In the wake of antibiotic resistance, treatment of intractable wound have been very challenging and any alternative treatment which may lead to less use of antibiotics deserves further exploitation. Nanoparticle conjugates has potentially not only reduce antibiotic use but it has been considered safe and effectively disinfect wounds already colonized with resistant bacteria as well as promoting granulation tissue formation. In this study, Iodine-doped silver nanoparticle Ointment (Ag-I NPs) was investigated for its toxicological effect on excisional wound of albino rats.
Methods
Aqueous extraction of Piper guineense leaf was carried out and used for the synthesis of Ag-I NPs. The synthesized Ag-I NPs were characterized by Ultraviolet visible spectrophotometer which confirmed the availability of silver nanoparticles. The particles were then used to prepare a wound healing ointment for treating excision wound inflicted on wistar rat model. Blood samples, liver and kidney biopsies were collected on the 21st day of the experiment from all the rats for hematology, biochemical and histopathological analysis.
Result
In the hematological and biochemical analysis, hemoglobin (Hb), packed cell volume (PCV) and mean corpuscular hemoglobin (MCH), superoxide dismutase (SOD), alkaline phosphatase (ALP) of experimental rats treated with Ag-I NPs were significantly different (p < 0.05) compared to the untreated group. In the histopathology, the photomicrograph of the liver showed the normal control, PEG, Ag-NP, and Ag-I NP groups remained intact displaying distinctive histo-morphological appearance and stable cell density while the untreated (UTD) group showed fatty liver and reduced cellular density. The kidney photomicrograph of the normal control and Ag- I NP groups were present with intact renal corpuscles while the other photomicrographs displayed corpuscular degeneration marked by the large halo-spaced bowman space.
Conclusion
Silver nanoparticles (Ag NPs) and iodine-doped silver nanoparticle (Ag-I NP) altered haematological parameters in the rats and also influenced some biochemical changes in the serum of the rats. While in the histopathological study, the antioxidant present in the plant extract used to synthesize Ag NPs and Ag I-NPs may have functioned in synergy to maintain and preserve the integrity of the hepatocytes and renal corpuscles of the rats.
Hinweise
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Introduction
Wounds are an inevitable occurrence that arises during one’s lifetime. They are triggered by microbial infection, physical or chemical accident. Occasionally, wounds may emerge as severe or chronic. Chronic wounds are often accompanied with the failure of a patient to heal effectively and ascertain the origin or trigger of the attrition as normally seen in diabetes [1‐3].
Wound care is an increasingly important worldwide issue owing to the rising rate of metabolic diseases and their susceptibility to microscopic infections which increases public health issues and creating a huge medical, economic, social and psychological strain especially in third world nations [4‐6]. With an approximately 7.3 billion population globally, nearly 1 billion individuals are likely to experience acute and/or chronic wound in which poverty, bad sanitation, malnutrition and poisoning may possibly trigger or exacerbate their effects [7]. Wound healing is a complicated predefined cascade of well-orchestrated histology occurrences that evolves in alternating stages, (hemostasis, inflammation, cell proliferation/granulation and remodeling/maturation) revealed through a sequence of molecular, biochemical and behavioral phenomena, generally contributing to anatomical tissue reconstitution [8, 9].
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Iodine a dark non-metallic crystalline solid is probably the best known antiseptic and has been used for more than a century [10]. Iodine nanoparticles have been reported to be synthesized chemically using calcium lactate, disodium hydrogen phosphate, polyvinyl pyrolidone and iodine solution as precursor [11]. The use of plants for nanoparticle synthesis has advantages over chemical and other biological processes because it is cheap, non-toxic, eliminates the process of maintaining cell cultures and is suitable for large-scale nanoparticle synthesis [12].
P. guineense belongs to the plant family Piperaceae. It is a well-known good reducing agent utilized in gold nanoparticles synthesis [13]. It has been reported to possess antioxidant properties, aids in uterine contractions and antimicrobial activities [14, 15]. The seed and leaf of P. guineense have also been reported to contain flavonoids, cardiac glycosides, alkaloid, terpenes and tannins [16]. In this study, the aqueous leaf extract of P. guineense was used as a bio-reducing agent in the biosynthesis of iodine-doped silver nanoparticle wound ointment and its safety was investigated in experimental rats.
Materials and methods
Plant preparation
Fresh leaves of P. guineense were collected from Oboloafor village in Enugu State, Nigeria. The plant was identified at in the Department of Plant Biology, Federal University of Technology Minna, Nigeria. The voucher number is FUT/PLB/Pip/025. The leaves were washed with distilled water and air dried at room temperature for 15 days to prevent the destruction of thermo labile constituents of the plant by direct sun rays. The dried leaves were pulverized into coarse powder, after which 5 g of the plant sample (P. guineense leaves) was weighed, add to 100 ml of sterile deionized water in conical flask, boiled for 5 min and filtered using a whatmann filter paper [13].
Biosynthesis of iodine-doped silver nanoparticle
Aqueous extract of P. guineense (10 ml) was added to 90 ml of aqueous solution of 1 mM AgNO3 and heated with stirrer at 70 °C for 60 min at pH 7. Then 50 ml of a 0.1 mM I2 aqueous solution was slowly dropped under magnetic stirring in 30-60 min and the solution was kept stirring continuously for 1 h to assure further reaction. Colour change was observed and the iodine-doped silver nanoparticle was collected and monitored with a UV-vis spectrophotometer (UV-1800 shimadzu) at the wavelength of 200-900 nm using a quartz cuvette [13].
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Preparation of wound healing ointment using Ag-I NPs
The ointment was prepared by dissolving 10 g of Polyethylene glycol (PEG) 3000 Mw in 30 ml of synthesized iodine-doped silver nanoparticles (Ag-I NPs) to stabilize it [17]. The mixture was poured into a plastic jars and stored in a cool dry place.
Experimental animals
Male and female albino wistar rats weighing between 176 ± 37.48 g were obtained from Niger State Polytechnic, Zungeru, Niger state. They were kept in cages at the School of life science’s animal housing unit, Federal University of Technology, Minna and allowed to acclimatize for 21 days with free access to feed and water ad-libitum.
Experimental design
The rats (24) were weighed and randomly assigned into six groups of four rats each. All rats were inflicted with wound except the normal control group.
Group 1: Normal control group
Group 2: treated with povidone iodine (standard drug)
Group 3: untreated group (Negative control)
Group 4: treated with poly ethylene glycol (PEG) alone
Group 5: treated with PEG + silver nanoparticles (Ag NPs)
Group 6: treated with PEG + iodine-doped silver nanoparticles (Ag-I NPs
Serum and liver collection
The method described by Yakubu et al., [18] was employed in the serum and liver collection. Formaldehyde was used to preserve harvested animal organs (liver and kidney) for histopathological examination.
Haematological studies
Automated hematologic analyzer (D&H 600 model), was used to determine Haemoglobin (Hb) count, packed cell volume (PCV), mean cell volume (MCV), Mean corpuscular haemoglobin (MCH), Mean corpuscular haemoglobin concentration (MCHC), red blood cells (RBC), platelet count (PLCx102), total white blood cells (TWBC), neutrophils, lymphocytes, monocytes, eosinophils, basophils and red cell distribution width (RDWC) by method described by Dacie and Lewis [19].
Biochemical analysis
Superoxide dismutase activity assay
Superoxide dismutase (SOD) activity was determined based on the ability of SOD to inhibit the auto-oxidation of epinephrine to adrenochrome at alkaline pH [20]. 25 μl of the supernatant obtained from the centrifuged liver homogenate was added to a mixture of 0.1 mM adrenaline in carbonate buffer (10.2) in a total volume of 1 ml and the formation of adrenochrome was measured at 295 nm.
Catalase activity assay
Catalase (CAT) was estimated by the method of Sinha et al., [21]. The reaction mixture 1.5 ml contained 1.0 ml of 0.01 M phosphate buffer (pH7.0) 0.1 ml of tissue homogenate and 0.4 ml of 2 M H2O2. The reaction was stopped by the addition of 2.0 ml dichromate-acetic acid reagent (5% potassium dichromate and glacial acetic acid were mixed in 1:3 ratio). Then the absorbance was measured at 530 nm.
Estimation of glutathione peroxidase (GPx)
Glutathione peroxidase (GPx) was measured by the method described by Rotruck et al., [22] Briefly, the reaction mixture contained 0.2 ml 0.4 M phosphate buffer (pH7.0), 0.1 ml 10 mM sodium azide, 0.2 ml tissue homogenized in 0.4 M phosphate buffer pH7.0. 0.2 ml tissue homogenized in 0.4 M, phosphate buffer, pH 7.0, 0.2 ml reduced glutathione, 0.1 ml 0.2 mM hydrogen peroxide. The contents were incubated for 10 min at 37 °C, 0.4 ml 10 % TCA was added to stop the reaction and centrifuged at 3200×g for 20 min. The supernatant was assayed for glutathione content using Ellman’s reagent (19.8 mg 5,5′-dithiobisnitrobenzoic acid [DTNB] in 100 ml 0.1 % sodium nitrate).
Assay of alkaline phosphatase (ALP)
The method described by Bassey et al. [23] as modified by Wright et al. [24] using Randox kits. In a cuvette, 10 μl of sample was mixed with 500 μl of the reagent. The initial absorbance was read at 405 nm, and subsequently over 3 min. The mean absorbance per minute was used in the calculation: ALP activity (IU/l) = 2742 × ΔA 405 nm/min; Where: 2742 = Extinction coefficient; ΔA 405 nm / min = change in absorbance per minute for the homogenate sample.
Assay of alanine transaminase (ALT) activity
The method described by IFCC [25] using Randox kits was used. 50 μl of the sample and 500 μl of the ALT reagent were mixed in a test tube, and the initial absorbance at 340 nm was read after 1 min. The timer was started simultaneously and further readings of the absorbance were taken after 1, 2, and 3 min. ALT activity (nm/min) = 1746 × ΔA 340 nm/min, ΔA 340 nm/min = change in absorbance per minute for the homogenate sample, 1746 = Extinction coefficient.
Assay of aspartate transaminase (AST) activity
The method described by IFCC [25] using Randox kits was used. 50 μl of the sample and 500 μl of the AST reagent were mixed in a test tube, and the initial absorbance at 340 nm was read after 1 min. The timer was started simultaneously and further readings of the absorbance were taken after 1, 2, and 3 min. AST activity (nm/min) = 1746 × ΔA 340 nm/min; ΔA 340 nm/min = change in absorbance per minute for the homogenate sample; 1746 = Extinction coefficient.
Total protein
Total protein concentration was determined according to the method of Lowry et al. [26].
In an alkaline medium, protein reacts with the copper in the Biuret reagent leading to an increase in absorbance due to formation of colored complex. Reagent (2.5 ml) and 0.05 ml serum sample were mixed. It was then incubated at room temperature for 10 min. The absorbance was read at 540 nm against reagent blank.
Statistical analysis
The analysis was performed using the SPSS statistical package for WINDOWS (version 21.0; SPSS Inc., Chicago). Results were subjected to analysis of variance (ANOVA) to determine their level of significance. Data were expressed as the mean ± standard error of mean. Values were considered statistically significant at p < 0.05 and non-significant at p < 0.05 difference.
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Result and discussion
Haematological studies
Examination of the volumes and structure of the blood cells serves a crucial role in the physiological and pathological condition of an animal [27]. The impact of 21 days treatment of excision wound with polyethylene glycol (PEG), silver nanoparticles (Ag NP) and iodine-doped silver nanoparticle (Ag-I NP) in haematological parameters of experimental animals is displayed on Table 1. The outcome indicates that TWBC decreases considerably (P < 0.05) in experimental animals treated with Ag-I NPs while lymphocyte, neutrophil, red blood cells (RBC), mean cell volume (MCV) and platelet count did not show any significant distinction (P > 0.05). Treatment with Ag-I NPs also produced significant decrease (P < 0.05) in Hb, PCV, MCH and MCHC, while the monocytes, eosinophils, basophils and red cell distribution width (RDWC) were significantly (P < 0.05) elevated. It is worthy of note in this research that wound surface application of Ag-I NPs can substantially change the normal range of hematological parameters either negatively or positively. Granulocytes are parts of the immune system that fight multicellular parasites, certain vertebrate diseases, influence allergy and respiratory related complications. Significant rise (P < 0.05) in eosinophil, monocyte and basophil improves the animal’s capacity to produce antibodies by phagocytosis, have a large degree of infection resistance and improved adaptability to local circumstances of the environment and disease [28].
Table 1
Effects of 21-days treatment of wound with PEG, Ag-NPs and Ag-INPs on haematological parameters of albino rats
Parameters
Control
Standard
Untreated
PEG
Ag NP
Ag-I NP
Hb (g/L)
10.95 ± 1.35bc
9.50 ± 0.00b
11.75 ± 1.05bc
13.35 ± 0.05c
13.50 ± 0.60c
4.95 ± 0.55a
PCV (%)
35.00 ± 3.00bc
30.00 ± 0.00b
37.00 ± 3.00bc
42.00 ± 2.00c
41.50 ± 1.50c
14.50 ± 1.50a
MCV (fL)
56.00 ± 2.00a
54.00 ± 1.00a
56.00 ± 2.00a
54.50 ± 2.50a
51.00 ± 0.00a
54.00 ± 0.00a
MCH (Pg)
15.50 ± 0.50b
17.00 ± 1.00b
16.00 ± 0.00b
17.00 ± 0.00b
13.00 ± 3.00ab
8.00 ± 2.00a
MCHC(g/dL)
28.00 ± 2.00b
31.00 ± 1.00b
30.00 ± 0.00b
31.50 ± 1.50b
26.00 ± 6.00b
13.50 ± 3.50a
RBC (× 1012/L)
7.25 ± 1.25ab
5.60 ± 0.30a
7.35 ± 0.55ab
7.75 ± 0.05ab
11.05 ± 1.95b
7.15 ± 2.45ab
PLC(× 109/L)
6.98 ± 0.00a
5.35 ± 0.00a
7.23 ± 0.00a
8.23 ± 6.50a
7.64 ± 3.40a
1.27 ± 9.28a
TWBC(× 109/L)
3.10 ± 0.00ab
5.25 ± 0.25bc
5.10 ± 1.10bc
5.60 ± 0.60c
10.20 ± 0.90d
2.65 ± 0.55a
Neu (%)
9.00 ± 1.00a
8.50 ± 0.50a
7.50 ± 0.50a
10.50 ± 0.50a
10.50 ± 3.50a
17.50 ± 12.50a
Lym (%)
75.00 ± 1.00a
72.00 ± 3.00a
70.50 ± 2.50a
75.50 ± 4.50a
80.50 ± 3.50a
52.00 ± 18.00a
MEB (%)
16.00 ± 2.00ab
19.50 ± 3.50ab
22.00 ± 2.00ab
14.00 ± 4.00a
9.00 ± 7.00a
30.50 ± 5.50b
RDWC (%)
15.30 ± 0.40a
15.85 ± 0.55a
16.15 ± 0.25ab
15.55 ± 0.85a
18.90 ± 0.60c
18.75 ± 1.35bc
Biochemical analysis Values are expressed in mean ± standard error of mean. Values with the same superscript across the row have no significant different at p < 0.05
Hb Haemoglobin count, PCV packed cell volume, MCV mean cell volume, MCH Mean corpuscular haemoglobin, MCHC Mean corpuscular haemoglobin concentration, RBC red blood cells, PLCx102 platelet count, TWBC total white blood cells, Neu neutrophils, Lym lymphocytes, MEB monocytes, eosinophils, basophils and RDWC red cell distribution width
Mean cell volume (MCV), haematocrit and haemoglobin are reported to be major indicators for the assessment of erythrocytes, anemia detection and red blood cell (RBC) production in the bone marrow of mammals [29, 30]. The non-significant impact of Ag-I NPs on the RBC maybe a sign of erythropoiesis or depressed RBC production and it also indicates that Ag-I NPs could have the ability to prevent the discharge of erythropoietin in the kidney, which is RBC production’s humoral regulator [31]. The significant impact of Ag-I NPs on hematocrit, MCH and haemoglobin, may suggest that the blood oxygen-carrying potential and the quantity of oxygen supplied to the tissues after the administration of Ag-I NPs was altered as hematocrit and haemoglobin are very essential in the transfer of respiratory substances [32]. The observed decrease in MCHC maybe sign of swollen erythrocytes which indicate that P. guineense extract is likely poisonous to MCHC and other RBC lineage. The platelets in the rats treated with Ag-I NPs were similar with the control and did not trigger any adverse effects on the blood component platelets population.
Reactive oxygen species are known to mediate cellular damage. Anti-oxidants enzymes such as superoxide dismutase (SOD), glutathione peroxidase (GPx), and catalase play crucial roles in removing reactive oxygen species (ROS) released during metabolic processes [33, 34]. NADPH oxidase (NOX2) is produced at elevated concentrations in inflammatory cell plasma membranes and enabled during phagocytosis, resulting in large amounts of superoxide radical anions being produced which attack invasive pathogens, ultimately destroying them to help with phagocytosis [35, 36]. However, when superoxide is secreted in high amount, it affects the neighboring tissues and it is either dis-mutated by superoxide dismutase (SOD) or a spontaneous reaction to O2 and H2O2. The H2O2 is further converted into water by catalase or by glutathione peroxidase (GPx). In this study, the activities of SOD were considerably greater (p < 0.05) after 21 days of Ag NP and Ag-I NPs wound surface treatment when compared to the control group. The comparison of the anti-oxidants enzymes is shown in Table 2. This suggests that Ag NPs improved the secretion of SOD and prevented the harmful effects of superoxide radicals generated in the rats. Antioxidant properties contained in natural or synthetic products are known to have potentials to reduce the harmful effects caused by oxidative stress [37].
Table 2
Effects of 21 days treatment of wound with PEG, Ag-np and Ag-INP on antioxidant enzymes of albino rats
Enzymes
Control
Standard
Untreated
PEG
Ag NP
Ag-I NP
SOD U/mL
1.06 ± 0.13a
2.26 ± 0.26bc
2.53 ± 0.13c
1.86 ± 0.35b
4.00 ± 0.00d
2.00 ± 0.00bc
GPx μg/mL
1.07 ± 0.22a
0.81 ± 0.11a
1.12 ± 0.12a
1.07 ± 0.19a
1.86 ± 0.02b
1.14 ± 0.28a
CAT U/mL
0.65 ± 0.03b
0.70 ± 0.01b
0.69 ± 0.05b
0.65 ± 0.04ab
0.55 ± 0.01a
0.62 ± 0.01ab
Values are expressed in mean ± standard error of mean. Values with the same superscript across the row have no significant different at p < 0.05. SOD Superoxide dismutase, GPx glutathione peroxidase and CAT catalase
The activity of GPx in Ag NPs group was significantly increased compared with control group. While CAT activity, revealed a non-significant distinction after treatment with Ag NPs and Ag-I NPs. The increase in GPx activity may have occurred in response to boost immunity of the animals or a complementary mechanism to support the elimination of free radicals from the system [38]. Ag NPs may have enhanced GPx to suppressed oxidative stress in-vivo by maintaining hydrogen peroxide at a low level and modulating mechanisms involved in wound healing process such as blood clotting, thrombosis, angiogenesis, migration and fibrosis [39].
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The assessment of serum biochemical indicators in experimental animals has become an invaluable technique for evaluating the clinical signs and functionality of organs as well as pathology and overall wellness status [40]. Alkaline phosphatase is frequently used to evaluate plasma membrane and endoplasmic reticulum integrity. The rise (p < 0.05) in ALP activity after 21 days of Ag NP and Ag-I NPs wound repair proposed that the functionality and structure of the endoplasmic reticulum and plasma membrane were compromised [41]. It also indicated that the nanoparticles prevented or stimulated the enzyme operations [42].
Aspartate transaminase (AST) and alanine transaminase (ALT) are hepatic tissue biomarkers that catalyze transamination reaction and used to evaluate the extent of hepatocellular damage. But the ALT activities provide more useful data relevant to hepatocyte integrity than the AST [43‐45]. In this research, serum AST activities were significantly (p < 0.05) reduced while the levels of ALT were not significantly altered by Ag NP and Ag-I NP treatment relative to the control groups after 21 days treatment (Table 3). Similarly, AST activities reduced significantly in rats serum treated with colloidal AgNPs for 7 and 14 days [46]. The alterations observed in the levels of AST may have been initiated by the ability of AgNPs and Ag-INPs to disrupt the activities of the transaminase enzymes required for their optimal operations [47, 48]. Ag NP and Ag-I NP may have influenced transaminases selectively as there was no alteration of ALT operations in the animal serum.
Table 3
Effects of 21-days treatment of wound with PEG, Ag NP and Ag-I NP on liver function enzymes of albino rats
E
Control
Standard
Untreated
PEG
Ag NP
Ag-I NP
TP (g/dl)
79.17 ± 1.27c
81.70 ± 3.96c
81.70 ± 5.48c
84.23 ± 3.85c
52.57 ± 0.63a
67.87 ± 0.53b
AST(U/L)
24.50 ± 0.00cd
23.33 ± 1.16cd
25.83 ± 2.42d
11.67 ± 1.17a
17.50 ± 0.00b
21.00 ± 0.00bc
ALT(U/L)
8.15 ± 0.63a
8.15 ± 0.63a
6.69 ± 2.71a
7.52 ± 1.09a
8.15 ± 0.63a
8.77 ± 1.25a
ALP(U/L)
294.40 ± 46.00ab
294.40 ± 24.34ab
294.40 ± 40.10ab
220.80 ± 27.60a
340.40 ± 18.40b
340.40 ± 9.20b
Values are expressed in mean ± standard error of mean. Values with the same superscript across the row have no significant different at p < 0.05. E Enzymes, TP total protein, AST aspartate transaminase, ALT alanine transaminase and ALP alkaline phosphatase
Total proteins are valuable indicator of secretory, synthetic and excretory function of the liver [49]. The total protein (TP) were significantly reduced in rats administered Ag NP and Ag-I NP relative to control groups after 21 days. However, such reduced actions of TP may adversely impact the amino acid and carbohydrate breakdown with consequent declining effects on the production of ATP [40].
Histopathological studies
The liver photomicrograph on Fig. 1 displays the hepatocyte histomorphology (black arrows) and histo-architectural cells of the experimental animals. This is to investigate the effect of surface application of Ag-NP, and Ag-I NP on the liver of experimental animals. Control (N), PEG, Ag-NP, and Ag-I NP display a distinctive histomorphological appearance with normal staining intensity and stable cell density and assortment. The central vein is represented by the black circles/CV. The STD (povidone iodine) shows a typical histomorphology of the liver by the central vein, it appears clogged suggesting signs of cholestasis. Untreated (UTD) shows a fatty liver as indicated by the halospaced tiny fat droplets (yellow arrow) and reduced cellular density while the hepatocytes of Ag-NP, and Ag-I NP treated group remain intact. This implies that the biosynthesized Ag-NP, and Ag-I NP may have not induced any toxic injury on the liver. This result is consistent with the study of Umbreit et al. [50] which reported that murine models revealed no evidence of tissue disruption in response to nanoparticle treatment.
×
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The kidney photomicrograph of experimental animals showing the renal cortex, component kidney corpuscles (black circle) and neighboring halo-spaced convoluted tubules (black arrows) shown in Fig. 2. The control group (N) and Ag- I NP are present with intact renal corpuscles. Zhang et al. [51] reported that titanium dioxide nanoparticle has no effect on the renal cells. The rest of the photomicrographs presented with corpuscular degeneration marked by the large halo-spaced bowman space (yellow and red circles) shows that Ag-I NP, preserved the integrity of the kidney cells.
×
Conclusion
Silver nanoparticles (Ag NPs) and iodine-doped silver nanoparticle (Ag-I NP) altered haematological parameters in the rats and also influenced some biochemical changes in the serum of the rats. While in the histopathological study, the antioxidant present in the plant extract used to synthesize Ag NPs and Ag I-NPs may have functioned in synergy to maintain and preserve the integrity of the hepatocytes and renal corpuscles of the rats.
Availability of materials
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Declarations
Ethics approval and consent to participate
The present study was approved by the Ethical Committee on the use of animals for research, Department of Biochemistry, Federal University Technology, Minna, Nigeria. Handling of the rats was in accordance with the standard principles of laboratory animal care of the United States National Institutes of Health (NIH, 1978).
Consent for publication
All authors consent to submission and publication of this manuscript.
Competing interests
The authors declare that they have no competing interests.
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