.org/10.1371/journal. pone.0140355

N. Nowacka R. Nowak M. Drozd M. Olech R. Los A. Malm 2015Antibacterial, antiradical potential and phenolic compounds of thirty-one polish mushroomsPLoS ONE10(10)11310.1371/journal. pone.0140355

41 

Nowacka, N., Nowak, R., Drozd, M., Olech, M., Los, R. & Malm, A. (2014). Analysis of phenolic constituents, antiradical and antimicrobial activity of edible mushrooms growing wild in Poland. LWT - Food Science and Technology, 59(2P1), 689-694. https://doi.org/10.1016/j.lwt.2014.05.041

N. Nowacka R. Nowak M. Drozd M. Olech R. Los A. Malm 2014Analysis of phenolic constituents, antiradical and antimicrobial activity of edible mushrooms growing wild in PolandLWT - Food Science and Technology59(2P1)68969410.1016/j.lwt.2014.05.041

42 

Özyürek, M., Bener, M., Güçlü, K. & Apak, R. (2014). Antioxidant/antiradical properties of microwave- assisted extracts of three wild edible mushrooms. Food Chemistry, 157, 323-331. https://doi.org/10.1016/j.foodchem.2014.02.053

M. Özyürek M. Bener K. Güçlü R. Apak 2014Antioxidant/antiradical properties of microwave- assisted extracts of three wild edible mushroomsFood Chemistry15732333110.1016/j.foodchem.2014.02.053

43 

Padilla, M. A. (2012). Inhibición in vitro del Enterococcus faecalis con hidróxido de calcio, clorexidina y ozono. Universidad Autónoma de Ciudad Juárez, Tesis de Maestría, 129.

M. A. Padilla 2012Inhibición in vitro del Enterococcus faecalis con hidróxido de calcio, clorexidina y ozonoUniversidad Autónoma de Ciudad JuárezMaestría129129

44 

Pavithra, M., Sridhar, K. R., Greeshma, A. A. & Tomita- Yokotani, K. (2016). Bioactive potential of the wild mushroom Astraeus hygrometricus in South-west India. Mycology, 7(4), 191-202. https://doi.org/10.1080/21501203.2016.1260663

M. Pavithra K. R. Sridhar A. A. Greeshma K. Tomita- Yokotani 2016Bioactive potential of the wild mushroom Astraeus hygrometricus in South-west IndiaMycology7(4)19120210.1080/21501203.2016.1260663

45 

Prasad, R., Varshney V. K., Harsh, N. S. K. & Kumar, M. (2015). Antioxidant Capacity and Total Phenolics Content of the Fruiting Bodies and Submerged Cultured Mycelia of Sixteen Higher Basidiomycetes Mushrooms from India. International Journal of Medicinal Mushrooms, 17(10), 933-941.

R. Prasad V. K. Varshney N. S. K. Harsh M. Kumar 2015Antioxidant Capacity and Total Phenolics Content of the Fruiting Bodies and Submerged Cultured Mycelia of Sixteen Higher Basidiomycetes Mushrooms from IndiaInternational Journal of Medicinal Mushrooms17(10)933941

46 

Quiñónez-Martínez, M., Ruan-Soto, F., Aguilar-Moreno, E., Garza-Ocañas, F., Lebgue-Keleng, T., Lavín-Murcio, A. & Enríquez-Anchondo, I. (2014). Knowledge and use of edible mushrooms in two municipalities of the Sierra Tarahumara, Chihuahua, Mexico. Journal of ethnobiology and ethnomedicine, 10(67), 1-13. DOI: 10.67.10.1186/1746-4269-10-67.

M. Quiñónez-Martínez F. Ruan-Soto E. Aguilar-Moreno F. Garza-Ocañas T. Lebgue-Keleng A. Lavín-Murcio I. Enríquez-Anchondo 2014Knowledge and use of edible mushrooms in two municipalities of the Sierra Tarahumara, Chihuahua, MexicoJournal of ethnobiology and ethnomedicine10(67),11310.67.10.1186/1746-4269-10-67

47 

Ren, L., Hemar, Y., Perera, C. O., Lewis, G., Krissansen, G. W. & Buchanan, P. K. (2014). Antibacterial and antioxidant activities of aqueous extracts of eight edible mushrooms. Bioactive Carbohydrates and Dietary Fibre, 3(2), 41-51. https://doi.org/10.1016/j.bcdf.2014.01.003

L. Ren Y. Hemar C. O. Perera G. Lewis G. W. Krissansen P. K. Buchanan 2014Antibacterial and antioxidant activities of aqueous extracts of eight edible mushroomsBioactive Carbohydrates and Dietary Fibre3(2)415110.1016/j.bcdf.2014.01.003

48 

Riain, N. U. (2013). Recommended management of common bacterial skin infections. Prescriber, 22(15-16), 15-25.

N. U. Riain 2013Recommended management of common bacterial skin infectionsPrescriber22(15-16)1525

49 

Ruiz, M. J., Pérez-Moreno, J., Almaraz-Suárez, J. J. & Torres- Aquino, M. (2013). Hongos silvestres con potencial nutricional, medicinal y biotecnológico comercializados en Valles Centrales, Oaxaca. Revista Mexicana de Ciencias Agrícolas, 4(4), 199-213.

M. J. Ruiz J. Pérez-Moreno J. J. Almaraz-Suárez M. Torres- Aquino 2013Hongos silvestres con potencial nutricional, medicinal y biotecnológico comercializados en Valles Centrales, OaxacaRevista Mexicana de Ciencias Agrícolas4(4)199213

50 

Smolskaite, L., Venskutonis, P. R. & Talou, T. (2015). Comprehensive evaluation of antioxidant and antimicrobial properties of different mushroom species. LWT - Food Science and Technology, 60(1), 462-471. https://doi.org/10.1016/j.lwt.2014.08.007

L. Smolskaite P. R. Venskutonis T. Talou 2015Comprehensive evaluation of antioxidant and antimicrobial properties of different mushroom speciesLWT - Food Science and Technology60(1)46247110.1016/j.lwt.2014.08.007

51 

Srikram, A. & Supapvanich, S. (2016). Proximate compositions and bioactive compounds of edible wild and cultivated mushrooms from Northeast Thailand. Agriculture and Natural Resources, 50(6), 432-436. https://doi.org/10.1016/j.anres.2016.08.001

A. Srikram S. Supapvanich 2016Proximate compositions and bioactive compounds of edible wild and cultivated mushrooms from Northeast ThailandAgriculture and Natural Resources50(6)43243610.1016/j.anres.2016.08.001

52 

Torres, C. & Cercenado, E. (2010). Lectura interpretada del antibiograma de cocos gram positivos. Enfermedades Infecciosas y Microbiologia Clínica, 28(8), 541-553. https://doi.org/10.1016/j.eimc.2010.02.003

C. Torres E. Cercenado 2010Lectura interpretada del antibiograma de cocos gram positivosEnfermedades Infecciosas y Microbiologia Clínica28(8)54155310.1016/j.eimc.2010.02.003

53 

Wright, G. D. (2010). Antibiotic resistance in the environment: A link to the clinic? Current Opinion in Microbiology, 13(5), 589-594. https://doi.org/10.1016/j.mib.2010.08.005

G. D. Wright 2010Antibiotic resistance in the environment: A link to the clinic?Current Opinion in Microbiology13(5)58959410.1016/j.mib.2010.08.005

54 

Yahia, E. M., Gutiérrez-Orozco, F. & Moreno-Pérez, M. A. (2017). Identification of phenolic compounds by liquid chromatography-mass spectrometry in seventeen species of wild mushrooms in Central Mexico and determination of their antioxidant activity and bioactive compounds. Food Chemistry, 226, 14-22. https://doi.org/10.1016/j.foodchem.2017.01.044

E. M. Yahia F. Gutiérrez-Orozco M. A. Moreno-Pérez 2017Identification of phenolic compounds by liquid chromatography-mass spectrometry in seventeen species of wild mushrooms in Central Mexico and determination of their antioxidant activity and bioactive compoundsFood Chemistry226142210.1016/j.foodchem.2017.01.044

Article Information (continued)

Categories:

Subject: Artículos originales

Keywords::

Keywords:

Keyword: bioactive compounds

Keyword: microorganisms

Keyword: edible fungi

Palabras clave::

Palabras clave:

Keyword: compuestos bioactivos

Keyword: microorganismos

Keyword: hongos comestibles

Counts:

Figures: 1

Tables: 4

Equations: 1

References: 54

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