Biogenesis of Silver Nanoparticles and Its Multifunctional Anti-Corrosion and Anticancer Studies

: In the present research, silver nanoparticles were synthesized using ground nutshell and characterized using UV-visible, FTIR and PXRD. The SEM and HR-TEM aided in conﬁrming the nano size, surface morphology and phase purity of the AgNPs. The quantum chemical, electrochemical, and structural studies were carried out to understand electrochemical properties. In addition, biological study such as anti-cancerous activity was carried out, and IC-50 values 80.25 µ g/mL for A549 lung cancer cell lines. The effective electrochemical anti-corrosion activities were also studied. The majority constituents of ground nutshell are ﬂavonoids, in a small quantity of alkaloids and phenolic acids, which provide more stability to synthesize silver nanoparticles and avoid agglomeration. These functional moieties enhance the unique properties in the ﬁeld, as in drug delivery systems, magnetic applications, and metallic, semi-conducting core-shell nanoparticles. the formation of the structure


Introduction
Recently, nanoscience and technology have developed rapidly all over the world, largely by adopting the quality, advancement, and efficiency of nanoparticles [1,2]. The transition of metal nano-materials grabbed the attention of researchers due to massive applications in the field of environmental sciences, biomedical sciences, and electrochemical sciences [2][3][4][5][6][7][8]. The physical and chemical methods of synthesis of nanoparticles have limited advantages due to high toxicity [9][10][11]. These methods have a long process involvement and costly chemical usage [8,12]. The green synthesis of metal nanoparticles is environmentally safe, plant-mediated, biologically active, requires around one hour, and is a cost-effective synthesis process [13][14][15][16][17]. In this approach, the phytochemicals, the biologically active ingredients found in the extract of the plant, help in the reduction and stabilization of metal nanoparticles.
The AgNPs can be prepared using various biological materials, plants, microorganisms, and other dairy items. Recently reported works include the synthesis of Ag nanoparticles employing different plant compounds, including certain pelargonium graveolens, extract in the present work using Soxhlet extraction techniques. The newly synthesized AgNPs were validated employing UV-Visible, FTIR, XRD, SEM and TEM studies. The corrosion studies were performed by using AAS, TAFEL and impedance spectroscopy techniques. Further, Chemical quantum studies are also employed to support AAS and electrochemical results. Similarly, anticancer activity on MTT cell lines A435 with IC 50 value 80.25 µg/mL have shown promising results for this investigation.

Materials and Methods
The fresh groundnuts are collected in August from the most fertile soil of Dharwad district, India. Groundnut shells were cleaned with purified water to eliminate dirt and mud contaminations which can toxicate the extract. Shells were dried in sunlight, blended into powder, stored in plastic bottles, and kept in the refrigerator until used. Soxhlet extraction is only needed if the target compound has minimal solubility, and the impurity is insoluble in the solvent. If the target compound has a high solvent solubility, a quick filtration isolates the compound from the insoluble material. Hence in the present investigation, Soxhlet extraction is preferred. The powder (50 g) is kept in the Soxhlet apparatus (Borosil, Gurgaon, India) and solvent, benzene, for the extraction. The round-bottomed flask is placed at the bottom of the thimble by adding 2-3 boiling chips (that avoids bumping of the solution). Extraction was carried out at 100 • C for a minimum of 18 to 20 cycles. After that, the phytocompounds from the ground nutshell get collected in the R. B. flask. During each cycle, the non-volatile compound of the sample gets concentrated in the extraction. The solution from R. B. flask is the ground nutshell extract (GNS extract) that acts as the reducing/capping agent. The solution is filtered, and the residue was collected into a separate beaker. The extract is light-brown in colour, as in Figure 1. species. Hence, we selected groundnut shells and the green species in ground nutshell extract in the present work using Soxhlet extraction techniques. The newly synthesized AgNPs were validated employing UV-Visible, FTIR, XRD, SEM and TEM studies. The corrosion studies were performed by using AAS, TAFEL and impedance spectroscopy techniques. Further, Chemical quantum studies are also employed to support AAS and electrochemical results. Similarly, anticancer activity on MTT cell lines A435 with IC50 value 80.25 μg/mL have shown promising results for this investigation.

Materials and Methods
The fresh groundnuts are collected in August from the most fertile soil of Dharwad district, India. Groundnut shells were cleaned with purified water to eliminate dirt and mud contaminations which can toxicate the extract. Shells were dried in sunlight, blended into powder, stored in plastic bottles, and kept in the refrigerator until used. Soxhlet extraction is only needed if the target compound has minimal solubility, and the impurity is insoluble in the solvent. If the target compound has a high solvent solubility, a quick filtration isolates the compound from the insoluble material. Hence in the present investigation, Soxhlet extraction is preferred. The powder (50 g) is kept in the Soxhlet apparatus (Borosil, Gurgaon, India) and solvent, benzene, for the extraction. The round-bottomed flask is placed at the bottom of the thimble by adding 2-3 boiling chips (that avoids bumping of the solution). Extraction was carried out at 100 °C for a minimum of 18 to 20 cycles. After that, the phytocompounds from the ground nutshell get collected in the R. B. flask. During each cycle, the non-volatile compound of the sample gets concentrated in the extraction. The solution from R. B. flask is the ground nutshell extract (GNS extract) that acts as the reducing/capping agent. The solution is filtered, and the residue was collected into a separate beaker. The extract is light-brown in colour, as in Figure 1.

Synthesis of AgNPs
About 200 mL of 0.01 N AgNO3 solution was added to the extract. The ground nutshell extract is reduced now to the AgNO3 (i.e., Ag + to Ag 0 ) to its nanoscale by mainly three steps: nucleation, accumulation, and stabilization. The extract solution changes from reddish-brown to dark brown color that indicates the formation of AgNO3. One to two drops of freshly prepared 0.1 N NaOH solution were added to maintain pH of 7-9 to form the AgNPs with higher yield and smaller size. After two to three days, the water in the container evaporates, and only AgNPs are placed on a magnetic stirrer (Remi, Thane, India) for heating. Thus, the AgNPs are obtained in the form of powder. The powdered AgNPs were weighed on balance to determine their concentrations per gm. About 5 mg of AgNPs were obtained per 50 gm of ground nutshell material. To understand the ease of structure, morphology and properties of synthesized silver nanoparticles were characterized employing UV-Visible, FTIR, SEM and TEM methods. Further, those are interconnected with applications in corrosion studies [38,39] and anticancer activities [30].

Synthesis of AgNPs
About 200 mL of 0.01 N AgNO 3 solution was added to the extract. The ground nutshell extract is reduced now to the AgNO 3 (i.e., Ag + to Ag 0 ) to its nanoscale by mainly three steps: nucleation, accumulation, and stabilization. The extract solution changes from reddish-brown to dark brown color that indicates the formation of AgNO 3 . One to two drops of freshly prepared 0.1 N NaOH solution were added to maintain pH of 7-9 to form the AgNPs with higher yield and smaller size. After two to three days, the water in the container evaporates, and only AgNPs are placed on a magnetic stirrer (Remi, Thane, India) for heating. Thus, the AgNPs are obtained in the form of powder. The powdered AgNPs were weighed on balance to determine their concentrations per gm. About 5 mg of AgNPs were obtained per 50 gm of ground nutshell material. To understand the ease of structure, morphology and properties of synthesized silver nanoparticles were characterized employing UV-Visible, FTIR, SEM and TEM methods. Further, those are interconnected with applications in corrosion studies [38,39] and anticancer activities [30].

Characterization Methods
Prime techniques incorporated to characterize are as follows, AgNPs were screened with UV-Visible spectroscopy on LABMAN LMSP-UV1200 (Lamaman, Chennai, India) with a wavelength accuracy of +0.5 nm. A Fourier-transform infrared spectroscopy (FT-IR) study was performed to confirm the formation of green silver nanoparticles in the range of 4500-400 cm −1 by instrumentation at the Sophisticated Analytical Instrumentation Facilities (SAIF) Centre, Karnatak University, Dharwad (KUD) India by using NICOLET 6700, (Thermo Scientific, Pune, India) instrument. X-ray Powder Diffraction (X-RD) of model Xpert MPD, Philips, Amsterdam, The Netherlands was used to analyze the structure of the newly synthesized AgNPs. The XRD patterns were recorded on X-ray diffractometer at the range of 2θ from 3 • to 136 • using Cu target X-ray tube, Cu Kα (λ = 1.5406 A) radiation with a tracking voltage of 40 kV. Scanning Electron Microscopy (SEM-EDX, (JEOL, Tokyo, Japan) was carried out to learn the external morphology of AgNPs. A scanning electron microscope (JEOL, Tokyo, Japan) was also used to study morphological characteristics of synthesized AgNPs with an accelerating voltage with LaB6 filament 2 nm 30 kV with W filament 3.5 nm at 30 kV by emission current of 0 to 200 µA and accelerating voltage: 0.2 to 30 kV. The size, shape, and morphology of synthesized AgNPs, were confirmed using HR-TEM(Thermofisher, New York, NY, USA), performed in TEM Lab, Centre for Nano and Soft Matter Sciences (CeNS), Bengaluru. Atomic absorption spectroscopic analysis (AAS) was performed using the Atomic Absorption spectrometer with graphite furnace and autosampler 222 Rn and 220 Rn mitigation systems gamma dosimeter (Thermofisher, New York, NY, USA), survey meter and GPS TLDs, Pinhole dosimeter (from Electronics and Engineering Pvt Ltd., Dadra, India), performed in DTPS and DRPS USIC Centre Mangalore University, India.

Phytochemical Screening
The qualitative and quantitative investigation of phytochemicals identify the molecules of the samples, and from this analysis, results obtained are shown in Table 1. Recent studies showed that GNS-extract contains a major quantity of flavonoids (catechin, epicatechin gallate, leucocyanidin, procyanidin B1 and rutin), some alkaloids (arecoline, arecaidine, guvacine, iso-guvacine) and traces of phenolic acids (gallic acid). Flavan-3-ol (catechin)is a secondary metabolite and natural polyphenol form and anti-oxidant. Another flavan-3-ol, flavonoid, epicatechin gallate is present in green tea, buckwheat and in grapes. The additional class of natural products, a derivative of flavonoid leucoanthocyanidins. Molecules of catechins and epicatechins produce extracellular substances. The procyanidins became part of the flavonoid proanthocyanidin family. The quercetin-3-O-rutinoside and sophorin together rutoside or Rutin. Alkaloids, like Arecaidine, Arecoline & Guvacine are acidbased alkaloids found in the areca nut and fruit of the areca palm. The iso-guvacine is a dimer of guvacine. Gallic acid is known of total phenolic identified in the extract and trihydroxybenzoic acid, found in tea leaves, oak bark, and gallnuts.
Phytochemicals like, alkaloids, terpenoids, carbohydrates and other active biomolecules reduce metal cations to their elemental metals. This transformation from positive to zero oxidation state enhances the size distribution of metal nanoparticles through indorsing new nuclei for faster reaction progress, and also by forming a monolayer (capping) on the nano-surface prevents the clustering of the nanoparticles. These surface-active molecules functionalize the nanoparticles towards biological activity. The enhanced anti-cancerous activity can be enlightened due to the phytochemicals attached at the surface [40,41]. The biomolecules of the ground nutshell extracted act here as both reductant as well as capping agents. The capped nature, the surface of nanomaterials becomes active therapeutic agents, reduces the level of toxicity, and prevents the accumulation of particles [42,43]. The core-shell nanoparticles (CSNPs) are described as containing the inner material, known as the core, and the outer layer material, which is known as the shell. They consist of a wide variety of combinations of close contact and inorganic/inorganic. The selection of core-shell material of the nanoparticle shell usually is highly dependent on the final application and use. The CSNPs are highly functional compounds with altered properties. Frequently, the properties of either core or shell materials can be very different. The properties can be changed by changing either the composition of the components or the ratio of the center to the shell. Due to the shell material covering, the core particles properties, such as the reduction of reactivity or thermal stability, can be improved to improve the overall stability of the particle and the dispersibility of the core particle. Finally, the particles exhibit distinctive characteristics of the various materials used together. The CSNPs are becoming more attractive as these nanoparticles have emerged at the boundary between chemical materials and many other fields, such as computing, biomedical, medicinal, optical, and catalysis.
An organic biological moiety encapsulates a cluster of a few nanoparticles to create a healthy core-shell morphology, as shown in Figure 2. The biological moiety consists of a significant part of flavonoids and alkaloids from groundnut extract. These act as reducing and stabilizing agents to create stable metal nanoparticles and contribute its tremendous surface interaction towards anticorrosion anticancer studies. The core-shell nanoparticles (CSNPs) are described as containing the inner material, known as the core, and the outer layer material, which is known as the shell. They consist of a wide variety of combinations of close contact and inorganic/inorganic. The selection of core-shell material of the nanoparticle shell usually is highly dependent on the final application and use. The CSNPs are highly functional compounds with altered properties. Frequently, the properties of either core or shell materials can be very different. The properties can be changed by changing either the composition of the components or the ratio of the center to the shell. Due to the shell material covering, the core particles properties, such as the reduction of reactivity or thermal stability, can be improved to improve the overall stability of the particle and the dispersibility of the core particle. Finally, the particles exhibit distinctive characteristics of the various materials used together. The CSNPs are becoming more attractive as these nanoparticles have emerged at the boundary between chemical materials and many other fields, such as computing, biomedical, medicinal, optical, and catalysis.
An organic biological moiety encapsulates a cluster of a few nanoparticles to create a healthy core-shell morphology, as shown in Figure 2. The biological moiety consists of a significant part of flavonoids and alkaloids from groundnut extract. These act as reducing and stabilizing agents to create stable metal nanoparticles and contribute its tremendous surface interaction towards anticorrosion anticancer studies.

Computational-Chemical Approach
The recent reports from computational chemists realized the understanding of the molecular structure and their reactivities. The quantum chemical parameters, electron movement in HOMO and LUMO, orbitals together are responsible for chemical reactivity. The HOMO is the maximum orbital energy and is filled by electrons. Hence, electrons can be removed from it. LUMO is the minimum orbital energy, which would be empty. Theoretical chemical calculations of HOMO-LUMO were considered in the present study to explain the different periodic properties of molecules involved. The E HOMO and E LUMO values were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2. Table 2. Values of HOMO-LUMO for chemical constituents.

Chemical Name Molecular Formula Structural Formula
Arecoline: The HOMO is the maximum orbital energy and is filled by electrons. Hence, electrons can be removed from it. LUMO is the minimum orbital energy, which would be empty. Theoretical chemical calculations of HOMO-LUMO were considered in the present study to explain the different periodic properties of molecules involved. The EHOMO and ELUMO values were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2. be removed from it. LUMO is the minimum orbital energy, which would be empty. Theoretical chemical calculations of HOMO-LUMO were considered in the present study to explain the different periodic properties of molecules involved. The EHOMO and ELUMO values were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2. oretical chemical calculations of HOMO-LUMO were considered in the present study to explain the different periodic properties of molecules involved. The EHOMO and ELUMO values were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2. explain the different periodic properties of molecules involved. The EHOMO and ELUMO values were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2. ues were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2. ues were gained from the advanced Argus Lab software (4.0.1). The chemical names, molecular structure, HOMO-LUMO and other quantum chemical values are tabulated in Table 2.     (1) and (2) are determined as, χ (Electronegativity) and η (Chemical hardness) can be related as respectively follows in 3 & 4, Chemical softness or Electron polarizability (σ) and Chemical potential (μ) are formulated according to the relations 5 & 6 I (Ionization potential) and E (electron affinity) The Equations (1) and (2) are determined as, χ (Electronegativity) and η (Chemical hardness) can be related as respectively follows in 3 & 4, Chemical softness or Electron polarizability (σ) and Chemical potential (µ) are formulated according to the relations 5 & 6 σ = I (5) Electrophilicity index (ω) can be equated as in 7, Above data I (ionization potential), E (electron affinity), η (chemical hardness), χ (Electronegativity), Electron polarizability (σ), chemical potential (µ) and band gap were calculated and tabulated in the Table 3. This study provides a wide idea for understanding structural features. The molecular structures of ten natural components contain double bonds, N and O atoms in their structures. The above investigations show natural constituents of the plants exhibit high values E HOMO in eV for alkaloids compared to flavonoids. These medicinal compounds, acecainide (HOMO = −0.617735), arecoline (HOMO = −0.613442), guvacine (HOMO = −0.664881) and iso-uvagcine (HOMO = −0.652635) with high E HOMO values are electron rich species, which donates electrons to species having empty molecular orbital of low energy and which can take an electron from the electron-rich organic compounds. The other related properties are discussed as follows,

•
Ionization potential (I), values of HOMO are higher and explain the stability of organic compounds. Lower is the I value, higher is the reactivity of organic moieties. Therefore reactivity, based on I values, is related as Procyanidin B1 > Rutin > Epicatechi gallate > Catechin > Gallic acid > Leucocyanidin > Arecaidine > Arecoline > Iso-Guvacine > Guvacine.

•
The increase in the energy gap value, decrease in the reactivity of organic compound on the surface. The trend is in the order of, Rutin > Epicatechi gallate > Procyanidin B1 > Catechin > Gallic acid > Leucocyanidin > Arecaidine > Guvacine > Iso-Guvacine > Arecoline.

•
The electrophilic or nucleophilic nature of natural components can be predicted by Electrophilicity (ω) values. Higher the ω values, the stronger the electrophile and the lower the ω values, the stronger the nucleophile. Thus, Rutin is a strong electrophile, and Procyanidin B1 is a strong nucleophile.

•
The softness and hardness are dynamic parameters to measure the reactivity and stabilities of the natural components. The greater the η, values the greater is the softness of the compound. Thus, Rutin is the less soft compound.

Characterization of GNS-AgNPs
The groundnut shell extract and silver nitrate solution mixture turning from light yellow to brown after the incubation time of half an hour indicates that Ag + reduces to Ag 0, and structural identification of metal nano-particles are confirmed by using the UV-Visible technique. In Figure 3, the surface plasmon resonance of electrons obtained for GNS-AgNPs is 378 nm, which explains the formation of silver nanoparticles. Further, the increase in the intensity of SPR peak which increases with time also confirms the formation of GNS-AgNPs.


The softness and hardness are dynamic parameters to measure the reactivity and stabilities of the natural components. The greater the η, values the greater is the softness of the compound. Thus, Rutin is the less soft compound.

Characterization of GNS-AgNPs
The groundnut shell extract and silver nitrate solution mixture turning from light yellow to brown after the incubation time of half an hour indicates that Ag + reduces to Ag 0, and structural identification of metal nano-particles are confirmed by using the UV-Visible technique. In Figure 3, the surface plasmon resonance of electrons obtained for GNS-AgNPs is 378 nm, which explains the formation of silver nanoparticles. Further, the increase in the intensity of SPR peak which increases with time also confirms the formation of GNS-AgNPs. The FTIR spectroscopic method is an essential tool to spot the new compound and recognize the secondary metabolites of the groundnut shell extract, which are acting as reducing and stabilizing agents for GNS-AgNPs. The plots obtained by transmittance with a wavelength of FTIR spectra show a clear difference in their results. The pure extract and of AgNPs bands as in Figure 4 about 3500 and 2500 cm −1 . The band shows the occurrence of O-H polyphenol stretching found in the extract. The 1624 cm −1 band refers to a group of carbonyl strip amides in the bark extract containing proteins. The 1628.56 is of C=O, and 1384.05 cm −1 is of C-O bands were stretching and bending frequencies respectively. The above bands demonstrate the identity of flavonoids and terpenoids from ground nutshell compounds [4 4,45].
The peak at 3431.33 cm −1 is due to the N-H extending the vibration of plant organic compounds absorbed into the body to silver NPs. In the same way, relative to pure ground  The X-ray diffractograms shown in Figure 5 identifies the phase purity and crystal structure of a sample-the silver nanoparticles, of the GNSE-AgNPs identified by diffraction peaks of XRD. The XRD pattern of GNSE-AgNPs obtained here is shown prominent peaks observed at (111), (200) and (220) a with agreeing 2θ values as 38.28°, 44°, 64.36° and 77.12°. It indicates the crystalline presence and is accredited to the fcc structure of GNSE-AgNPs (JCPDS 89-3722). The calculated crystallite size of GNSE-AgNPs is to be 12-15 nm. However, grain size of GNSE-AgNPs is marked by the peaks at (111) using the Scherer formula. The XRD studies also reflect a synthesis of GNSE-AgNPs by the reduc-  The peak at 3431.33 cm −1 is due to the N-H extending the vibration of plant organic compounds absorbed into the body to silver NPs. In the same way, relative to pure ground nutshell extract, the IR bands are moved from 2960.24 to 2955.03, 1632.24 to 1628.52 and 1514.38 to 1577.43 cm −1 . These changes demonstrate that types of proteins and metabolites, terpenoids, flavonoids and polyphenols are implicated in the reduction and bio-encapsulation of AgNPs. The peak at 1620.88 cm −1 , aromatic C=C in carboxyl group, which also quercetin peaks (12). The X-ray diffractograms shown in Figure 5 identifies the phase purity and crystal structure of a sample-the silver nanoparticles, of the GNSE-AgNPs identified by diffraction peaks of XRD. The XRD pattern of GNSE-AgNPs obtained here is shown prominent peaks observed at (111)  The X-ray diffractograms shown in Figure 5 identifies the phase purity and crystal structure of a sample-the silver nanoparticles, of the GNSE-AgNPs identified by diffraction peaks of XRD. The XRD pattern of GNSE-AgNPs obtained here is shown prominent peaks observed at (111), (200) and (220) a with agreeing 2θ values as 38.28°, 44°, 64.36° and 77.12°. It indicates the crystalline presence and is accredited to the fcc structure of GNSE-AgNPs (JCPDS 89-3722). The calculated crystallite size of GNSE-AgNPs is to be 12-15 nm. However, grain size of GNSE-AgNPs is marked by the peaks at (111) using the Scherer formula. The XRD studies also reflect a synthesis of GNSE-AgNPs by the reduction of GNSE-AgNPs. From the observed results, it is clear that GNS-extract is effective in reducing metal salts into its nanoparticles. The presence of bioactive compounds is successful in maintaining stabilization and dispersion to prevent aggregation [46]. The morphology of the shaped AgNPs is studied using a scanning electron microscope. Adsorption of organic moieties from the plant extract is clearly shown by SEM image (Figure 6). The average bio-capped GNSE-are AgNPs circular with a size of 20 nm or less. maintaining stabilization and dispersion to prevent aggregation [46]. The morphology of the shaped AgNPs is studied using a scanning electron microscope. Adsorption of organic moieties from the plant extract is clearly shown by SEM image (Figure 6). The average bio-capped GNSE-are AgNPs circular with a size of 20 nm or less. The size, scale, form and structure of the synthesized AgNPs have been verified using TEM. TEM pictures are shown, almost spherical Ag particle structures and polydisperse. The histogram of the distribution of the particle size is calculated by TEM in Figure 7. The AgNPs nanoparticles range from 35-40 nm, and the average particle-size length is ±30 nm in diameter. The selected area electron diffraction pattern (SAED) for AgNPs corresponds to crystallographic planes of FCC pattern of silver.    The size, scale, form and structure of the synthesized AgNPs have been verified using TEM. TEM pictures are shown, almost spherical Ag particle structures and polydisperse. The histogram of the distribution of the particle size is calculated by TEM in Figure 7. The AgNPs nanoparticles range from 35-40 nm, and the average particle-size length is ±30 nm in diameter. The selected area electron diffraction pattern (SAED) for AgNPs corresponds to crystallographic planes of FCC pattern of silver.  When it comes small scale observations, the nanoparticles, and their activated surface, from getting charged, causes slight image degradation. The shape of metal nanoparticles is known to significantly vary their optical and elemental properties, which may be determined using the EDX method [47,48]. The optical absorption of Ag is clearly shown in the EDAX profile ( Figure 8). AgNPs contain 20.05% of Ag at 3 keV, and in addition to Cl, S, and Ower, AgNPs also include Mg, P, K, Ca, Cu, which are captured from the green extract used for synthesis. The percentage of carbon in Fe-PAni fluctuated, which was due to the carbon tape used to attach the samples to the sample holder [49]. FTIR analysis was used to identify the functional groups connected to the AgNPs. The phenolic group in the crude green extract binds to the AgNPs with a high affinity. Other functional groups that AgNPs have connected to include phenol (-OH) at 3442 cm −1 , carboxylic acids at 2923 cm −1 , and ethers at 1019 cm −1 (Figure 4). After the green production of AgNPs, the supernatant contained less phenol and flavonoid than the green extract ( Figure 4). As a result, it was shown that the phytochemical contents may be linked to AgNPs during the green When it comes small scale observations, the nanoparticles, and their activated surface, from getting charged, causes slight image degradation. The shape of metal nanoparticles is known to significantly vary their optical and elemental properties, which may be determined using the EDX method [47,48]. The optical absorption of Ag is clearly shown in the EDAX profile ( Figure 8). AgNPs contain 20.05% of Ag at 3 keV, and in addition to Cl, S, and Ower, AgNPs also include Mg, P, K, Ca, Cu, which are captured from the green extract used for synthesis. The percentage of carbon in Fe-PAni fluctuated, which was due to the carbon tape used to attach the samples to the sample holder [49]. FTIR analysis was used to identify the functional groups connected to the AgNPs. The phenolic group in the crude green extract binds to the AgNPs with a high affinity. Other functional groups that AgNPs have connected to include phenol (-OH) at 3442 cm −1 , carboxylic acids at 2923 cm −1 , and ethers at 1019 cm −1 (Figure 4). After the green production of AgNPs, the supernatant contained less phenol and flavonoid than the green extract ( Figure 4). As a result, it was shown that the phytochemical contents may be linked to AgNPs during the green synthesis process. The peaks observed in EDX graph and profile may be due to Kα 1 and Kedge. When the incident energy of a photon equalled the binding energy of an electron shell in the absorber, such as K, L, or M, etc., a substantial rise was observed for that particular element. This is used to produce a void in the shell while using the least amount of energy possible. This energy was referred to as critical excitation or edge. An electron transfer from another shell filled an initial vacancy in an inner shell produced by an electron or X-ray, leaving a final vacancy in that shell resulting in the characteristic X-ray lines ( Figure 5). The energy of lines is equal to the difference between the binding energy of the shells in which the initial and final voids were formed. The excitation of the K, L, M, N or O levels lines in an element's X-ray spectra were detected depending on its atomic number.
transfer from another shell filled an initial vacancy in an inner shell produced by an electron or X-ray, leaving a final vacancy in that shell resulting in the characteristic X-ray lines ( Figure 5). The energy of lines is equal to the difference between the binding energy of the shells in which the initial and final voids were formed. The excitation of the K, L, M, N or O levels lines in an element's X-ray spectra were detected depending on its atomic number.

Atomic Absorption Spectroscopy (AAS) Technique
The AAS was used to evaluate the effects of GNS-AgNPs on aluminium (Al) corrosion in the 1M hydrochloric acid solution. The pre-weighed Al was submerged in the 1M hydrochloric acid (HCl) solution without and with four various concentrations of GNS-AgNPs for 10 h immersion time at 303 K. After the time, the Al is withdrawn from the 1M HCl solution and weight is recorded. The results of AAS are shown in Table 4. The table showed the robust adherence of the GNS-AgNPs on the surface of aluminium in the 1M HCl. The table shown that the Al weight loss reduced with the introduction of GNS-AgNPs of 0.1, 0.2, 0.3, and 0.4 mg/L in 1M HCl soltion. The protection rate enhances with rise in the concentration of GNS-AgNPs is due to an increase in the surface coverage of green nanoparticles over the Al surface in the 1M HCl solution. The adsorption of GNS-AgNPs over the Al surface generates a barrier for mass and charge transfer, leading to a reduction in the interaction between the 1M HCl solution and Al surface. The existence of GNS-AgNPs film on the Al surface blocks the Al surface disintegration. The protection efficiency of GNS-AgNPs on the aluminium surface could be associated with the adsorption of electron-rich elements on the empty or partially filled orbitals of Al in 1M HCl solution. As a result, the enhancing stability of newly generated bonds with the green nano particles [35,38,50].  AC impedance spectroscopy explores the kinetics of reactions at the Al/molar hydrochloric acid solution interface. Figure 9a represents the Nyquist curves obtained from the inhibition of Al corrosion by using the 1 to 4 mg/L of GNS-AgNPs. The Nyquist readings are shown the Table 5. The Nyquist plots (impedance curves) of protected system are not different from the unprotected system except in terms of the diameter of the depressed semi-circle. AC impedance spectroscopy explores the kinetics of reactions at the Al/molar hydrochloric acid solution interface. Figure 9a represents the Nyquist curves obtained from the inhibition of Al corrosion by using the 1 to 4 mg/L of GNS-AgNPs. The Nyquist readings are shown the Table 5. The Nyquist plots (impedance curves) of protected system are not different from the unprotected system except in terms of the diameter of the depressed semi-circle.  The Nyquits plots in the presence and absence of GNS-AgNPs is not a perfect semicircle due to frequency dispersion. The charge transfer resistance values are and precisely related to the difference of the GNS-AgNPs. The charge transfer resistance values enhance, and the corrosion rate reduces with an increasing concentration of the Al, 0.1 mg/L, 0.2 milligram per liter, 0.3 mg/L and 0.4 milligram per liter of GNS-AgNPs. The radius of  The Nyquits plots in the presence and absence of GNS-AgNPs is not a perfect semicircle due to frequency dispersion. The charge transfer resistance values are and precisely related to the difference of the GNS-AgNPs. The charge transfer resistance values enhance, and the corrosion rate reduces with an increasing concentration of the Al, 0.1 mg/L, 0.  Table 6 shows the impedance spectroscopy technique. The inhibitor can be classified as cathodic, anodic or mixed type by using the Tafel plot technique. The Tafel plot studies showed that (Figure 9b), by addition of green nanoparticles, they had a significant influence on the aluminum corrosion current density values and low at higher concentration of GNS-AgNPs. As a result of this, there is a remarkable enhancement in the protection efficiency values. The surface area of Al covered by GNS-AgNPs species enhances with a rise in the amount of GNS-AgNPs, which shows that the aluminum protection is mainly due to the green nanoparticles' adsorption over the Al surface. The adsorption process suppresses the Al dissolution process. Further, significant change in the anodic Tafel slope values (from 0.003 to 5.494) compared to cathodic one clearly shows the anodic corrosion inhibition property of the GNS-AgNPs over the Al surface in the 1M HCl solution.
The SEM texture of the aluminium surfaces showing to 1M HCl without and with the GNS-AgNPs are observed. The results (Figure 9c) show that the absence of GNS-AgNPs revealed that the aluminium surface was strongly damaged due to corrosive attack by the acid solution. It is seen from Figure 9d, that a shielding film was formed on the aluminum metal surface in the presence of GNS-AgNPs and the surface became smooth, without any pits, roughness characteristics and cracks over Al surface.

Anti-Cancerous Activity on Human Alveolar Cell Lina549, Human Lung Cancer Cells
The decrease in the efficiency of mitochondrial activity is studied effectively by the toxicity action of ground nutshell extract silver nanoparticles. The large reductions in tetrazolium salts are now well accepted as a healthy tool for measuring cell proliferation. The yellow tetrazolium (C 18 H 16 BrN 5 S) is diminished by metabolically active cells, and delivers a measurable resolve of viable cells through the operation of dehydrogenase enzymes to produce reduced derivatives.
The corresponding intracellular purple formazan can also be solubilized and analyzed by spectrophotometric methods [51,52]. The assay measures the rate of cell proliferation, and vice versa. However, as metabolic processes contribute towards apoptosis or necrosis, cellular uptake declines. The cells being placed on 96 well plates in 100 µL of RPMI 1640 and permitted to expand in the subsequent subcellular purple formazan can always be dissolved and studied using spectroscopic methods. The different sampling compositions for 45 to 48 h, the incubation of cells 24 to 28 h. 20 µL C 18 H 16 BrN 5 S stock solution is then added to both the plates and incubated for 5 h. The medium is now extracted, and 200 µL of DMSO is applied to dissolve the metabolic in each well MTT substance. The plate is rattled at 150 rpm for five minutes and the absorption spectrum at 560 nm. The unprocessed cells (basal) are used to control the viability (100%), and the influence is reflected in relation to the regulation as a percent viability (log), as shown in Figure 10a compositions for 45 to 48 h, the incubation of cells 24 to 28 h. 20 μL C18H16BrN5S stock solution is then added to both the plates and incubated for 5 h. The medium is now extracted, and 200 μL of DMSO is applied to dissolve the metabolic in each well MTT substance. The plate is rattled at 150 rpm for five minutes and the absorption spectrum at 560 nm. The unprocessed cells (basal) are used to control the viability (100%), and the influence is reflected in relation to the regulation as a percent viability (log), as shown in Figure  10a,b. The transformation of yellow tetrazolium salt (C18H16BrN5S) into purple formazan crystals by metabolically active cells gives an accurate confirmation of viable cells. The expected mechanism for cell death is given in the graphical representation ( Figure 10)   The transformation of yellow tetrazolium salt (C 18 H 16 BrN 5 S) into purple formazan crystals by metabolically active cells gives an accurate confirmation of viable cells. The expected mechanism for cell death is given in the graphical representation ( Figure 10) [53][54][55]. IC-50 value of 85.47 µg/mL for 24 h. The percent inhibition of growth was determined after subtracting the history and the null, and the test drug concentration required to inhibit cell proliferation was created by 50 percent (IC 50) of the dosages curves for the cancer cell [56,57]. The probable mechanism for cell apoptosis is explained in Figure 11.
As shown in Figure 11, Apoptosis is the process commonly known as programmed cell death. It is the molecular programming of the cell which leads to its death. In this process the cell is broken down by the protein of itself called Caspases. Thus, for apoptosis to occur, these caspases must be activated. This mechanism of apoptosis, that is, the activation of Caspases, occurs through these three different steps; Step one involves the nitiation, followed by execution and finally phagocytosis. The initiation might be by extrinsic or intrinsic pathways. The process takes place leading to the shrinkage of the cell, either by the intracellular or extracellular process. The synthesized silver nanoparticles act as angiogenesis inhibitors [58], which block this angiogenesis process by blocking the nutrient and oxygen sources of a tumour. Further cell starving leads to ell death. inhibit cell proliferation was created by 50 percent (IC 50) of the dosages curves for the cancer cell [56,57]. The probable mechanism for cell apoptosis is explained in Figure 11. As shown in Figure 11, Apoptosis is the process commonly known as programmed cell death. It is the molecular programming of the cell which leads to its death. In this process the cell is broken down by the protein of itself called Caspases. Thus, for apoptosis to occur, these caspases must be activated. This mechanism of apoptosis, that is , the activation of Caspases, occurs through these three different steps; Step one involves the nitiation, followed by execution and finally phagocytosis. The initiation might be by extrinsic or intrinsic pathways. The process takes place leading to the shrinkage of the cell, either by the intracellular or extracellular process. The synthesized silver nanoparticles act as angiogenesis inhibitors [58], which block this angiogenesis process by blocking the nutrient and oxygen sources of a tumour. Further cell starving leads to ell death.

Conclusions
In the present work, we successfully achieved the rapid production of stable and modified sphere shaped (15-20 nm) GNS-AgNPs with high efficiency. Utilizing extracts of groundnut shells as both a reducing agent and a stabilizing agent makes the process cost-effective. The role of Ruthin chemical moieties from the ground nutshell extracts in the reduction process was evaluated, elaborated in detail, and characterized thoroughly. Further, GNS-AgNPs applied as anticorrosion studies found robust anti-corrosion (anodic type) behaviour on Al in 1M HCl system time-dependent mode. The GNS-AgNPs inhibits corrosion, and this property was very helpful in increase the lifetime of aluminium. This property, GNS-AgNPs obtained here, can be useful in various industrial units to mitigate Al corrosion problems. In addition, GNS-AgNPs are biologically active, and it further enhanced phytochemicals and polyphenols etc., present in the bio extract utilized during synthesis. The biological activity realized in the current study, with an important-anticancer activity of GNS AgNPs to effectively control over the A549, human lung Cancer cell viabilities.

Conclusions
In the present work, we successfully achieved the rapid production of stable and modified sphere shaped (15-20 nm) GNS-AgNPs with high efficiency. Utilizing extracts of groundnut shells as both a reducing agent and a stabilizing agent makes the process cost-effective. The role of Ruthin chemical moieties from the ground nutshell extracts in the reduction process was evaluated, elaborated in detail, and characterized thoroughly. Further, GNS-AgNPs applied as anticorrosion studies found robust anti-corrosion (anodic type) behaviour on Al in 1M HCl system time-dependent mode. The GNS-AgNPs inhibits corrosion, and this property was very helpful in increase the lifetime of aluminium. This property, GNS-AgNPs obtained here, can be useful in various industrial units to mitigate Al corrosion problems. In addition, GNS-AgNPs are biologically active, and it further enhanced phytochemicals and polyphenols etc., present in the bio extract utilized during synthesis. The biological activity realized in the current study, with an importantanticancer activity of GNS AgNPs to effectively control over the A549, human lung Cancer cell viabilities.

Data Availability Statement:
The data presented in this study are available on request from the corresponding author.