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Abanico veterinario
versión On-line ISSN 2448-6132versión impresa ISSN 2007-428X
Abanico vet vol.12 Tepic ene./dic. 2022 Epub 31-Oct-2022
https://doi.org/10.21929/abavet2022.1
Short communication
In vitro anthelmintic and antibacterial effect of Kalanchoe daigremontiana leaves and stems hydroalcoholic extract
1
http://orcid.org/0000-0002-6154-9983
2
http://orcid.org/0000-0001-5705-1704
3
http://orcid.org/0000-0003-2592-6689
1Universidad Autónoma del Estado de Hidalgo, Instituto de Ciencias Agropecuarias, Área Académica de Medicina Veterinaria y Zootecnia, México.
2Universidad Autónoma del Estado de Hidalgo, Instituto de Ciencias Agropecuaria, Área Académica de Ciencias Agrícolas y Forestales.
3Universidad Autónoma del Estado de Hidalgo, Instituto de Ciencias Agropecuarias. Área Académica de Agronegocios e Ingeniería en Alimentos.
Five concentrations (200 to 12.5 mg mL -1) of Kalanchoe daigremontiana hydroalcoholic extract, were used to determine its anthelmintic and antibacterial effect in vitro. To determine the anthelmintic effect, eggs hatching inhibition, inhibition of motility and larval mortality tests were performed Haemonchus contortus (HC). The determination of the Minimum Inhibitory Concentration and Minimum Bactericidal Concentration allowed to evaluate the antibacterial activity of extract on L. monocytogenes, S. typhi, P. aeruginosa, S. choleraesuis, B. subtilis, E. coli and S. aureus. Kalanchoe daigremontiana hydroalcoholic extract inhibited the 99.5% of HC eggs hatching and reduced the motility of 85.2% of L3 larvae at 400 mg mL -1. The lethal concentrations 50 and 90 for the inhibition of hatching were 66.5 and 87.3 mg mL -1 and 1.5 and 240.9 mg mL -1, for the inhibition of motility. The extract showed activity on Gram positive and Gram-negative bacteria, determining a MIC of 100 mg mL -1 on P. aeruginosa and L. monocytogenes and 0.781 mg mL -1 for B. subtilis and S. aureus. These results indicate that the hydroalcoholic extract of Kalanchoe daigremontiana has a potential anthelmintic and antibacterial effect and that it could be used as a biological control strategy.
Keywords: Kalanchoe daigremontiana; hydroalcoholic extract; anthelmintic; antibacterial
Cinco concentraciones (200 a 12.5 mg mL-1) del extracto hidroalcohólico de Kalanchoe daigremontiana fueron usadas para determinar su efecto antihelmíntico y antibacteriano in vitro. Para determinar el efecto antihelmíntico se realizaron las pruebas de inhibición de la eclosión, inhibición de la motilidad y mortalidad larvaria sobre Haemonchus contortus (HC). La determinación de la Concentración Mínima Inhibitoria y Concentración Mínima Bactericida, permitieron evaluar la actividad antibacteriana del extracto sobre L. monocytogenes, S. typhi, P. aeruginosa, S. choleraesuis, B. subtilis, E. coli and S. aureus. El extracto hidroalcohólico de Kalanchoe daigremontiana a 400 mg mL-1 inhibió la eclosión de huevos de HC en un 99.5%, y redujo la motilidad del 85.2% de larvas L3 del mismo nematodo. Las concentraciones letales 50 y 90 para la inhibición de la eclosión fueron de 66.5 y 87.3 mg mL-1 y de 1.5 y 240.9 mg mL-1, para la inhibición de la motilidad. El extracto mostró actividad sobre bacterias Gram positivas y Gram negativas, determinándose una CMI de 100 mg mL−1 sobre P. aeruginosa y L. monocytogenes y 0.781 mg mL−1 para B. subtilis and S. aureus. Estos resultados indican que el extracto hidroalcohólico de Kalanchoe daigremontiana presenta potencial efecto antihelmíntico y antibacteriano y que podría ser utilizado como una estrategia de control biológico.
Palabras clave: Kalanchoe daigremontiana; extracto hidroalcohólico; antihelmíntico; antibacteriano
INTRODUCTION
Central Mexico is a well-known area of sheep breeding, mainly for the meat market. Meat yield and quality, and therefore the economic viability of the industry, depends on the health of the animals. Sheep production requires a continuous vigilance for infection by parasitic nematodes, since their presence impacts on meat productivity Alcala et al., (2016). Abomasal worms, especially Haemonchus contortus [barber’s pole worm; Nematoda: Strongylida] (Aguilar et al., 2016; Castillo et al., 2017) are the main nematodes causing gastrointestinal disease to sheep in Mexico. Several anthelmintic products have been used to address this problem, many of which have been reported to cause resistance (González et al., 2017). On the other hand, traditional medicine in veterinary, especially the use of plant extracts, has been proposed as an environmental-friendly alternative against this parasitic infection (Hernández et al., 2011; López et al., 2008; Abdelfatta et al., 2017).
The use of plants as anthelmintic agents is well documented. Among the species used for this purpose are Chenopodium album (Bashir et al., 2017), Digitaria insularis (Santos et al., 2017), Artemisa parviflora (Irum-S et al., 2017), Ziziphus jujube (Preet et al., 2017), Acacia cochliacantha Argemone mexicana, Taraxacum officinale, Ruta chalepensis, and Tagetes filifolia (Olmedo et al., 2017). Kalanchoe daigremontiana (also known as “mother of thousands”) is an endemic plant in Mexico (Kolodziejczyk et al., 2017) with several reported uses in human herbal medicine (Hamburger et al., 2017) and various active compounds have been found in the extracts of the leaves and stems of this plant in particular (Huang et al., 2013). There are reports on the use of K. daigremontiana as an antimicrobial agent. Some of the genera Kalanchoe isolated compounds and functions follow (Table 1). Therefore, this study was aimed to evaluate the anthelminthic and antibacterial capacity of a hydroalcoholic extract from K. daigremontiana.
Table 1 Insolated compounds and functions of some Kalanchoe genera plants
| Species | Isolated compounds | Function | Reference |
|---|---|---|---|
| Kalanchoe pinnata | KPB-100 and KPB-200 | inhibitors of HHV-2 and VACV | Cryer et al., 2017 |
| Kalanchoe pinnata | Bryophyllin C | Insecticidal | Supratman et al., 2000 |
| Kalanchoe daigremontiana×tubiflora | Methyl daigremonate | Insecticidal | Supratman et al., 2001 |
| Kalanchoe daigremontiana × butiflora | Bryophyllin A | Anti-tumor promoting activity | Supratman et al., 2001 |
| Kalanchoe prolifera | Kaempferol, Quercetin, Quercetin-3-O-β-D-glucopyranoside, Kaempferol-3-O-β-D-glucopyranoside, Kaempferol-3-O-α-L-rhamnoside , Quercetin-3-O-sophoriside, Quercetin-3-O-rutinoside | Citotoxic activity against leukimia cells | Aisyah et al., 2017 |
| Kalanchoe pinnata | Flavonoids in methanol extract | In vitro anti-diabetic activity | George et al., 2018 |
| Kalanchoe daigremontiana | 11α,19-dihydroxytelocinobufagin, bersaldegenin-1-acetate, bersaldegenin-1, 3,5-orthoacetate, 19-acetyloxy-11α-hydroxy-12-oxo-telocinobufagin, 19-acetyloxy-1β-hydroxytelocinobufagin | Antioxidant | Kolodziejczyk-Czepas et al., 2016 |
| Kalanchoe daigremontiana | Bufadienolides such as 11α,19-dihydroksytelocinobufagin, bersaldegenin-1-acetate, daigredorigenin-3-acetate, | Inhibition of amidolytic activity of thrombin | Kolodziejczyk-Czepas et al., 2017 |
| Kalanchoe daigremontiana | Bersaldegenin-1,3,5-orthoacetate | increasing apopthosis in deteriorated cells and promoting celular death | Stefanowicz-Hajduk et al., 2020 |
| Kalanchoe pinnata | Quercitrin | increasing apopthosis in deteriorated cells and promoting celular death | Muzitano et al., 2006 |
| Kalanchoe thrysiflora, Kalanchoe marmorata | 3-oxo-olean-12-ene, β-sitosterol | increasing apopthosis in deteriorated cells and promoting celular death | Singab et al., 2012 |
| Kalanchoe tubiflora | kalanchosine dimalate | Citotoxic activity | Huang et al., 2013 |
| Bryophyllum pinnatum | Bersaldegenin-1,3,5-orthoacetate | In Vitro enzymes inhibition activity, for modern pharmaceuticals | Prasad Pandey et al., 2020 |
MATERIALS AND METHODS
Plant material collection and species identification: K. daigremontiana specimens were collected in Ulapa de Melchor Ocampo, Tetepango, Hidalgo, in Central Mexico (latitude 20.142500, longitude −99.167778). Local inhabitants have traditionally used this plant as an herbal medication. Whole plants (roots, leaves, and stems) were collected phenological stage of flowering and prepared for transportation. Species identification was performed in the botany laboratory of the Institute of Biological Sciences of the Universidad Autónoma del Estado de Hidalgo. A representative voucher specimen of the plant material was deposited in the herbarium of the Institute of Biological Sciences of the Universidad Autónoma del Estado de Hidalgo, and the identification code 06 was assigned to it.
Extract preparation: One-hundred grams of dried leaves and steams (4-6 mm) were macerated with 3000 mL of extraction solvent (30% methanol, 70% water); after 72 h, the extract was separated from the solid residue using a filter paper (Whatman™ qualitative filter paper, grade 1), and the solvent was removed by distillation under reduced pressure in a BÜCHI™ R-210 (Flawil, Germany) rotary evaporator, following the methodology described by Rivero-Pérez et al., (2016). The concentrations evaluated for egg hatching and larval motility inhibition, as well as larval mortality, were 200, 100, 50, 25, and 12.5 mg mL−1. Dried extracts (35 g) were stored at −20 °C until used.
Anthelmintic activity
H. contortus (HC) eggs and L3-stage larvae were used to evaluate anthelmintic activity. Parasites of the strain INIFAP were obtained from the National Institute for Forestry, Animal and Agronomic Research (INIFAP).
Egg hatching test
HC eggs were obtained following a protocol approved by the Bioethics Committee of the Institute of Agricultural Sciences of the Universidad Autonoma del Estado de Hidalgo. Briefly, a Hampshire lamb (3-months and 37 kg PV), clinically healthy and free of gastrointestinal nematodes, was infested with HC L3-stage larvae (350 larvae kg−1 PV). Twenty-one days after infestation, fecal samples were collected and the number of eggs per gram of feces was determined by the McMaster method (Cordero-Miguel et al., 2000). To recover HC eggs, the methodology described by Olmedo et al., (2017) was followed. Thirty grams of feces were washed with distilled water in 200-, 100-, 75-, and 37-µm sieves and concentrated in the 37-µm sieve. The material retained in the last sieve was washed with 6 mL of saturated saline solution and centrifuged at 3000 rpm for 3 min. The supernatant was discarded, and the sediment was washed three times with distilled water to obtain free eggs.
A 96-well ELISA plate was used for the assay. Each well was added with 150-200 eggs in 50 µL of distilled water and 50 µL of extract (200, 100, 50, 25, or 12.5 mg mL−1). Each extract concentration was assayed with four replicates, using Ivermectin (5 mg mL−1) and distilled water as positive and negative controls, respectively. The plates were incubated at 30 °C for 48 h in a constant-humidity chamber. After incubation, ten 10-μL aliquots were observed under the microscope to count the number of unhatched eggs and larvae (dead or alive) per well. Finally, the percentage of egg hatching inhibition was calculated using the equation 1.
Larval mortality test
Feces from infested lambs were mixed with distilled water and polyurethane foam (1.5 × 1.5 × 0.5 cm) and incubated for 10 days at room temperature (15-20 °C). After incubation, HC L3-stage larvae were recovered following the Baermann technique. L3-stage larvae were unsheathed with 3% sodium hypochlorite (NaClO) for one minute and washed three times with distilled water to remove residual NaClO.
The assay was performed in 96-well plates. Each well was added with 150-200 larvae suspended in 50 µL of water and 50 µL of K. daigremontiana extract (200, 100, 50, 25, or 12.5 mg mL−1). Each extract concentration was assayed with four replicates, using Ivermectin (5 mg mL−1) and distilled water as positive and negative controls, respectively.
The plates were incubated in a constant-humidity chamber at 30° C for 72 h. After incubation, ten 10-µL aliquots were observed under the microscope to determine the number of larvae alive or dead per well. Mortality rate for each extract concentration was determined using equation 2:
Larval motility test
For this assay, unsheathed L3-stage HC larvae were placed in 96-well plates. Each well was added with 150-200 larvae suspended in 50 µL of water and 50 µL of extract (200, 100, 50, 25, or 12.5 mg mL−1). Each extract concentration was assayed with four replicates, using Ivermectin (5 mg mL−1) and distilled water as positive and negative controls, respectively. The plates were incubated in a constant-humidity chamber at 30° C for 72 h. After incubation, 10-µL aliquots were observed under the microscope to determine the number of alive/dead, motile/immobile larvae per well. The rate of motility inhibition for each extract concentration was determined using equation 3:
Antibacterial activity
The microorganisms used to determine the antibacterial activity of the hydroalcoholic extract from K. daigremontiana were Staphylococcus aureus (ATCC 6538), Bacillus subtilis (ATCC 6633), Salmonella typhimurium (ATCC 14028), Pseudomonas aeruginosa (ATCC 9027), Listeria monocytogenes (ATCC 19113), and Escherichia coli (ATCC 35218).
The broth microdilution method described by Kaewpiboo et al., (2012) was used with some modifications to determine the minimal inhibitory concentration (MIC) of the K. daigremontiana hydroalcoholic extract. Two-fold serial dilutions of K. daigremontiana hydroalcoholic extract (from 400 to 0.781 mg mL−1) were prepared by duplicate (100 μL per well). A bacterial cell suspension was adjusted to 0.5 McFarland units (approximately 1.5 × 106 colony forming units [CFU] mL−1). A 10-μL aliquot was added to each well. Kanamycin (AppliChem 4K10421™) was used as a positive control (64-0.5 µg mL−1) and nutritive broth was used as a negative control. Plates were incubated at 37 °C under agitation (70 rpm) for 24 h.
After incubation, 20 μL of 0.04% (w/v) p-iodonitrotetrazolium solution was added to each well and incubated for 30 min. A change in color from yellow to pink indicated the reduction of the dye due to bacterial growth. The MIC was determined for each extract concentration as the lowest concentration at which no microbial growth was observed, as determined by the absence of color change (Figure 1).
Statistical analysis
Data were analyzed by one-way analysis of variance and the Tukey-Kramer post hoc test (α = 0.05). Concentrations that inhibited 50% (LC50) and 90% (LC90) of HC egg hatching and motility, as well as those that killed 50% and 90% of larvae, were calculated by a PROBIT analysis using the statistical package SAS 9.0.
RESULTS AND DISCUSSION
Anthelmintic activity
The mean efficacy of the hydroalcoholic extract from K. daigremontiana against HC is shown in Table 2. A significantly different egg hatching inhibition rate (EHI%) with respect to positive and negative controls (P < 0.0001) was found in the range 100-200 mg mL−1 (99.5%). On the other hand, mortality (MOR%) was also significantly different with respect to controls (P < 0.0001), being the highest MOR% values observed at 50 and 25 mg mL−1 (16.4 and 14.5%, respectively). Finally, significant differences were found among treatments in terms of motility inhibition (IMOT%). The highest IMOT% value was observed at 200 and 100 mg mL−1 (85.2 % and 73.1 %, respectively).
As shown in Figures 1 and 2, the LC50 and LC90 values for egg hatching were 66.5 and 87.3, and 1.5 and 240.9 for motility inhibition in HC L3-stage larvae.
Figure 2 Lethal concentration (LC50 and LC90) of Kalanchoe daigremontiana hydroalcoholic extract to inhibit motility in Haemonchus contortus L3-stage larvae
Table 2 Mean efficacy (percentage ± Standard Deviation) of the hydroalcoholic extract from Kalanchoe daigremontiana on H. contortus
| Treatment (mg mL−1) | EHI%±SD | IMOT%±SD | MOR%±SD |
|---|---|---|---|
| Water | 3.7±0.4c | 0e | 2.8±1.3cd |
| KD (200) | 99.5±0.94a | 85.2±4.2b | 6.9±3.1c |
| KD (100) | 99.5±0.95a | 73.1±5.3c | 13.5±2.6b |
| KD (50) | 10.1±0.88b | 64.8±5.7cd | 16.4±1.8b |
| KD (25) | 4.7±0.29c | 63.0±3.5d | 14.5±2.2b |
| KD (12.5) | 3.6±0.30 c | 59.5±2.1d | 13.5±1.1b |
| Ivermectin 5 | 100a | 100a | 100a |
| SEM | 0.019 | 0.147 | 0.061 |
| P-value | < 0.0001 | < 0.0001 | < 0.0001 |
KD: Kalanchoe daigremontiana hydroalcoholic extract. EHI: egg hatching inhibition. IMOT: motility inhibition. MOR: mortality. SEM: standard error of the mean. For each column, different letters indicate significant differences (α = 0.05, Tukey test).
Antibacterial activity
As shown in Table 3, K. daigremontiana hydroalcoholic extract showed antibacterial activity against both Gram-negative (P. aeruginosa) and Gram-positive (L. monocytogenes, B. subtilis, and S. aureus) bacteria. The MIC was 100 mg mL−1 for P. aeruginosa and L. monocytogenes and 0.781 mg mL−1 against B. subtilis and S. aureus.
Table 3 The minimal inhibitory concentration of Kalanchoe daigremontiana hydroalcoholic extract on the Gram (+) and Gram (−) bacteria
| Bacterial | Minimal inhibitory concentration (MIC)KD mg mL−1 | Kanamycin µg mL−1 | Water |
|---|---|---|---|
| E. coli | NA | 4 | NA |
| S. typhimurium | NA | 4 | NA |
| S. choleraesuis | NA | 1 | NA |
| P. aeruginosa | 100 b | 64 | NA |
| L. monocytogenes | 100 b | 2 | NA |
| B. subtilis | 0.781a | 8 | NA |
| S. aureus | 0.781a | 64 | NA |
KD: Kalanchoe daigremontiana hydroalcoholic extract. NA: No activity. Different literals a,b in the column indicate significant statistical differences (P≤0.05)
Our results suggest that the K. daigremontiana hydroalcoholic extract has a significant activity against H. contortus egg hatching in vitro (Figure 1). The activity of the extract was as good as that of the positive control (Ivermectin 5 mg mL−1), indicating the feasibility of using this plant species as an anthelmintic agent. Since no significant differences were found between 100 and 200 mg mL−1 treatments, the lowest dose could be used to reduce the risk of nematode resistance to the drug. Interestingly, death was not the main effect of the extract, but motility inhibition.
K. daigremontiana hydroalcoholic extract is capable of inhibiting egg hatching and larval motility (Figure 2). Other plant-derived molecules, like flavonoids, flavones, saponins, alkaloids, xanthones (Rivero et al., 2016), polyphenols (Akkari et al., 2016), tannins (Desrues et al., 2016) and pyrazole-5-carboxamide derivatives (Jiao et al., 2017), have also been reported to reduce larval motility. The presence in K. daigremontiana of flavonoids and polyphenols (Karwatzki et al., 1993) has been reported, and it is feasible that these compounds play a role in larval motility inhibition.
Our results show that the K. daigremontiana hydroalcoholic extract inhibits the motility of HC L3-stage larvae but are not effective in killing them. This could be relevant for the proposed use of K. daigremontiana extracts as an anthelmintic, since (Moradpour et al., 2013) have described the morphological changes in abomasal tissues due to parasite migration to different parts of sheep abomasa. The results of anthelmintic activity herein reported are similar to those observed by Phatak (2013), who did not find any activity in methanolic and petroleum-ether extracts from Kalanchoe pinnata on larval survival; however, the extracts reduced larval motility Unlike that study, however, we also evaluated egg hatch inhibition, finding that 99.5% of eggs did not hatch when exposed to 100 and 200 mg mL−1 of the extract, with an LC50 of 66.5 mg mL−1 and an LC90 of 87.3 mg mL−1.According to Lunkad et al., (2016), extracts of species of the subgenus Bryophyllum, such as B. pinnatum, showed anthelmintic activity in various concentrations (30 and 50 mg/ml) against Indian earthworms Pheretima posthuman, counting as antihelmintic activity the paralisis and death of more than 50% of the organisms.
A possible action mechanism of plant secondary metabolites on the eggs and larvae of nematodes like H. contortus involves the inhibition or delay of parasite growth and maturation by the affinity of glycoproteins in the cuticle of the parasite to phenolic compounds (mediated by proline residues); polyphenols may bind these proteins, inhibiting parasite motility, feeding, and reproduction, eventually causing their death; additionally, saponins have membranolytic actions (Hernández et al., 2018; Irshad et al., 2010).
With respect to antibacterial activity, K. daigremontiana hydroalcoholic extract showed a higher activity on gram-positive than on gram-negative bacteria; this could be explained considering that gram-negative bacteria have a phospholipidic outer membrane and porins; the phospholipidic membrane that covers structural lipopolysaccharide components make the cell wall impermeable to lipophilic solutes.
Mothana et al., (2009) evaluated 25 plants with antibacterial activity, including Kalanchoe farinacea. The methanolic extract of this plant had inhibitory activity on S. aureus, B. subtilis, and multi-resistant Staphylococcus epidermidis and S. aureus at a concentration of 4 mg mL−1, producing 15- and 16-mm inhibition zones on S. aureus and multi-resistant S. epidermidis and S. aureus cultures, respectively, and 10-mm inhibition zones on B. subtilis cultures, but had no effect against gram-negative bacteria.
Dichloromethane extracts from K. pinnata leaves produced 18-mm inhibition zones when assayed against E. coli, but had no effect on S. aureus nor P. aeruginosa. Those results are in partial agreement with those herein reported. K. daigremontiana hydroalcoholic extract had no effect on E. coli, but was effective against P. aeruginosa, with a MIC of 100 mg mL−1. The same study reported that the methanolic extract contained saponins, cardiac glycosides, and steroids as secondary metabolites with possible antibacterial activity.
Richwagen et al., (2019) reported antibacterial activity of extracts from two Kalanchoe species, K. mortagei and K. fedtschenkoi, against ESKAPE pathogens (Enterococcus faecium, Staphylococcus aureus, Klebsiella pneumoniae, Acinetobacter baumannii, Pseudomonas aeruginosa and Enterobacter cloacae). Growth inhibition greater than 50% (IC50) was generally observed at concentrations of 256 μg mL-1 and 128 μg mL-1.
De Souza Barboza et al., (2016), corroborated antimicrobial activity of aqueous extracts of leaves and flavonoids occurring in Kalanchoe pinnata (Lam.), concentrations of 100 μg.mL-1, showed a growth reduction higher than 50% for Pseudomonas aeruginosa and Citrobacter freundii.
Akinnibosun et al., (1994) reported that an ethanolic extract from K. pinnata leaves was more effective against S. aureus, E. coli, and P. aeruginosa than aqueous and methanolic extracts of the same plant, showing inhibition zones of 17.3 ± 1.2, 12.7 ± 0.9, and 8.3 ± 0.9 mm for S. aureus, E. coli, and P. aeruginosa, respectively. A qualitative chemical analysis of the ethanolic extract detected flavonoids, steroids, alkaloids, tannins, cardiac glycosides, and reducing sugars, along with secondary metabolites with reported antimicrobial activity, mainly saponins and phenolic compounds like tannins.
CONCLUSION
The present study shows the potential anthelmintic and antibacterial effect of Kalanchoe daigremontiana hydroalcoholic extract, against Haemonchus contortus, Gram-negative and Gram-positive bacteria, showing the best effect over eggs hatching inhibition and larval motility of Haemonchus contortus and on the growth of B. subtilis and S. aureus. These results indicate that Kalanchoe daigremontiana hydroalcoholic extract can be used as alternative natural for control or treatment of diseases associated with these microorganisms. Although the identification of the secondary metabolites associated with these biological activities is necessary, as well in vitro and in vivo toxicity tests.
REFERENCES
Abdelfatta S, Elghandour M, Kholif A, López S, Pliego A, Cipriano-Salazar M, Alonso M. 2017. Tree leaves of Salix babylonica extract as a natural anthelmintic for smallruminant farms in a semiarid region in Mexico. Agroforestry Systems. 91(1):111-122. ISSN: 1572-9680. https://doi.org/10.1007/s10457-016-9909-z [ Links ]
Aguilar-Marcelino L, Mendoza-De-Give P, Torres-Hernández G, López-Arellano M, Becerril-Pérez C, Orihuela-Trujillo A, Olmedo-Juárez A. 2016. Consumption of nutritional pellets with Duddingtonia flagrans fungal chlamydospores reduces infective nematode larvae of Haemonchus contortus in faeces of Saint Croix lambs. Journal Helminthology. 91(6): 665-671. ISSN: 1475-2697. https://doi.org/10.1017/S0022149X1600081X [ Links ]
Akinnibosun FI, Eedionwe O. 1994. Evaluation of the phytochemical and antimicrobial potential of the leaves extracts of Bryophyllum pinnatum L. and Citrus aurantifolia Sw and their synergy. Journal of Applied Sciences and Environmental Management. 4:611-619. ISSN: 2659-1502. http://dx.doi.org/10.4314/jasem.v19i4.7 [ Links ]
Alcala-Canto Y, Camberos L, López H, Olvera L, Pérez G. 2016 Anthelmintic resistance status of gastrointestinal nematodes of sheep to the single or combined administration of benzimidazoles and closantel in three localities in Mexico. Veterinaria México. 3(4). ISSN: 2448-6760. https://doi.org/10.21753/vmoa.3.4.374 [ Links ]
Aisyah ls, Yun YF, Herlina T, Julaeha E, Zainuddin A, Nurfarida I, Shiono Y. 2017. Flavonoid compounds from the leaves of Kalanchoe prolifera and their cytotoxic activity against P-388 murine leukimia cells. Natural Product Sciences. 23(2):139-145. ISSN: 2288-9027. https://doi.org/10.20307/nps.2017.23.2.139 [ Links ]
Akkari h, Hajaji S, B'Chir F, Rekik M, Gharbi M. 2016. Correlation of polyphenolic content with radical-scavenging capacity and anthelmintic effects of Rubus ulmifolius (Rosaceae) against Haemonchus contortus. Veterinary Parasitology. 221:46-53. ISSN: 0304-4017. https://doi.org/10.1016/j.vetpar.2016.03.007 [ Links ]
Bashir L, Chishti M, Bhat F, Tak H, Bandh S, Khan A. 2017. Evaluation of anthelmintic antimicrobial and antioxidant activity of Chenopodium album. Tropical Animal Health and Production. 49(8):1597-1605. ISSN: 1573-7438. https://doi.org/10.1007/s11250-0171364-y [ Links ]
Castillo-Mitre G, Olmedo-Juárez A, Rojo-Rubio R, González-Cortázar M, Mendozade Givesh P, Hernández-Beteta E, Zamilpa A. 2017. Caffeoyl and coumaroyl derivatives from Acacia cochliacantha exhibit ovicidal activity against Haemonchus contortus. Journal of Ethnopharmacology. 204: 125-131. ISSN: 0378-8741. https://doi.org/10.1016/j.jep.2017.04.010 [ Links ]
Cordero CM, Rojo A, Hernández R, Calvalho V. Parasitología Veterinaria. Barcelona, España. Editorial McGraw-Hill Interamericana. 2000.ISBN: 84-486-0236-6 https://dialnet.unirioja.es/servlet/libro?codigo=489596 [ Links ]
Cryr M, Lane K, Greer M, Cates R, Burt S, Andrus M, Johnson FB. 2017. Isolation and identification of compounds from Kalanchoe pinnata having human alphaherpesvirus and vaccinia virus antiviral activity. Pharmaceutical biology. 55(1):1586-1591. PMID: 28395583. https://doi.org/10.1080/13880209.2017.1310907 [ Links ]
De Souza Barboza TJE, Ferreira AEF, Ignacio ACDPR, Albarello N. 2016. Cytotoxic, antibacterial and antibiofilm activities of aqueous extracts of leaves and flavonoids occurring in Kalanchoe pinnata (Lam.) Pers. Journal of Medicinal Plants Research. 10(41):763-770. https://doi.org/10.5897/JMPR2016.6260 [ Links ]
George LO, Radha HR, Somasekariah BV. 2018. In vitro anti-diabetic activity and GCMS analysis of bioactive compounds present in the methanol extract of Kalanchoe pinnata. Indian Journal of Chemistry. 57: 1213-1221. https://api.semanticscholar.org/CorpusID:91497628 [ Links ]
Hernández-Alvarado J, Zaragoza-Bastida A, López-Rodríguez G, Peláez-Acero A, Olmedo-Juárez A, Rivero-Pérez N. 2018. Antibacterial and antihelmintic activity of plant secondary metabolites: approach in Veterinary Medicine. Abanico Veterinario. 8:14-27. ISSN: 2448-6132. https://doi.org/10.21929/abavet2018.81.1 [ Links ]
Hernández-Villegas M, Borges-Argaez R, Rodríguez-Vivas R, Torres-Acosta J, Méndez-González M, Cáceres-Farfán M. 2011. Ovicidal and larvicidal activity of the crude extracts from Phytolacca icosandra against Haemonchus contortus. Veterinary Parasitology. 179(1-3):100-106. ISSN: 0304-4017. https://doi.org/10.1016/j.vetpar.2011.02.019 [ Links ]
Huang HC, Lin MK, Yang HL, Hseu YC, Liaw CC, Tseng YH, Kuo YH. 2013. Cardenolides and bufadienolide glycosides from Kalanchoe tubiflora and evaluation of cytotoxicity. Planta Medica. 79(14):1362-1369. ISSN: 0032-0943. https://doi.org/10.1055/s-0033-1350646 [ Links ]
Irshad M, Man S, Rizvi MA. 2010. Assessment of anthelmintic activity of Cassia fistula L. Middle East Journal of Scientific Research. 5(5):346-349. IISSN:1999-8147. http://www.idosi.org/mejsr/mejsr5(5)/5.pdf [ Links ]
Jiao YQ, Preston S, Song HJ, Jabbar A, Liu YX, Baell J, Gasser RB. 2017. Assessing the anthelmintic activity of pyrazole-5-carboxamide derivatives against Haemonchus contortus. Parasit Vectors. 10:214-234. ISSN: 1756-3305. https://doi.org/10.1186/s13071-017-2191-8 [ Links ]
Karwatzki B, Herget A, Beerhues L, Wiermann R. 1993. In-situ localization of chalcone synthase in tannin-containing plants. Phytochemistry. 32(3):585. ISSN: 00319422. https://doi.org/10.1016/S0031-9422(00)95141-0 [ Links ]
Kolodziejczyk-Czepas J, Stochmal A. 2017. Bufadienolides of Kalanchoe species: an overview of chemical structure, biological activity and prospects for pharmacological use. Phytochemistry Reviews. 16(6):1155-1171. ISSN: 1572-980X. https://dx.doi.org/10.1007%2Fs11101-017-9525-1 [ Links ]
Kolodziejczyk-Czepas J, Nowak P, Wachowicz B, Piechocka J, Głowacki R, Moniuszko-Szajwaj B, Stochmal A. 2016. Antioxidant efficacy of Kalanchoe daigremontiana bufadienolide-rich fraction in blood plasma in vitro. Pharmaceutical biology. 54(12): 3182-3188. PMID: 27488985. https://doi.org/10.1080/13880209.2016.1214740 [ Links ]
López-Aroche U, Salinas-Sánchez D, de Gives P, López-Arellano M, LiebanoHernández E, Valladares-Cisneros G, Hernandez-Velázquez V. 2008. In vitro nematicidal effects of medicinal plants from the Sierra de Huautla, Biosphere Reserve, Morelos, México against Haemonchus contortus infective larvae. Journal of Helminthology. 82(1):25-31. ISSN:1475-2697 https://doi.org/10.1017/S0022149X07873627 [ Links ]
Lunkad AS, Agrawal MR, Kothawade SN. 2016. Anthelmintic activity of Bryophyllum pinnatum. Research Journal of Pharmacognosy and Phytochemistry. 8(1):21-24. https://doi.org/10.5958/0975-4385.2016.00005.4 [ Links ]
Mothana R, Lindequist U, Gruenert R, Bednarski JP. 2009. Studies of the in vitro anticancer, antimicrobial and antioxidant potentials of selected Yemeni medicinal plants from the island Soqotra. BMC Complementary Medicine and Therapies. 9:7. ISSN: 26627671. https://doi.org/10.1186/1472-6882-9-7 [ Links ]
Moradpour N, Borji H, Razmi G, Maleki M, Kazemi H. 2013. Pathophysiology of Marshallagia marshalli in experimentally infected lambs. Parasitology. ISSN: 1469-8161 140(14):1762-1767. https://doi.org/10.1017/s0031182013001042 [ Links ]
Muzitano MF, Tinoco LW, Guette C, Kaiser CR, Rossi-Bergmann B, Costa SS. 2006. The antileishmanial activity assessment of unusual flavonoids from Kalanchoe pinnata. Phytochemistry. 67(18): 2071-2077. PMID: 16930642. https://doi.org/10.1016/j.phytochem.2006.06.027 [ Links ]
Olmedo-Juárez A, Rojo-Rubio R, Zamilpa A, de Gives PM, Arece-García J, LópezArellano ME, von Son-de Fernex E. 2017. In vitro larvicidal effect of a hydroalcoholic extract from Acacia cochliacantha leaf against ruminant parasitic nematodes. Veterinary Research Communications. 41 (3):227-232. ISSN :1573-7446. https://doi.org/10.1007/s11259-017-9687-8 [ Links ]
Phatak RS. 2016. Lack of anthelmintic activity of Kalanchoe pinnata fresh leaves. Journal of Pharmaceutical Negative Results. 7(1):21. ISSN: 2229-7723. https://www.pnrjournal.com/fulltext/219-1599738067.pdf?1623436039 [ Links ]
Prasad PB, Prakash S, Adhikari K. 2020. LC ESI QTOF MS for the Profiling of the Metabolites and in Vitro Enzymes Inhibition Activity of Bryophyllum pinnatum and Oxalis corniculata Collected from Ramechhap District of Nepal. Chemistry & biodiversity. 17(6): e2000155. https://doi.org/10.1002/cbdv.202000155 [ Links ]
Preet S, Tomar R. 2017. Anthelmintic effect of biofabricated silver nanoparticles using Ziziphus jujuba leaf extract on nutritional status of Haemonchus contortus. Small Ruminant Research. 154:45-51. ISSN: 0921-4488. https://doi.org/10.1016/j.smallrumres.2017.07.002 [ Links ]
Richwagen N, Lyles JT, Dale BL, Quave CL. 2019. Antibacterial activity of Kalanchoe mortagei and K. fedtschenkoi against ESKAPE pathogens. Frontiers in pharmacology, 10, 67. https://doi.org/10.3389/fphar.2019.00067 [ Links ]
Rivero-Pérez N, Ayala-Martinez M, Zepeda-Bastida A, Meneses-Mayo M, OjedaRamirez D. 2016. Anti-inflammatory effect of aqueous extracts of spent Pleurotus ostreatus substrates in mouse ears treated with 12-O-tetradecanoylphorbol-13-acetate. The Indian Journal of Pharmacology. 48:141-144. ISSN: 0253-7613. https://ijp-online.com/article.asp?issn=0253-7613;year=2016;volume=48;issue=2;spage=141;epage=144;aulast=RiveroPerez;type=0 [ Links ]
Santos FO, de Lima HG, Santos N, Serra T, Uzeda RS, Reis IMA. 2017. Batatinha, MJM. In vitro anthelmintic and cytotoxicity activities the Digitaria insularis (Poaceae). Veterinary Parasitology. 245:48-54. ISSN:0304-4017. https://doi.org/10.1016/j.vetpar.2017.08.007. [ Links ]
Sanos S, Zurfluh L, Mennet M, Potterat O, Von Mandach U, Hamburger M, SimõesWüst, AP. 2021. Bryophyllum pinnatum Compounds Inhibit Oxytocin-Induced Signaling Pathways in Human Myometrial Cells. Frontiers in Pharmacology.12:142. https://doi.org/10.3389/fphar.2021.632986 [ Links ]
Singab AB, El-Ahamdy SH, Labib RM, Fekry SS. Kalanchoe thrysiflora Harv. And Kalanchoe marmorata Baker; DNA Profiling, biological guided fractionation of different extracts; isolation and identification of cytotoxic compounds. 2012. Journal of Applied Pharmaceutical Science. 02 (08): 215-220. ISSN: 2231-3354. http://japsonline.com/admin/php/uploads/652_pdf.pdf [ Links ]
Supratman U, Fujita T, Akiyama K, Hayashi H. 2000. New insecticidal bufadienolide, bryophyllin C, from Kalanchoe pinnata. Bioscience, biotechnology, and biochemistry. 64(6): 1310-1312. PMID: 10923811. https://doi.org/10.1271/bbb.64.1310 [ Links ]
Supratman, U, Fujita T, Akiyama K, Hayashi H. 2001. Insecticidal compounds from Kalanchoe daigremontiana× tubiflora. Phytochemistry. 58(2): 311-314. PMID: 11551556 https://doi.org/10.1016/S0031-9422(01)00199-6 [ Links ]
Supratman U, Fujita T, Akiyama K, Hayashi H, Murakami A, Sakai H, Ohigashi H. 2001. Anti-tumor Promoting Activity of Bufadienolides from Kalanchoe pinnata and K. daigremontiana× butiflora. Bioscience, biotechnology, and biochemistry. 65(4): 947-949. PMID: 11388478. https://doi.org/10.1271/bbb.65.947 [ Links ]
Stefanowicz-Hajduk J, Asztemborska M, Krauze-Baranowska M, Godlewska S, Gucwa M, Moniuszko-Szajwaj B, Ochocka JR. 2020. Identification of flavonoids and bufadienolides and cytotoxic effects of Kalanchoe daigremontiana extracts on human cancer cell lines. Planta medica. 86(04): 239-246. PMID: 31994149. https://doi.org/10.1055/a-1099-9786 [ Links ]
Stefanowicz-Hajduk J, Hering A, Gucwa M, Hałasa R, Soluch A, Kowalczyk M, Ochocka R. 2020. Biological activities of leaf extracts from selected Kalanchoe species and their relationship with bufadienolides content. Pharmaceutical Biology. 58(1):732-740. PMID: 32715869. https://doi.org/10.1080/13880209.2020.1795208 [ Links ]
Xing LZ, Ni HJ, Wang L. 2017. Quercitrin attenuates osteoporosis in ovariectomized rats by regulating mitogen-activated protein kinase (MAPK) signaling pathways. Biomedicine & Pharmacotherapy: 89: 1136-1141. PMID: 28314242. https://doi.org/10.1016/j.biopha.2017.02.073 [ Links ]
Received: February 10, 2021; Accepted: December 13, 2021
Este es un artículo publicado en acceso abierto bajo una licencia Creative Commons
