Imidazo-Pyrazole-Loaded Palmitic Acid and Polystyrene-Based Nanoparticles: Synthesis, Characterization and Antiproliferative Activity on Chemo-Resistant Human Neuroblastoma Cells

Neuroblastoma (NB) is a childhood cancer, commonly treated with drugs, such as etoposide (ETO), whose efficacy is limited by the onset of resistance. Here, aiming at identifying new treatments for chemo-resistant NB, the effects of two synthesized imidazo-pyrazoles (IMPs) (4G and 4I) were investigated on ETO-sensitive (HTLA-230) and ETO-resistant (HTLA-ER) NB cells, detecting 4I as the more promising compound, that demonstrated IC50 values lower than those of ETO on HTLA ER. Therefore, to further improve the activity of 4I, we developed 4I-loaded palmitic acid (PA) and polystyrene-based (P5) cationic nanoparticles (P5PA-4I NPs) with high drug loading (21%) and encapsulation efficiency (97%), by a single oil-in-water emulsification technique. Biocompatible PA was adopted as an emulsion stabilizer, while synthesized P5 acted as an encapsulating agent, solubilizer and hydrophilic–lipophilic balance (HLB) improver. Optic microscopy and cytofluorimetric analyses were performed to investigate the micromorphology, size and complexity distributions of P5PA-4I NPs, which were also structurally characterized by chemometric-assisted Fourier transform infrared spectroscopy (FTIR). Potentiometric titrations allowed us to estimate the milliequivalents of PA and basic nitrogen atoms present in NPs. P5PA-4I NPs afforded dispersions in water with excellent buffer capacity, essential to escape lysosomal degradation and promote long residence time inside cells. They were chemically stable in an aqueous medium for at least 40 days, while in dynamic light scattering (DLS) analyses, P5PA-4I showed a mean hydrodynamic diameter of 541 nm, small polydispersity (0.194), and low positive zeta potentials (+8.39 mV), assuring low haemolytic toxicity. Biological experiments on NB cells, demonstrated that P5PA-4I NPs induced ROS-dependent cytotoxic effects significantly higher than those of pristine 4I, showing a major efficacy compared to ETO in reducing cell viability in HTLA-ER cells. Collectively, this 4I-based nano-formulation could represent a new promising macromolecular platform to develop a new delivery system able to increase the cytotoxicity of the anticancer drugs.


Introduction
Neuroblastoma (NB) is a cancer of immature nerve cells representing the most common extracranial solid tumour in childhood [1].In the USA, about 700-800 new cases are detected per year, with about 1 case per 7000 live births [2][3][4].Particularly, the occurrence is 10.2 cases per 1 million per year in children under 15 years old.The overall incidence in children up to 15 years of age is approximately 15,000 new cases per year in the world, of which approximately 130 are in Italy [2].
Generally, NB is rare in people over the age of 10 years and rarely it is detected by ultrasound even before birth [3].About 37% of patients are diagnosed as infants, and 90% are younger than 5 years at diagnosis, with a median age at diagnosis of 17 months [4,5], thus establishing that NB is a disease of infancy, with the highest rate of diagnosis in the first month of life [6].Treatments for NB patients currently include surgery, to remove nonmetastatic cancer, chemotherapy, radiation therapy and treatment using iodine 131-MIBG to kill the cancer cells of primary localized NB, while high-dose chemotherapy and radiation therapy with stem cell rescue are used to kill any post-treatment residual cancer cells that may cause cancer relapse [7].Additionally, a targeted therapy, using drugs or other substances to identify and attack specifically cancer cells, can be adopted in case of relapse or when NB is not responsive to other treatments [7,8].Furthermore, new types of treatment, including immunotherapy, are being tested in clinical trials, and for some patients taking part in a clinical trial could be the best choice of treatment [7,8].Table 1 collects some therapeutic approaches currently used to treat NB.

Standard Chemotherapeutics [9]
Maintenance Therapeutics [8] Targeted Therapeutics [7] Immunotherapy [ Unfortunately, NB treatments cause severe side effects [12] and following long-term treatments, the onset of therapy resistance is often inevitable and leads to treatment failure and cancer relapse [13].Moreover, despite advances in the molecular aspect of paediatric cancers, the treatment of approximately 50% of children with high-risk neuroblastoma (HR-NB) lack efficacy [14], and current therapies are not operative in the long-term treatment of almost 80% of patients with this clinically aggressive form [15]. Also, when therapies are successful, survivors remain at risk for a wide variety of potential treatment-related complications, or "late effects", which may lead to excess morbidity and premature mortality [8,16].As an example, ETO, a DNA damage-inducing agent widely used to treat NB, can have some long-term side effects, including increased risk of developing secondary cancers, such as leukaemia or myelodysplastic syndrome.In this scenario, alternative therapeutic strategies are urgently necessary, both to counteract the development of chemoresistance and to reduce the side and late effects of current available treatments [17].In this context, the Neuroblastoma New Drug Development Strategy (NDDS) is an initiative commenced in 2012 to accelerate the development of new drugs for NB [18].Since drugs at nanosized dimensions reduce toxicity, prolong half-life, and increase the permeability of not nanoformulated compounds, our aim was to develop a novel possible therapeutic agent for NB treatment using a nanotechnological approach to formulate imidazo-pyrazole derivatives, which have previously demonstrated an interesting antiproliferative activity on several tumour cell lines [19].To this end, we first screened the synthesized imidazopyrazole derivatives (IMPs) 4G and 4I (Figure 1) [19], on ETO-sensitive (HTLA-230) and ETO-resistant (HTLA-ER) NB cells.
Strategy (NDDS) is an initiative commenced in 2012 to accelerate the development of new drugs for NB [18].Since drugs at nanosized dimensions reduce toxicity, prolong half-life, and increase the permeability of not nano-formulated compounds, our aim was to develop a novel possible therapeutic agent for NB treatment using a nanotechnological approach to formulate imidazo-pyrazole derivatives, which have previously demonstrated an interesting antiproliferative activity on several tumour cell lines [19].To this end, we first screened the synthesized imidazo-pyrazole derivatives (IMPs) 4G and 4I (Figure 1) [19], on ETO-sensitive (HTLA-230) and ETO-resistant (HTLA-ER) NB cells.Secondly, by a single oil-in-water nano-emulsion method, we employed the more active derivative (4I) to prepare 4I-loaded NPs using palmitic acid (PA) as an emulsion stabilizer and the synthesized cationic polystyrene-based copolymer (P5) as both an encapsulating and solubilizing macromolecule (Figure 2).P5PA-4I NPs were achieved, which were completely characterized by several analytical techniques and biologically tested on HTLA-230 and HTLA-ER cells.In parallel, NPs not containing 4I (P5PA NPs) were prepared, characterized and tested on NB cells, in the same conditions used for P5PA-4I NPs.

The Reasons of Our Choice
We selected PA (Figure 2a) as a stabilizer, because it is a biocompatible saturated fatty acid (FA), with a C16 chain found in animal and vegetable oils, which was reported for having intrinsic anti-tumour activity in a variety of tumour types, including colorectal, liver, prostate and breast cancer [20][21][22][23][24][25], as many other exogenous FAs, which were effective in overcoming drug resistance and metastasis in tumour cells [26,27].
In this regard, Urso and Zhou have reported that PA is lipotoxic also to Neuro-2a (N2a) neuroblastoma cells by causing cell cycle defects [28].Unfortunately, the poor water solubility and cellular impermeability of PA strongly limit its clinical application [29].Secondly, by a single oil-in-water nano-emulsion method, we employed the more active derivative (4I) to prepare 4I-loaded NPs using palmitic acid (PA) as an emulsion stabilizer and the synthesized cationic polystyrene-based copolymer (P5) as both an encapsulating and solubilizing macromolecule (Figure 2).
Int. J. Mol.Sci.2023, 24, x FOR PEER REVIEW 3 of 39 Strategy (NDDS) is an initiative commenced in 2012 to accelerate the development of new drugs for NB [18].Since drugs at nanosized dimensions reduce toxicity, prolong half-life, and increase the permeability of not nano-formulated compounds, our aim was to develop a novel possible therapeutic agent for NB treatment using a nanotechnological approach to formulate imidazo-pyrazole derivatives, which have previously demonstrated an interesting antiproliferative activity on several tumour cell lines [19].To this end, we first screened the synthesized imidazo-pyrazole derivatives (IMPs) 4G and 4I (Figure 1) [19], on ETO-sensitive (HTLA-230) and ETO-resistant (HTLA-ER) NB cells.Secondly, by a single oil-in-water nano-emulsion method, we employed the more active derivative (4I) to prepare 4I-loaded NPs using palmitic acid (PA) as an emulsion stabilizer and the synthesized cationic polystyrene-based copolymer (P5) as both an encapsulating and solubilizing macromolecule (Figure 2).P5PA-4I NPs were achieved, which were completely characterized by several analytical techniques and biologically tested on HTLA-230 and HTLA-ER cells.In parallel, NPs not containing 4I (P5PA NPs) were prepared, characterized and tested on NB cells, in the same conditions used for P5PA-4I NPs.

The Reasons of Our Choice
We selected PA (Figure 2a) as a stabilizer, because it is a biocompatible saturated fatty acid (FA), with a C16 chain found in animal and vegetable oils, which was reported for having intrinsic anti-tumour activity in a variety of tumour types, including colorectal, liver, prostate and breast cancer [20][21][22][23][24][25], as many other exogenous FAs, which were effective in overcoming drug resistance and metastasis in tumour cells [26,27].
In this regard, Urso and Zhou have reported that PA is lipotoxic also to Neuro-2a (N2a) neuroblastoma cells by causing cell cycle defects [28].Unfortunately, the poor water solubility and cellular impermeability of PA strongly limit its clinical application [29].P5PA-4I NPs were achieved, which were completely characterized by several analytical techniques and biologically tested on HTLA-230 and HTLA-ER cells.In parallel, NPs not containing 4I (P5PA NPs) were prepared, characterized and tested on NB cells, in the same conditions used for P5PA-4I NPs.

The Reasons of Our Choice
We selected PA (Figure 2a) as a stabilizer, because it is a biocompatible saturated fatty acid (FA), with a C16 chain found in animal and vegetable oils, which was reported for having intrinsic anti-tumour activity in a variety of tumour types, including colorectal, liver, prostate and breast cancer [20][21][22][23][24][25], as many other exogenous FAs, which were effective in overcoming drug resistance and metastasis in tumour cells [26,27].
In this regard, Urso and Zhou have reported that PA is lipotoxic also to Neuro-2a (N2a) neuroblastoma cells by causing cell cycle defects [28].Unfortunately, the poor water solubility and cellular impermeability of PA strongly limit its clinical application [29].Very recently, such restrictions were addressed by the group of He, encapsulating PA into a poly (D, L-lactic co-glycolic acid) (PLGA) nanoparticle (NP) platform, alone and in combination with doxorubicin (DOX), achieving PLGA-PA-DOX NPs and PLGA-PA NPs, which significantly reduced the viability and migratory capacity of breast cancer cells in vitro [29].Additionally, in in vivo studies in mice models of mammary tumours, the authors demonstrated that PLGA-PA-NPs were effective in reducing primary tumour growth and metastasis as NPs loaded with DOX, PA and DOX, or free DOX [29].Moreover, Andrés González-González and colleagues demonstrated that the interaction of PA and SiNPs had a strong synergistic character in terms of emulsion stabilization, leading to an enhanced emulsion stability [30].On these examples, in place of commercial PLGA utilized by He et al. [29] or SiNPs used by González-González et al. [30], we used the cationic P5 NPs (Figure 2b) [31] dispersed in water in association with PA dissolved in the oily phase with or without 4I, to prepare both P5PA and 4I-loaded P5PA oil-in-water (O/W) nano-emulsions stabilized by PA.Specifically, PA was able to interact with P5 dispersed in water by mean of hydrogen bond interactions [30].Notably, P5 was selected also due to its intrinsic anti-cancer effects reported on HTLA-230, HTLA-ER [32], as well as on IMR-32 and SHSY 5Y NB cells [33].

Screening of the Cytotoxic Effects of 4G and 4I on NB Cells
The first aim of this study was to evaluate the cytotoxicity of 4G and 4I on HTLA-230, an ETO-sensitive NB cell line and HTLA-ER, the ETO-resistant counterpart [34].As shown in Figure 3, 4G exerted a dose-and time-dependent cytotoxic effect on both cell populations.In contrast, 4I induced a more marked cytotoxic effect, especially in HTLA-ER, that reached a plateau level at 5 µM, thus resulting as more effective than 4G (Figure 4).
Very recently, such restrictions were addressed by the group of He, encapsulating PA into a poly (D, L-lactic co-glycolic acid) (PLGA) nanoparticle (NP) platform, alone and in combination with doxorubicin (DOX), achieving PLGA-PA-DOX NPs and PLGA-PA NPs, which significantly reduced the viability and migratory capacity of breast cancer cells in vitro [29].Additionally, in in vivo studies in mice models of mammary tumours, the authors demonstrated that PLGA-PA-NPs were effective in reducing primary tumour growth and metastasis as NPs loaded with DOX, PA and DOX, or free DOX [29].Moreover, Andrés González-González and colleagues demonstrated that the interaction of PA and SiNPs had a strong synergistic character in terms of emulsion stabilization, leading to an enhanced emulsion stability [30].On these examples, in place of commercial PLGA utilized by He et al. [29] or SiNPs used by González-González et al. [30], we used the cationic P5 NPs (Figure 2b) [31] dispersed in water in association with PA dissolved in the oily phase with or without 4I, to prepare both P5PA and 4I-loaded P5PA oil-in-water (O/W) nano-emulsions stabilized by PA.Specifically, PA was able to interact with P5 dispersed in water by mean of hydrogen bond interactions [30].Notably, P5 was selected also due to its intrinsic anti-cancer effects reported on HTLA-230, HTLA-ER [32], as well as on IMR-32 and SHSY 5Y NB cells [33].

Screening of the Cytotoxic Effects of 4G and 4I on NB Cells
The first aim of this study was to evaluate the cytotoxicity of 4G and 4I on HTLA-230, an ETO-sensitive NB cell line and HTLA-ER, the ETO-resistant counterpart [34].As shown in Figure 3, 4G exerted a dose-and time-dependent cytotoxic effect on both cell populations.In contrast, 4I induced a more marked cytotoxic effect, especially in HTLA-ER, that reached a plateau level at 5 µM, thus resulting as more effective than 4G (Figure 4).Moreover, 4G was capable of reducing cell viability by about 45-50% after 72 h, at 8-10 µM concentration in HTLA-230 cells and 20 µM in HTLA-ER.Differently, 4I induced a similar cytotoxic effect in both cell populations at 5 µM, thus further supporting that 4G was less effective than 4I (Figure 4).By using GraphPad Prism 5.4.2Software (GraphPad Software, Boston, MA, USA), and the mean data showed in Figures 3 and 4, we obtained the values of IC50 for both 4G and 4I.As observed in Table 2, only the IC50 values at 48 and 72 h of exposure have been reported since at 24 h the cell viability was >50% at all concentrations tested.Moreover, 4G was capable of reducing cell viability by about 45-50% after 72 h, at 8-10 µM concentration in HTLA-230 cells and 20 µM in HTLA-ER.Differently, 4I induced a similar cytotoxic effect in both cell populations at 5 µM, thus further supporting that 4G was less effective than 4I (Figure 4).By using GraphPad Prism 5.4.2Software (GraphPad Software, Boston, MA, USA), and the mean data showed in Figures 3 and 4, we obtained the values of IC 50 for both 4G and 4I.As observed in Table 2, only the IC 50 values at 48 and 72 h of exposure have been reported since at 24 h the cell viability was >50% at all concentrations tested.Data reported in Table 2 confirmed that the cytotoxic effects of 4G and 4I were marked after 72 h, with 4I more active than 4G.According to data previously reported [19], both compounds would exert cytotoxic effects on tumour cells affecting the cell-cycle phases with the appearance of polyploid cells, altering microtubules and targeting the tubulin system.The higher activity of 4I with respect to 4G observed here could consequently depend on the different ways the two compounds interact with the tubulin system [19].Particularly, it seems that although the shorter chain of 4G allows the molecule to fit into a small cleft formed by tubulin β and stathmin3, thus reinforcing the binding between the two proteins, molecule 4I is positioned in a way that might prevent the correct binding of tubulin tyrosine ligase to the tubulin α chain [19].Given that, in HTLA-230, 4I and 4G had IC 50 values of 10.78 and 12.31 µM, respectively, and that 10 µM IC 50 has been retained by the National Cancer Institute (NCI), the threshold useful to qualify a new product as active in terms of in vitro antitumor activity, 4I and 4G can be considered as promising new agents to develop novel formulations to cure HR-NB.Although, in HTLA-ER, the IC 50 values were 2-fold higher than the threshold dictated by NCI, 4I was 1.8-fold more active than ETO.Based on this evidence, the following biological assays were carried out exclusively with 4I with the aim to investigate the possibility of enhancing the 4I activity by a nano-formulation approach.

Dose Dependent Reactive
Oxygen Species (ROS) Production in HTLA-230 and HTLA-ER Cells ETO, as several chemotherapeutic drugs, exerts an anticancer effect mainly via ROS production and oxidative DNA damage [34][35][36].In this context, it has been reported that glutathione-mediated antioxidant response has a pivotal role in determining the chemoresistance of HR-NB cells [34].Therefore, to investigate if the cytotoxic effects of 4I could depend on ROS production, the levels of H 2 O 2 , the most long-lived ROS, were analysed and the results have been reported in Figure 5.
DCFH-DA staining is a simple and cost-effective way to detect ROS in cells after chemical treatment or genetic modifications [37].As shown in Figure 5, in HTLA-230, a significant increase in H 2 O 2 production was observed at concentrations ≥1 µM, both after 24 h of exposure (statistical significance *** vs. Ctr) and 48 h (statistical significance **** vs. Ctr), while at concentration 0.5 µM (statistical significance ** vs. Ctr), after 72 h of exposure.Anyway, when HTLA-230 cells were exposed to 4I for 24 h, the H 2 O 2 production remained constant for concentrations ≥8 µM.On the contrary, in HTLA-ER cells, after 24 h of treatment, no significant variation of H 2 O 2 production was observed in the range of concentrations tested.A significant production of H 2 O 2 (statistical significance ** vs. Ctr) was observed in HTLA-ER cells treated with 4I for 48 and 72 h at concentrations ≥1 µM.However, while H 2 O 2 production increased further for concentrations ≥1 µM after 72 h of exposure, it remained constant after 48 h of exposure for concentrations ≥5 µM.DCFH-DA staining is a simple and cost-effective way to detect ROS in cells after chemical treatment or genetic modifications [37].As shown in Figure 5, in HTLA-230, a significant increase in H2O2 production was observed at concentrations ≥1 µM, both after 24 h of exposure (statistical significance *** vs. Ctr) and 48 h (statistical significance **** vs. Ctr), while at concentration 0.5 µM (statistical significance ** vs. Ctr), after 72 h of exposure.Anyway, when HTLA-230 cells were exposed to 4I for 24 h, the H2O2 production remained constant for concentrations ≥8 µM.On the contrary, in HTLA-ER cells, after 24 h of treatment, no significant variation of H2O2 production was observed in the range of concentrations tested.A significant production of H2O2 (statistical significance ** vs. Ctr) was observed in HTLA-ER cells treated with 4I for 48 and 72 h at concentrations ≥1 µM.However, while H2O2 production increased further for concentrations ≥1 µM after 72 h of exposure, it remained constant after 48 h of exposure for concentrations ≥5 µM.
Moreover, in HTLA-230 cells treated with 10 µM 4I for 72 h, H2O2 levels were 2-fold higher than in the control cells.In this contest, Nambiar et al. demonstrated that the antiproliferative mechanism of an analogue of noscapine in different tumour cell lines, depended on the alteration of the tubulin system that in turn depended on high ROS levels (2-3-fold higher than in the control) [38].As mentioned above, according to Nambiar, Brullo et al. demonstrated that 4I altered the microtubules [19] even if they did not investigate the effects of 4I on ROS levels.Based on these findings, we can speculate that 4Itreated HTLA-230 cells die in consequence of the microtubule alterations [19] that are probably triggered by the increased ROS production in agreement with the study of Nambiar et al. [38].

Correlation between ROS Production and Cytotoxic Effects of 4I
To confirm the possible mechanism hypothesized in Section 2.2, we correlated data of cytotoxicity with those of ROS production by plotting cell viability (%) vs. DCFH positive cells (%). Figure 6a (HTLA-230) and Figure 6b (HTLA-ER) show the obtained dispersion graphs at 24, 48, and 72 h of exposure.Moreover, in HTLA-230 cells treated with 10 µM 4I for 72 h, H 2 O 2 levels were 2-fold higher than in the control cells.In this contest, Nambiar et al. demonstrated that the antiproliferative mechanism of an analogue of noscapine in different tumour cell lines, depended on the alteration of the tubulin system that in turn depended on high ROS levels (2-3-fold higher than in the control) [38].As mentioned above, according to Nambiar, Brullo et al. demonstrated that 4I altered the microtubules [19] even if they did not investigate the effects of 4I on ROS levels.Based on these findings, we can speculate that 4I-treated HTLA-230 cells die in consequence of the microtubule alterations [19] that are probably triggered by the increased ROS production in agreement with the study of Nambiar et al. [38].

Correlation between ROS Production and Cytotoxic Effects of 4I
To confirm the possible mechanism hypothesized in Section 2.2, we correlated data of cytotoxicity with those of ROS production by plotting cell viability (%) vs. DCFH positive cells (%).The values of R 2 of the linear regressions of all dispersion graphs, obtained by the Ordinary Least Squares (OLS) method, offered information about the correlation existing between ROS levels and cell death.Specifically, a very good correlation was found in HTLA-230 cells at all times of exposure, confirming that 4I acted mainly by enhancing ROS production, whose effects were cytotoxic for ETO sensitive cells displaying insufficient antioxidant defences.With regard to HTLA-ER cells, 4I-induced cytotoxic effects were very low, especially at 24 h according to ROS decrease, probably due to the high amount of glutathione in these cells [34].As evidenced by the very low value of R 2 of the linear regression in Figure 6b (purple dispersion), the minimal cell death was not correlated to ROS production at 24 h of exposure.When HTLA-ER cells were treated with 4I for prolonged periods of time, the higher ROS production, probably due to the failure of the developed antioxidant defences of cells, was well correlated with cell deaths.Based on the findings reported by Brullo et al. [19] and Nambiar et al. [38], we can hypothesize The values of R 2 of the linear regressions of all dispersion graphs, obtained by the Ordinary Least Squares (OLS) method, offered information about the correlation existing between ROS levels and cell death.Specifically, a very good correlation was found in HTLA-230 cells at all times of exposure, confirming that 4I acted mainly by enhancing ROS production, whose effects were cytotoxic for ETO sensitive cells displaying insufficient antioxidant defences.With regard to HTLA-ER cells, 4I-induced cytotoxic effects were very low, especially at 24 h according to ROS decrease, probably due to the high amount of glutathione in these cells [34].As evidenced by the very low value of R 2 of the linear regression in Figure 6b (purple dispersion), the minimal cell death was not correlated to ROS production at 24 h of exposure.When HTLA-ER cells were treated with 4I for prolonged periods of time, the higher ROS production, probably due to the failure of the developed antioxidant defences of cells, was well correlated with cell deaths.Based on the findings reported by Brullo et al. [19] and Nambiar et al. [38], we can hypothesize that probably the increased level of ROS caused by 4I affected the cell-cycle phases by targeting the tubulin system and causing microtubules alteration, thus prompting cells death.Even if already higher than that of ETO in HTLA-ER NB cells, we enhanced the cytotoxic activity of 4I by a nanotechnological approach.To this end, 4I-loaded PA/P5based NPs (P5PA-4I NPs) were prepared by the slightly modified single emulsification technique described in the literature [39] according to Scheme 1. Upon sonication at r.t., oily NPs made of 4I, and PA dissolved in dichloromethane (DCM) (yellow spheres in Scheme 1) entrapped in P5 (blue circles in Scheme 1), were obtained dispersed in the water phase.After removal of DCM by the oil-in-water (O/W) nano-emulsion stabilized by PA, an aqueous dispersion of P5PA-4I NPs was achieved, which was washed with DCM to remove the not encapsulated PA and/or 4I.Lyophilization of the aqueous dispersion provided solid P5PA-4I NPs.In parallel, we prepared P5PA NPs by the same method and in the same conditions without using 4I.No additional surfactant or other additive was used, except for the biocompatible fatty acid PA which, by interacting with P5 through hydrogen bonds, stabilized the O/W nano-emulsion [30].The employed concentration of PA in both cases <30 mM allowed to avoid the emulsion inversion which has reported to occur for PA concentrations >50 mM [30].P5PA NPs (337.5 mg) and P5PA-4I NPs (402.0 mg) were obtained as pale-brown glassy solids (Figure S1, Supplementary Materials), which were stored in a dryer on P2O5 for further analyses.

Particles Characterization
We characterized P5PA and P5PA-4I particles by optical microscopy, dynamic light scattering analyses and flow cytometric experiments.

Morphology of P5PA and P5PA-4I by Optical Microscopy
The morphology of P5PA and of P5PA-4I were investigated by optical microscopy (OM) analysis and compared with that of P5 particles.In the performed experiments, first powdery samples were observed (Figure 7), then sonicated aqueous dispersions of P5, P5PA and P5PA-4I were examined (Figure 8).Analogously, PA/P5-based NPs (P5PA NPs) were obtained without using 4I.Table 3 collects useful experimental data concerning the preparation of P5PA and P5PA-4I NPs.Upon sonication at r.t., oily NPs made of 4I, and PA dissolved in dichloromethane (DCM) (yellow spheres in Scheme 1) entrapped in P5 (blue circles in Scheme 1), were obtained dispersed in the water phase.After removal of DCM by the oil-in-water (O/W) nano-emulsion stabilized by PA, an aqueous dispersion of P5PA-4I NPs was achieved, which was washed with DCM to remove the not encapsulated PA and/or 4I.Lyophilization of the aqueous dispersion provided solid P5PA-4I NPs.In parallel, we prepared P5PA NPs by the same method and in the same conditions without using 4I.No additional surfactant or other additive was used, except for the biocompatible fatty acid PA which, by interacting with P5 through hydrogen bonds, stabilized the O/W nano-emulsion [30].The employed concentration of PA in both cases <30 mM allowed to avoid the emulsion inversion which has reported to occur for PA concentrations >50 mM [30].P5PA NPs (337.5 mg) and P5PA-4I NPs (402.0 mg) were obtained as pale-brown glassy solids (Figure S1, Supplementary Materials), which were stored in a dryer on P 2 O 5 for further analyses.

Particles Characterization
We characterized P5PA and P5PA-4I particles by optical microscopy, dynamic light scattering analyses and flow cytometric experiments.

Morphology of P5PA and P5PA-4I by Optical Microscopy
The morphology of P5PA and of P5PA-4I were investigated by optical microscopy (OM) analysis and compared with that of P5 particles.In the performed experiments, first powdery samples were observed (Figure 7), then sonicated aqueous dispersions of P5, P5PA and P5PA-4I were examined (Figure 8).P5, P5PA, as well as P5PA-4I, when observed in the solid state, appeared as aggregates of large dimensions.However, while P5 appeared to be formed by aggregates of bright crystal-like flakes (Figure 7a,b), spherical protuberances of about 200 µm could be identified in the aggregates of P5PA (Figure 7c,d).On the contrary, P5PA-4I appeared as an array of amorphous aggregates, within which dispersed microparticles of about 70 µm can be identified (Figure 7e-g, evidenced by red arrows).When the sonicated aqueous dispersions of P5, P5PA and P5PA-4I were analysed, separated beads of smaller dimensions, which could be micro-aggregates of the NPs later detected in the DLS analyses (see the following Section 2.5.2), were observed for all samples (Figure 8, evidenced by red circles or red arrows) especially when the meniscus of the water drop on the glass-slide was examined (Figure 8b,c (P5), Figure 8e,f (P5PA NPs), Figure 8h,i,j (P5PA-4I NPs).Interestingly, even if the concentrations of dispersions were similar for all samples, an increasing amount of dispersed material was observed going from the dispersion of P5 (Figure 8a), to that of P5PA (Figure 8d) and then to that of P5PA-4I (Figure 8g).This finding evidenced a higher tendency of P5 to settle down and a greater stability of the aqueous dispersions of P5PA and P5PA-4I due to the stabilizing action of PA [30].Moreover, while the particles of P5 appeared as spherical beads, those of P5PA and of P5PA-4I were morphologically more irregular.Curiously, during the analyses, after an initial inertia of the dispersed particles, an ever more rapid migration was observed from the centre of the drop towards its meniscus where they accumulated, tending to form larger aggregates.As an example of this phenomenon, a link to a video (Video S1) has been included here and in Supplementary Materials, showing the described rapid migration of P5PA-4I NPs (https://clipchamp.com/watch/O9s7mm5bxkS), (accessed on 28 September 2023).

Particle Size, Zeta Potential (ζ-p) and Polydispersity Index (PDI) of P5PA and P5PA-4 by DLS Analyses
The hydrodynamic diameter (Z-AVE, nm) and PDI of P5PA and P5PA-4I NPs were determined by DLS analysis, while ζ-p measurements were carried out to determine their surface charge (mV).The results have been reported both in Table 4 and in Figure 9.While the previously reported particles of P5 alone showed an average size of 334 nm with a PDI of 1.012, those of both P5PA and P5PA-4I showed larger sizes of 516.4 and 541.5 nm and significantly lower DPIs of 0.391 and 0.195, respectively.Probably, the inner oily core made of PA or PA and 4I decorated in the surface by P5, significantly increased both the usual dimensions of PA NPs obtainable by emulsion techniques (about 100-158 nm) [29,40] and those of P5 NPs previously prepared by radical polymerization and solvent-antisolvent precipitation method [31].By comparing the size of P5PA-4I NPs with that of empty P5PA NPs, we can assume that the larger size of the first ones was due to the incorporation of 4I [41].Anyway, it is known that nano-emulsion techniques could provide nanoparticles in the size range of 20-1000 nm [42] and that PA-based NPs with dimensions in the range 500-567 nm have been reported by Yan et al. [43].Concerning the significantly lower polydispersity of P5PA and P5PA-4I NPs with respect to P5, it was due to the emulsification method with respect to other methods that allow us to obtain NPs with lower PDI.In this context, PA-modified human serum albumin paclitaxel nanoparticles have been recently reported showing PDI values of about 0.2 [40], while PA-containing NPs were developed by He et al. having PDI in the range 0.120-0.147[29].According to this latter study, the presence of PA in NPs caused the reduction of the PDI value of doxorubicin (DOX)-loaded PLGA NPs from 0.259 to 0.147, thus confirming the contribute of PA in reducing the very large PDI of original P5 NPs.Curiously, while the encapsulation of DOX in PLGA/PA NPs reported by He and co-workers caused a significant increasing in the DPI values [29], in our case the encapsulation of 4I favoured a remarkably decrease in PDI from 0.391 to 0.195.Values of 0.2 and below are most commonly deemed acceptable in practice for polymer-based nanoparticle materials finalized to drug delivery [44].The ζ-p of both P5PA (+6.97 mV) and P5PA-4I NPs (+8.38 mV) were positive but much lower than the ζ-p of P5 (+58 mV), probably due to the presence of PA, which demonstrated negative values of ζ-p [29,41].Although polymer particles with high positive ζ-p are reported to be capable of faster absorption on cells' surface by electrostatic interactions, with a possible easier internalization than particles with negative ζ-p [31], the low ζ-p and cationic character of NPs developed here could reduce the possible activity as membrane disruptors and the cytotoxic effects on normal cells.In fact, it was reported that low positive ζ-p of gelatine nanoparticles loaded with cryptolepine showed low haemolytic effects on human blood [45], while another study found that high positive or negative ζ-p of nanobubbles caused haemolysis of red blood cells [46].While the previously reported particles of P5 alone showed an average size of 334 nm with a PDI of 1.012, those of both P5PA and P5PA-4I showed larger sizes of 516.4 and 541.5 nm and significantly lower DPIs of 0.391 and 0.195, respectively.Probably, the inner oily core made of PA or PA and 4I decorated in the surface by P5, significantly increased both the usual dimensions of PA NPs obtainable by emulsion techniques (about 100-158 nm) [29,40] and those of P5 NPs previously prepared by radical polymerization and solvent-antisolvent precipitation method [31].By comparing the size of P5PA-4I NPs with that of empty P5PA NPs, we can assume that the larger size of the first ones was due to the incorporation of 4I [41].Anyway, it is known that nano-emulsion techniques could provide nanoparticles in the size range of 20-1000 nm [42] and that PA-based NPs with dimensions in the range 500-567 nm have been reported by Yan et al. [43].Concerning the significantly lower polydispersity of P5PA and P5PA-4I NPs with respect to P5, it was due to the emulsification method with respect to other methods that allow us to obtain NPs with lower PDI.In this context, PA-modified human serum albumin paclitaxel nanoparticles have been recently reported showing PDI values of about 0.2 [40], while PA-containing NPs were developed by He et al. having PDI in the range 0.120-0.147[29].According to this latter study, the presence of PA in NPs caused the reduction of the PDI value of doxorubicin (DOX)-loaded PLGA NPs from 0.259 to 0.147, thus confirming the contribute of PA in reducing the very large PDI of original P5 NPs.Curiously, while the encapsula-

Estimation of Particles Size and Complexity Distributions by Cytofluorimetric Analyses
Cytofluorimetric analyses were performed on clear dispersions of P5, P5PA and P5PA-4I to further investigate their particle size and complexity distributions.Flow cytometry is a potent technology that rapidly analyses single cells or particles suspended in deionized water or in a buffered salt-based solution, while they flow past single or multiple lasers [47].Each particle can be analysed for both visible light scatter and for one or multiple fluorescence parameters [48].Concerning visible light scatter, it is measured in two different directions, the forward direction (Forward Scatter or FSC) and at 90 • (Side Scatter or SSC).FSC values are proportional to the diameter of the cell or particle, while SSC measurements to their complexity or granularity [48,49].Light scatter is independent of fluorescence [48].In our case, a dispersion of unstained polystyrene particles with 1 micron diameter was used as the standard to calculate the diameters of P5, P5PA and P5PA-4I, while Type I deionized water was used as the control.Several types of plots were obtained, which were reported in Figures S2 and S3 (Supplementary Materials) and in Figures 10-12.
Int. J. Mol.Sci.2023, 24, x FOR PEER REVIEW 14 Figure 13 shows a comparison between the histogram plots of FSC (proportiona size distributions) (a) and SSC (proportional to materials complexity) (b) of all sampl      The mean and median FSC values of water, P5, P5PA, and P5PA-4I were used to estimate the diameter of their particles against that of standard beads (1000 nm), while the mean and median SSC values were used to estimate the complexity of particles.Interestingly, the diameter of P5 particles perfectly matched that provided by DLS analyses [31].DLS provided a value slightly higher (334 vs. 317 nm) because it measures the hydrodynamic diameter of particles that are larger than the diameter of the not solvated particles.On the contrary, the size of P5PA and P5PA NPs was significantly higher than that found in the DLS analyses (988 and 1094 vs.516 and 542 nm).This because, while flow cytometry is a static light scattering technique in which single particles scatter light elastically [50], DLS is a dynamic quasi-elastic light scattering technique based on the diffusion properties of particles in a solution over time, which primarily measures their Brownian motion.As a consequence, larger particles tending to settle are not or are barely perceived by the instrument, thus shifting the maximum of the pseudo-gaussian size distribution toward minor dimensions.However, also in the flow cytometry analyses as in the DLS ones, the difference in size between P5PA and P5PA-4I was almost proportionally respected.
Figure 13 shows a comparison between the histogram plots of FSC (proportional to size distributions) (a) and SSC (proportional to materials complexity) (b) of all samples.
Light orange graphs referred to standard beads.Figure 13a evidenced that the size distributions of P5PA and P5PA-4I were very similar to each other with mean and median values like that of standard beads.Anyway, since having a very large coefficient of variation (CV%), their size distributions also comprehended smaller particles, as those detected in the DLS analyses.Analogously, Figure 13b highlighted that the less complex material was P5 consisting only of the monomer M4 and dimethylacrylamide (DMAA) [31], while complexity increases in P5PA, containing M4, DMAA and PA and increases slightly again in P5PA-4I also containing 4I.

Principal Component Analysis (PCA) on Statistics by Flow Cytometry
All statistics data were arranged in a 4 × 29 matrix of 116 variables that was processed by using the principal components analysis (PCA) [51].PCA allowed us to visualize the reciprocal positions occupied by standard beads, P5, P5PA NPs and P5PA-4I NPs in the scores plot of component 1 (PC1 explaining the 77.9% of variance) vs. component 2 (PC2 explaining the 20.6% of variance) (Figure S4).Samples located close to each other along either component PC1 or PC2 had similar statistics, while those placed far apart had different statistics.
According to the score plot showed in Figure S4, the samples were well-separated both on PC1 and on PC2.On PC1 they were located on the base of their size and complexity, while on PC2 they were clustered on the base of their chemical composition.Particularly, on PC1 going from the bottom of the score plot (negative scores) to the top (positive scores) both the size and the complexity of materials increases.Differently, on PC2, synthetic materials were located at positive scores, while commercial polystyrene beads were positioned at negative scores.Light orange graphs referred to standard beads.Figure 13a evidenced that the size distributions of P5PA and P5PA-4I were very similar to each other with mean and median values like that of standard beads.Anyway, since having a very large coefficient of variation (CV%), their size distributions also comprehended smaller particles, as those detected in the DLS analyses.Analogously, Figure 13b highlighted that the less complex material was P5 consisting only of the monomer M4 and dimethylacrylamide (DMAA) [31], while complexity increases in P5PA, containing M4, DMAA and PA and increases slightly again in P5PA-4I also containing 4I.

Principal Component Analysis (PCA) on Statistics by Flow Cytometry
All statistics data were arranged in a 4 × 29 matrix of 116 variables that was processed by using the principal components analysis (PCA) [51].PCA allowed us to visualize the   In particular, Figure 14 highlighted as in the spectrum of P5PA NPs that we can observe bands that are peculiar for both P5 and PA.From the left side of the spectrum, we found the broad and weak band of the NH stretching of P5 (3600-3200 cm −1 ), two intense bands relative to the CH stretching of the numerous methylene groups of PA (2916 and 2848 cm −1 ), which surmounted those weaker of P5, and two intense bands relative to the C=O stretching of the carboxylic group of PA (1699 cm −1 ) and to the C=O stretching of the amide groups of P5 (1616 cm −1 ).Moreover, in the fingerprint region of the spectrum of P5PA, we can observe many bands belonging to functional groups existing in PA, and not observable in the spectrum of P5, including the bands at 1472, 1430, 940 and 720 cm −1 .On the contrary, a band non-present in the spectrum of PA but existing in that of P5 is detectable at 1143 cm −1 , thus further confirming the presence of P5 in the obtained NPs. Figure 15, showing the comparison between the empty NPs, the ingredient (4I) and the NPs loaded with 4I, highlighted that in the spectrum of P5PA-4I NPs (green), in addition to the bands observed in the light blue spectrum of P5PA in Figure 14 (3422, 2916, 2848, 2679, 1699 and 1622 cm −1 ), new bands peculiar of 4I, such as bands at 3292 (CH aromatic stretching), 1406, 1270, 1140, 1003, 938, 861, 697 and 620 cm −1 , were observable, thus confirming the success of the encapsulation reaction.
explaining the 20.6% of variance) (Figure S4).Samples located close to each other along either component PC1 or PC2 had similar statistics, while those placed far apart had different statistics.
According to the score plot showed in Figure S4, the samples were well-separated both on PC1 and on PC2.On PC1 they were located on the base of their size and complexity, while on PC2 they were clustered on the base of their chemical composition.Particularly, on PC1 going from the bottom of the score plot (negative scores) to the top (positive scores) both the size and the complexity of materials increases.Differently, on PC2, synthetic materials were located at positive scores, while commercial polystyrene beads were positioned at negative scores.

Chemometric Assisted ATR-FTIR Analyses
ATR-FTIR analyses were carried out on 4I, PA, P5, P5PA NPs and P5PA-4I NPs to have qualitative indication of the chemical structure and composition of P5PA and of P5PA-4I NPs.Figures 14 and 15 show comparisons of the obtained spectra.In particular, Figure 14 highlighted as in the spectrum of P5PA NPs that we can observe bands that are peculiar for both P5 and PA.From the left side of the spectrum, we found the broad and weak band of the NH stretching of P5 (3600-3200 cm −1 ), two intense bands relative to the CH stretching of the numerous methylene groups of PA (2916 and 2848 cm −1 ), which surmounted those weaker of P5, and two intense bands relative to the C=O stretching of the carboxylic group of PA (1699 cm −1 ) and to the C=O stretching of the amide groups of P5 (1616 cm −1 ).Moreover, in the fingerprint region of the spectrum of P5PA, we can observe many bands belonging to functional groups existing in PA, and not

Principal Components Analysis (PCA) on the ATR-FTIR Data
As explained in the previous section, just by observing the ATR-FTIR spectra in Figures 14 and 15, the presence of PA with P5 in P5PA NPs and of 4I in P5PA-4I NPs was unequivocable.Anyway, we found further confirmation processing the ATR-FTIR spectral data of all samples using PCA as previously made with statistics data by cytofluorimetric analyses.PCA allowed us to visualize the reciprocal positions occupied by 4I, P5, PA, P5PA NPs and P5PA-4I NPs in the scores plot of PC1 (explaining the 64.9% of variance) vs. PC2 (explaining the 21.8% of variance) (Figure 16).In this case, samples located close to each other along either component PC1 or PC2 are structurally similar, while those placed far apart are structurally different.As observable, PC1 differentiated between empty NPs (P5PA), which were located at positive scores as with their components (P5 and PA) and NPs loaded with 4I, which were positioned at negative scores as 4I, thus evidencing structural similarities between the obtained NPs and their ingredients.Anyway, empty and loaded NPs were very close to the zero-score and to each other, evidencing a structural similarity even between them (both are made of P5PA).On PC2, P5PA and P5PA-4I NPs results were placed at score zero, confirming the structural similarity previously evidenced on PC1.The minor distance between both types of NPs and P5 respect to PA, recognized this copolymer as the component loaded in a major amount.

Determination of the Exact Amount of 4I Loaded in P5PA-4I NPs
The exact amount of 4I contained in an exactly weighted quantity of P5PA-4I NPs was estimated using the 4I calibration curve constructed as reported in the Experimental Section and as shown in Figure S5.
Once obtained, the quantity of 4I (mg) present in the total amount of P5PA-4I prepared (mg), it was used to calculate the values of drug loading (DL%) and entrapment efficiency (EE%).To this end, we dispersed P5PA-4I NPs in MeOH, obtaining a fine suspension, which was vigorously stirred to promote the full release of 4I.The sample was centrifugated and the clear solution was reacted with the Schiff reagent up to a magenta coloration.Considering the amount of 4I mathematically estimated according to the initial loading (Table 3), aliquots of the obtained coloured solution were diluted 1:10 to remain within the limits of the calibration curve before UV-Vis analysis at 543.88 nm.The obtained Abs values were used to determine the 4I concentration (mg/mL) by employing the equation shown in Figure S5.Determinations were made in triplicate and reported in Table 6.
The content of 4I in the total amount of P5PA-4I prepared (402.0 mg) was 83.9 mg, DL (%) was 20.87%, thus confirming the estimated value reported in Table 2 and the EE (%) was 96.55%.In this regard, the EE% of P5PA-4I was very good, comparable to that reported by Sari et al. [52], and close to 100% as reported recently [53].On the contrary, the DL% was much higher (20.9% vs. 0.74%) than that obtained by the same authors [53], and that reported by other authors for lipid core nano-capsules [54].As observable, PC1 differentiated between empty NPs (P5PA), which were located at positive scores as with their components (P5 and PA) and NPs loaded with 4I, which were positioned at negative scores as 4I, thus evidencing structural similarities between the obtained NPs and their ingredients.Anyway, empty and loaded NPs were very close to the zero-score and to each other, evidencing a structural similarity even between them (both are made of P5PA).On PC2, P5PA and P5PA-4I NPs results were placed at score zero, confirming the structural similarity previously evidenced on PC1.The minor distance between both types of NPs and P5 respect to PA, recognized this copolymer as the component loaded in a major amount.

Determination of the Exact Amount of 4I Loaded in P5PA-4I NPs
The exact amount of 4I contained in an exactly weighted quantity of P5PA-4I NPs was estimated using the 4I calibration curve constructed as reported in the Experimental Section and as shown in Figure S5.
Once obtained, the quantity of 4I (mg) present in the total amount of P5PA-4I prepared (mg), it was used to calculate the values of drug loading (DL%) and entrapment efficiency (EE%).To this end, we dispersed P5PA-4I NPs in MeOH, obtaining a fine suspension, which was vigorously stirred to promote the full release of 4I.The sample was centrifugated and the clear solution was reacted with the Schiff reagent up to a magenta coloration.Considering the amount of 4I mathematically estimated according to the initial loading (Table 3), aliquots of the obtained coloured solution were diluted 1:10 to remain within the limits of the calibration curve before UV-Vis analysis at 543.88 nm.The obtained Abs values were used to determine the 4I concentration (mg/mL) by employing the equation shown in Figure S5.Determinations were made in triplicate and reported in Table 6.The content of 4I in the total amount of P5PA-4I prepared (402.0 mg) was 83.9 mg, DL (%) was 20.87%, thus confirming the estimated value reported in Table 2 and the EE (%) was 96.55%.In this regard, the EE% of P5PA-4I was very good, comparable to that reported by Sari et al. [52], and close to 100% as reported recently [53].On the contrary, the DL% was much higher (20.9% vs. 0.74%) than that obtained by the same authors [53], and that reported by other authors for lipid core nano-capsules [54].

Potentiometric Titrations of P5PA and of P5PA-4I NPs
Upon titrations of both P5PA and P5PA-4I NPs dispersed in water as described in the Experimental Section, by plotting the measured pH values vs. the aliquots of HCl 0.1 N added, the titration curves of the samples were obtained as shown in Figure 17a.The first derivative (FD) curves of the titration lines shown in Figure 17b were obtained by computing the values of dpH/dV and plotting them against the corresponding volumes of HCl 0.1 N. The maxima of the FD lines represent the different titration end points.For comparison purposes, P5 alone was titrated in the same conditions as P5PA and P5PA-4I NPs and the titration curve, as well as the related FD are available in Figure S6 in the Supplementary Materials file.The representative titration curve of P5PA (Figure 17a) and related FD (Figure 17b) evidenced that the potentiometric titration of the aqueous solution of P5PA added with NaOH 0.1 N (pH = 10.19)exhibited mainly three successive end points, upon the adding of 1.3, 3.5 and 8.5 mL HCl 0.1N, corresponding to the major maxima of 2.15, 0.86 and 1.66 (Figure 17b).As reported by the group of Zu in 2021, the first end point corresponded to the titration of any excess NaOH [55].
Due to the presence of PA, which at a physiological pH of 7.4 is in the anionic form [56], the second end point (maximum 0.86) occurring at pH = 7.12 corresponded to the titration of palmitate, while the third one can be ascribed to the protonation of the amine groups of P5.In these conditions, the number of millimoles of PA and primary amine groups can be obtained using the volumes of HCl 0.1 N added between the first and the second and between the second and the third end point (2.2 mL and 5.0 mL), respectively.As reported in Table 7 the milliequivalents of PA and those of the primary amine groups were 3.6 ± 0.03 mmol/g and 8.3 ± 0.03 mmol/g, respectively.The milliequivalents of NH2 The representative titration curve of P5PA (Figure 17a) and related FD (Figure 17b) evidenced that the potentiometric titration of the aqueous solution of P5PA added with NaOH 0.1 N (pH = 10.19)exhibited mainly three successive end points, upon the adding of 1.3, 3.5 and 8.5 mL HCl 0.1N, corresponding to the major maxima of 2.15, 0.86 and 1.66 (Figure 17b).As reported by the group of Zu in 2021, the first end point corresponded to the titration of any excess NaOH [55].
Due to the presence of PA, which at a physiological pH of 7.4 is in the anionic form [56], the second end point (maximum 0.86) occurring at pH = 7.12 corresponded to the titration of palmitate, while the third one can be ascribed to the protonation of the amine groups of P5.In these conditions, the number of millimoles of PA and primary amine groups can be obtained using the volumes of HCl 0.1 N added between the first and the second and between the second and the third end point (2.2 mL and 5.0 mL), respectively.As reported in Table 7 the milliequivalents of PA and those of the primary amine groups were 3.6 ± 0.03 mmol/g and 8.3 ± 0.03 mmol/g, respectively.The milliequivalents of NH 2 groups contained in 1 g of P5 (12.5 ± 0.03 mmol/g) computed on the basis of its titration results (Figure S6, Supplementary Materials) have been reported in Table 7 for comparison purposes [31].In this regard, considering that, 1 g of P5PA should contain 0.667 g P5 (Table 2), the milliequivalents of primary amine groups per gram of P5 estimated here were 12.4 mmol/g, perfectly in accordance with the result obtained titrating P5 alone (12.4 vs. 12.5 mmol/g, error = −0.4%).The titration curve of the aqueous solution of P5PA-4I added with NaOH 0.1 (pH = 9.20) demonstrated an additional maximum, since the groups that can undergo titration are the hydroxyl group deriving by the NaOH added, the carboxylate group of PA, the primary amine groups of P5 and finally the two weakly basic nitrogen atoms (the sp 2 nitrogen atom of the pyrazole ring and the nitrogen atom of the Schiff base) of 4I.As shown in Figure 17b, the FD of the titration curve of P5PA-4I revealed four major maxima (0.70, 0.60, 1.60 and 1.58) corresponding to the addition of 1.5, 4.5, 7.5 and 8 mL of HCl 0.1N and representing the titration end points of NaOH, PA, primary amine groups of P5 and the two basic nitrogen atoms of the imidazo-pyrazole.We have used the volume of HCl employed between the first end point and the second one and that employed between the second and the fourth end point to estimate the equivalents of PA and those of the total basic nitrogen atoms of P5 and 4I, respectively.As reported in Table 7, the milliequivalents of PA and of basic nitrogen atoms were 4.9 ± 0.03 mmol/g and 5.8 ± 0.03 mmol/g, respectively.Additional speculations on possible uses of titration data are available in Supplementary Materials (Section S1).

Buffer Capacity
Cationic materials such as those developed here and those used to bind and transport genetic material inside the cell for gene-therapy purposes, are reported to be internalized by several methods including endocytosis [57].Once inside the cells by endocytosis, cationic materials are within the endosome, and need to escape it so as to not be degraded into the lysosomes.It was reported that materials capable of avoiding lysosomal degradation act as a "proton sponge", attracting protons inside the endosome, thus causing osmotic swelling and bursting [57].In this context, the proton sponge activity of cationic macromolecules mainly depends on their buffer capacity (β = dV HCl )/d(pH)) [58], as well as on their average buffer capacity (β AVE ) defined as the volume of HCl necessary to cause a variation of pH equal to one unit in the pH range 4.5-7.5 [59].Particularly, the higher the values of β and β AVE , the higher the proton sponge activity, the faster the lysosome escape and the longer the residence time in cells.Thus, to predict the capability of P5PA and P5PA-4I NPs to avoid premature degradation and inactivation, we evaluated their β and β AVE by data of potentiometric titration.The max β values and values of β AVE determined for P5PA and P5PA-4I NPs have been reported in Table 8 and compared with those obtained for P5 and for commercial branched polyethyleneimine (b-PEI 25K), a reference standard recognized for having good buffer capacity [60].By reporting in graphs all the β values calculated for P5, P5PA, P5PA-4I NPs and b-PEI vs. the values of corresponding pH, their buffer capacity curves were obtained (Figures 18a and S7), while in Figure 18b the β AVE values computed for all samples have been reported using a bars graph.By reporting in graphs all the β values calculated for P5, P5PA, P5PA-4I NPs and b-PEI vs. the values of corresponding pH, their buffer capacity curves were obtained (Figures 18a and S7), while in Figure 18b the βAVE values computed for all samples have been reported using a bars graph.As evidenced in Figure S7 in Supplementary Materials, b-PEI has two maxima of β (Table 8) in the pH range of interest (pH = 6.81 and 7.33), which confer b-PEI a buffer capacity suitable to exert an adequate proton sponge activity [60].Anyway, the maxima of b-PEI are not visible in Figure 18a because almost 10-fold lower than the maximum of P5 (0.6667 at pH = 6.10) and extremely lower than the maxima of P5PA and P5PA-4I.Particularly, P5PA demonstrated two maxima at pH = 6.18 and 6.76, while P5PA-4I showed two maxima of equal height (4.5455) and even more intense than those of P5PA at pH = 6.49and 7.45, thus assuring strong proton sponge activity, rapid lysosomal escape and high residence time in cells.Curiously, as reported in Figure 18b, while the buffer capacity of b-PEI was lower than that of P5, its βAVE was more than two-fold higher, thus justifying its reported high efficiency as a proton sponge [60].However, our P5PA and P5PA-4I NPs demonstrated the highest average buffer capacity as well, thus confirming what was previously evidenced by data of buffer capacity.

Evaluation of the Chemical Stability of P5PA and P5PA-4I NPs Dispersions over Time
To evaluate the chemical stability over time at room temperature of both P5PA and P5PA-4I NPs aqueous dispersions, potentiometric titrations of both materials were carried out after 1, 5, 10 and 15 days from the first one performed, in the same conditions obtaining the related titration data.All obtained titration data (pH values) were arranged in a matrix 24 × 10 of 240 variables, which was subjected to PCA as previously described for cytofluorimetric and ATR-FTIR data.Figure 19 shows the score plot of PC1 (explaining As evidenced in Figure S7 in Supplementary Materials, b-PEI has two maxima of β (Table 8) in the pH range of interest (pH = 6.81 and 7.33), which confer b-PEI a buffer capacity suitable to exert an adequate proton sponge activity [60].Anyway, the maxima of b-PEI are not visible in Figure 18a because almost 10-fold lower than the maximum of P5 (0.6667 at pH = 6.10) and extremely lower than the maxima of P5PA and P5PA-4I.Particularly, P5PA demonstrated two maxima at pH = 6.18 and 6.76, while P5PA-4I showed two maxima of equal height (4.5455) and even more intense than those of P5PA at pH = 6.49and 7.45, thus assuring strong proton sponge activity, rapid lysosomal escape and high residence time in cells.Curiously, as reported in Figure 18b, while the buffer capacity of b-PEI was lower than that of P5, its β AVE was more than two-fold higher, thus justifying its reported high efficiency as a proton sponge [60].However, our P5PA and P5PA-4I NPs demonstrated the highest average buffer capacity as well, thus confirming what was previously evidenced by data of buffer capacity.

Evaluation of the Chemical Stability of P5PA and P5PA-4I NPs Dispersions over Time
To evaluate the chemical stability over time at room temperature of both P5PA and P5PA-4I NPs aqueous dispersions, potentiometric titrations of both materials were carried out after 1, 5, 10 and 15 days from the first one performed, in the same conditions obtaining the related titration data.All obtained titration data (pH values) were arranged in a matrix 24 × 10 of 240 variables, which was subjected to PCA as previously described for cytofluorimetric and ATR-FTIR data.Figure 19 shows the score plot of PC1 (explaining the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance) with the confidence ellipses at 95% (red solid line), 99% (red dashed line) and 99.9% (red dotted line).The confidence ellipses enclosed samples at different levels of confidence, from the more restrictive (95%) to the larger one (99.9%)not significantly different in terms of titration data, thus indicating chemical stability.
Int. J. Mol.Sci.2023, 24, x FOR PEER REVIEW 24 of 39 the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance) with the confidence ellipses at 95% (red solid line), 99% (red dashed line) and 99.9% (red dotted line).The confidence ellipses enclosed samples at different levels of confidence, from the more restrictive (95%) to the larger one (99.9%)not significantly different in terms of titration data, thus indicating chemical stability.Based on the results in Figure 19, on PC1 samples that were clustered in a manner dependent on the presence or not of 4I, with samples containing 4I located at negative scores, while those without 4I were at positive values.Collectively, all samples of both materials were comprised within the more restrictive ellipse, evidencing that no significant difference existed in titrations data measured up to 15 days, thus establishing for good stability of both types of NPs during this monitoring time.Additionally, while P5PA NPs showed samples P5PA_1 and P5PA_5 within the confidence ellipse, but not overlapped with the other samples of the group, no sample in the group of compounds containing 4I was clearly separated from others, thus indicating very minimal differences and a stability higher than that of P5PA NPs.
To further confirm the absence of outliers, intending compounds with titration data significantly different from those of the first titrated ones, among the samples analysed, we make Q and T 2 tests using the diagnostic tools of CAT.We obtained both separate Q and T 2 contribution plots (Figures S8a,b, respectively, in Supplementary Materials), and the influencing plot of T 2 Hotelling index vs.Q index (Figure S8c).All plots evidenced that no outlier existed among the analysed samples, which were located all within the solid lines, indicating the more restrictive critical values (p = 0.05).Then, we performed further titrations of our samples after 20 days in aqueous dispersion at room temperature and arranged the measured data in a matrix 2 × 24 of 48 variables that was processed by PCA, obtaining the score plot reported in Figure S9 in Supplementary Materials.This new score plot confirmed that P5PA-type samples located at positive scores while the P5PA-4I-type ones at negative scores.We used this new data as an external data set and projected them in the data set of the ten samples previously processed, which acted as a training set representing a population of not-degraded samples.Figure 20 shows the obtained score plot, Based on the results in Figure 19, on PC1 samples that were clustered in a manner dependent on the presence or not of 4I, with samples containing 4I located at negative scores, while those without 4I were at positive values.Collectively, all samples of both materials were comprised within the more restrictive ellipse, evidencing that no significant difference existed in titrations data measured up to 15 days, thus establishing for good stability of both types of NPs during this monitoring time.Additionally, while P5PA NPs showed samples P5PA_1 and P5PA_5 within the confidence ellipse, but not overlapped with the other samples of the group, no sample in the group of compounds containing 4I was clearly separated from others, thus indicating very minimal differences and a stability higher than that of P5PA NPs.
To further confirm the absence of outliers, intending compounds with titration data significantly different from those of the first titrated ones, among the samples analysed, we make Q and T 2 tests using the diagnostic tools of CAT.We obtained both separate Q and T 2 contribution plots (Figure S8a,b, respectively, in Supplementary Materials), and the influencing plot of T 2 Hotelling index vs.Q index (Figure S8c).All plots evidenced that no outlier existed among the analysed samples, which were located all within the solid lines, indicating the more restrictive critical values (p = 0.05).Then, we performed further titrations of our samples after 20 days in aqueous dispersion at room temperature and arranged the measured data in a matrix 2 × 24 of 48 variables that was processed by PCA, obtaining the score plot reported in Figure S9 in Supplementary Materials.This new score plot confirmed that P5PA-type samples located at positive scores while the P5PA-4I-type ones at negative scores.We used this new data as an external data set and projected them in the data set of the ten samples previously processed, which acted as a training set representing a population of not-degraded samples.Figure 20 shows the obtained score plot, where the new samples titrated after standing in dispersion for 20 days,  Based on the results shown in Figure 20, evidencing both P5PA_20 and P5PA4I_20 located within the most restrictive confidence ellipse (p = 0.05), it was established that also after 20 days no significant difference was detected in the titration data, thus further establishing a good stability over time of our materials.Further titrations were performed after 25, 30 and 40 days from the first one and data were treated as just described with similar results.

Evaluation of 4I In Vitro Release Profile
The in vitro release profile of 4I from P5PA-4I NPs was investigated by the dialysis method as described in the Experimental Section.In parallel, the release of 4I from a 4I suspension in PBS was monitored in the same conditions.The obtained concentrations were used to compute the cumulative drug release percentages of 4I over time, which were plotted vs. times obtaining the curves shown in Figure 21.Based on the results shown in Figure 20, evidencing both P5PA_20 and P5PA4I_20 located within the most restrictive confidence ellipse (p = 0.05), it was established that also after 20 days no significant difference was detected in the titration data, thus further establishing a good stability over time of our materials.Further titrations were performed after 25, 30 and 40 days from the first one and data were treated as just described with similar results.

Evaluation of 4I In Vitro Release Profile
The in vitro release profile of 4I from P5PA-4I NPs was investigated by the dialysis method as described in the Experimental Section.In parallel, the release of 4I from a 4I suspension in PBS was monitored in the same conditions.The obtained concentrations were used to compute the cumulative drug release percentages of 4I over time, which were plotted vs. times obtaining the curves shown in Figure 21.Based on the results shown in Figure 20, evidencing both P5PA_20 and P5PA4I_20 located within the most restrictive confidence ellipse (p = 0.05), it was established that also after 20 days no significant difference was detected in the titration data, thus further establishing a good stability over time of our materials.Further titrations were performed after 25, 30 and 40 days from the first one and data were treated as just described with similar results.

Evaluation of 4I In Vitro Release Profile
The in vitro release profile of 4I from P5PA-4I NPs was investigated by the dialysis method as described in the Experimental Section.In parallel, the release of 4I from a 4I suspension in PBS was monitored in the same conditions.The obtained concentrations were used to compute the cumulative drug release percentages of 4I over time, which were plotted vs. times obtaining the curves shown in Figure 21.As is observable, the release profiles of 4I from P5PA-4I and from its suspension were very similar and characterized by a burst release within the first four hours.A very slow release was observed up to 24 h, followed by an increment in the release rate, especially from P5PA-4I, in the subsequent four hours leading to a linear sustained release during the subsequent 44 h up to the 72 h of the monitoring.The main differences between the release of 4I from P5PA-4I NPs and that from the 4I suspension was the amount of 4I released.Notably, at any stage the 4I released from P5PA-4I NPs was about two-fold higher than that released from the suspension, thus indicating that by formulating 4I in NPs, its aqueous solubility was remarkably improved, thus assuring a higher bioavailability in a possible future oral administration.Collectively, the amount of untreated 4I released in the acceptor medium at 72 h was only the 45% of the 4I suspended in the dialysis bag, while that released by NPs was the 93% of the 4I loaded in NPs, thus assuring a systemic concentration more than two-fold higher than that achievable by not formulated 4I.Curiously, the release of 4I from the 4I suspension in PBS observed this time was very different from that previously observed by us (study non yet published), which was faster and quantitative.Probably, the higher concentration of 4I in the dialysis bag used here (4.2 mg/mL vs. 0.35 mg/mL) could have led to flocculation and aggregates formation, which hampered the release of 4I in the acceptor medium.Anyway, such phenomenon did not occur when the same concentration of 4I was transported by P5PA-4I NPs, thus allowing an almost quantitative release.

Kinetic Studies
The kinetics and main mechanisms governing the releases of 4I were investigated by fitting the data plotted in Figure 21 to the most common kinetic models [61,62].
The obtained dispersion graphs with the related linear regressions provided by Microsoft Excel software 635 using the OLS method and their equations are available in Figures S10-S14 in Supplementary Materials.The value of the coefficient of determination (R 2 ) associated with each equation was the parameter used to determine which model better fit the release data.The model with the highest R 2 value was declared the best fitting one.The R 2 values obtained for all models tested were reported in Table 9, and accordingly, the 4I release from both P5PA-4I NPs and from the 4I suspension best fit with the Higuchi kinetic model.The Higuchi kinetics are expressed by Equation ( 1): where Qt (variable y of the equation in Figure S12) is the amount of 4I released at time t, Kh is the Higuchi kinetic constant, t is time, and n is the release exponent, which in the Higuchi models is equal to 0.5, thus establishing that the mechanism that governs both the releases of 4I from NPs and from the 4I suspension is based on Fickian diffusion.The kinetic constants (Kh) corresponded to the slopes of the equations in Figure S12 and were equal to 10.12 (P5PA-4I) and 5.27 (4I suspension), thus establishing that at the same time point the 4I released from NPs was about two-times higher than from the suspension, as previously observed in Figure 21.

Cytotoxic Effects of 4I, P5PA and of P5PA-4I on NB Cells
Both NB cell populations were exposed to increasing concentrations (0.5-50 µM) of 4I, P5PA-4I NPs (administered in a dose capable of providing 0.5-50 µM 4I), and P5PA NPs (administered at the same dose of those contained in the P5PA-4I) for 24, 48 and 72 h and the effect of these treatments on cell viability was evaluated.As shown in Figure 22a,b, when administered at the same concentrations, nanotechnologically manipulated 4I provided by P5PA-4I NPs was more cytotoxic than pristine 4I, especially in HTLA-ER cells.Specifically, it reduced the cell viability by a further 10% with respect to pristine 4I, at any time of exposure tested (Figure 22b).These findings agree perfectly with the release profiles of 4I from P5PA-4I NPs and from its suspension observed previously (Section 2.9).Specifically, regardless of the time of the experiment, the amount of 4I released by NPs was always higher than that released by the suspensions.Particularly, at 72 h, the amount of 4I released by NPs was 93% against the 45% released by the 4I-suspension, thus assuring a remarkably high concentration of 4I at the target cells, which was responsible for the higher cytotoxic activity.Additionally, the time dependent cytotoxic activity of P5PA-4I NPs which markedly increased from 42 to 72 h of exposure also depended on the controlled and sustained release profile of 4I for the nano-formulation.Notably, although P5 [32] and PA [20][21][22][23][24][25] have been reported to have antiproliferative activity, P5PA per se did not induce changes in cell viability (Figure S15).The reason is probably due to the acid-base interaction between the ammonium groups of P5 and the PA, that, at physiological pH of the experimental medium, was in the carboxylate form [56], thus causing a reciprocal inactivation by providing a salt.Therefore, the cationic groups of P5, responsible for its cytotoxic [32] and antibacterial activity [31], were neutralized, determining the activity loss.
The cytotoxic effects of P5PA-4I NPs were further confirmed by calculating the IC 50 values.In fact, as reported in Table 10, this value was 1.2-, 1.4-and 1.5-fold lower (24, 48 and 72 h, respectively) in HTLA-230 cells treated with P5PA-4I NPs respect to those treated with pristine 4I.An even greater reduction of IC 50 values (1.9-, 1.5-, 1.6-fold lower) was observed in HTLA-ER cells treated with the 4I-enriched NPs compared to their treatment with 4I.Table 10.IC 50 value evaluated in HTLA-230 and HTLA-ER cells exposed to increasing concentrations of 4I and P5PA-4I NPs for 24, 48 and 72 h The IC 50 of ETO at 24 h of exposure reported by Colla et al. [34] has been also included (N.R. = not reported).

Compound
Cells IC 50  point the 4I released from NPs was about two-times higher than from the suspension, as previously observed in Figure 21.

Cytotoxic Effects of 4I, P5PA and of P5PA-4I on NB Cells
Both NB cell populations were exposed to increasing concentrations (0.5-50 µM) of 4I, P5PA-4I NPs (administered in a dose capable of providing 0.5-50 µM 4I), and P5PA NPs (administered at the same dose of those contained in the P5PA-4I) for 24, 48 and 72 h and the effect of these treatments on cell viability was evaluated.As shown in Figure 22a,b, when administered at the same concentrations, nanotechnologically manipulated 4I provided by P5PA-4I NPs was more cytotoxic than pristine 4I, especially in HTLA-ER cells.Specifically, it reduced the cell viability by a further 10% with respect to pristine 4I, at any time of exposure tested (Figure 22b).These findings agree perfectly with the release profiles of 4I from P5PA-4I NPs and from its suspension observed previously (Section 2.9).Specifically, regardless of the time of the experiment, the amount of 4I released by NPs was always higher than that released by the suspensions.Particularly, at 72 h, the amount of 4I released by NPs was 93% against the 45% released by the 4I-suspension, thus assuring a remarkably high concentration of 4I at the target cells, which was responsible for the higher cytotoxic activity.Additionally, the time dependent cytotoxic activity of P5PA-4I NPs which markedly increased from 42 to 72 h of exposure also depended on the controlled and sustained release profile of 4I for the nano-formulation.Notably, although P5 [32] and PA [20][21][22][23][24][25] have been reported to have antiproliferative activity, P5PA per se did not induce changes in cell viability (Figure S15).The reason is probably due to the acidbase interaction between the ammonium groups of P5 and the PA, that, at physiological pH of the experimental medium, was in the carboxylate form [56], thus causing a reciprocal inactivation by providing a salt.Therefore, the cationic groups of P5, responsible for its cytotoxic [32] and antibacterial activity [31], were neutralized, determining the activity loss.
(a) The cytotoxic effects of P5PA-4I NPs were further confirmed by calculating the IC50 values.In fact, as reported in Table 10, this value was 1.2-, 1.4-and 1.5-fold lower (24, 48 and 72 h, respectively) in HTLA-230 cells treated with P5PA-4I NPs respect to those treated with pristine 4I.An even greater reduction of IC50 values (1.9-, 1.5-, 1.6-fold lower) was observed in HTLA-ER cells treated with the 4I-enriched NPs compared to their treatment with 4I.
Table 10.IC50 value evaluated in HTLA-230 and HTLA-ER cells exposed to increasing concentrations of 4I and P5PA-4I NPs for 24, 48 and 72 h The IC50 of ETO at 24 h of exposure reported by Colla et al. [34] has been also included (N.R. = not reported).The application of two sample Student t test established that the IC50 values of P5PA-4I NPs were significantly lower than those of 4I in both NB cell populations and at both confidence intervals (p = 0.01 and p = 0.05), in particular in HTLA-ER cells at all times of exposure.Then, to analyse the efficacy of these compounds in counteracting the chemoresistance of HTLA-ER cells, the cytotoxic activity of 4I and of P5PA-4I NPs (0-50 µM, Figure 23) were compared with that of ETO reported by Colla [34].The results are shown in Figure S16 and in Figure 23.The application of two sample Student t test established that the IC 50 values of P5PA-4I NPs were significantly lower than those of 4I in both NB cell populations and at both confidence intervals (p = 0.01 and p = 0.05), in particular in HTLA-ER cells at all times of exposure.Then, to analyse the efficacy of these compounds in counteracting the chemoresistance of HTLA-ER cells, the cytotoxic activity of 4I and of P5PA-4I NPs (0-50 µM, Figure 23) were compared with that of ETO reported by Colla [34].The results are shown in Figure S16 and in Figure 23.As shown in Figure S16b, 10 µM 4I was significantly more cytotoxic than ETO administered at the same dose.Interestingly, a two-sample Student t test showed that 4Iinduced effects in HTLA-ER cells, already at 24 h exposure, were significantly higher (p = 0.05 and p = 0.01) than those induced by ETO.Moreover, the cytotoxic effects of P5PA-4I NPs on HTLA-ER cells were confirmed to be significantly higher than those of 4I (p = 0.05 and p = 0.01) and also higher than those of ETO (p = 0.05 and p = 0.01).In fact, the IC50 values of P5PA-4I NPs were 1.9-and 3.3-fold lower than those of 4I and ETO, respectively.Based on these findings, the embedment of 4I in P5PA NPs represents a promising nanotechnological strategy to strongly enhance the cytotoxic action of 4I as well as of other imidazo-pyrazole derivatives [19].Collectively, empty PAP5 NPs, which have been found deprived of intrinsic cytotoxic effects, could represent a safe novel delivery system capable of increasing the cytotoxic action of entrapped traditional or novel anticancer drugs.In this regard, experiments to verify the level of cytotoxicity of P5PA and P5PA-4I NPs on As shown in Figure S16b, 10 µM 4I was significantly more cytotoxic than ETO administered at the same dose.Interestingly, a two-sample Student t test showed that 4I-induced effects in HTLA-ER cells, already at 24 h exposure, were significantly higher (p = 0.05 and p = 0.01) than those induced by ETO.Moreover, the cytotoxic effects of P5PA-4I NPs on HTLA-ER cells were confirmed to be significantly higher than those of 4I (p = 0.05 and p = 0.01) and also higher than those of ETO (p = 0.05 and p = 0.01).In fact, the IC 50 values of P5PA-4I NPs were 1.9-and 3.3-fold lower than those of 4I and ETO, respectively.Based on these findings, the embedment of 4I in P5PA NPs represents a promising nanotechnological strategy to strongly enhance the cytotoxic action of 4I as well as of other imidazo-pyrazole derivatives [19].Collectively, empty PAP5 NPs, which have been found deprived of intrinsic cytotoxic effects, could represent a safe novel delivery system capable of increasing the cytotoxic action of entrapped traditional or novel anticancer drugs.In this regard, experiments to verify the level of cytotoxicity of P5PA and P5PA-4I NPs on normal cells are programmed to assess better their clinical applicability.

Effects of 4I and P5PA-4I on ROS Production in NB Cells
As reported in Section 2.2, the effects of pristine 4I (range 0-50 µM) and P5PA-4I NPs on ROS levels were investigated (Figure 24).P5PA NPs, administered to provide P5PA at the same concentration given by P5PA-4I NPs, induced a decrease in H 2 O 2 levels (Figure S15).As shown in Figure 24, P5PA-4I increased H2O2 levels in a time-and dose-dependent manner, although the effect was more evident at 72 h, because of a controlled and sustained release of 4I from the nano-formulation.In fact, compared to 4I-treated cells, H2O2 levels were increased by a further 30% after 72 h in both cell populations treated with 50 µM P5PA-4I (Figure 24).Notably, the prooxidant effects induced by 24 h ETO exposure (range 0-50 µM) in HTLA-ER cells [34] were compared to those induced by 4I and P5PA- As shown in Figure 24, P5PA-4I increased H 2 O 2 levels in a time-and dose-dependent manner, although the effect was more evident at 72 h, because of a controlled and sustained release of 4I from the nano-formulation.In fact, compared to 4I-treated cells, H 2 O 2 levels were increased by a further 30% after 72 h in both cell populations treated with 50 µM P5PA-4I (Figure 24).Notably, the prooxidant effects induced by 24 h ETO exposure (range 0-50 µM) in HTLA-ER cells [34] were compared to those induced by 4I and P5PA-4I NPs (Figure 24b).These results have been analysed and shown in Figure 25.Also in this case, when 4I was administered as a nano-formulation (P5PA-4I NPs), already at 24 h, it caused an increase in H2O2 levels in HTLA-ER cells not only higher than that caused by the pristine 4I, but also higher than that caused by ETO, at all concentrations tested, and in particular at low concentrations (0.5-5 µM).

Correlation between H2O2 Production and Cytotoxicity of P5PA-4I NPs
To validate the hypothesis of a possible relationship between the cytotoxic and prooxidant effect of P5PA-4I NPs, their correlation was tested by plotting the data of cell viability (%) vs. DCFH positive cells (%) obtained in P5PA-4I NPs-treated HTLA-230 and HTLA-ER cells.The dispersion graphs were reported in Figure 26.According to results reported in Figure 26, a correlation from discrete to good was shown both in HTLA-230 and HTLA-ER cells.Particularly, a discrete correlation was observed in HTLA-230, regardless of the time of exposure.A better correlation was observed in HTLA-ER cells and mainly for 24 h treatment, thus suggesting that, despite the high antioxidant defence in ETO resistant cells, the cytotoxic effects induced by P5PA-4I NPs were dependent on H2O2 production.On the contrary, the reduced correlation between peroxide production and cytotoxicity of P5PA-4I NPs at 48 and 72 h exposure suggested an adaptive cell response to H2O2 and the implication of other factors responsible for cancer cell death.Furthermore, these data were also confirmed by the results obtained with Also in this case, when 4I was administered as a nano-formulation (P5PA-4I NPs), already at 24 h, it caused an increase in H 2 O 2 levels in HTLA-ER cells not only higher than that caused by the pristine 4I, but also higher than that caused by ETO, at all concentrations tested, and in particular at low concentrations (0.5-5 µM).

Correlation between H 2 O 2 Production and Cytotoxicity of P5PA-4I NPs
To validate the hypothesis of a possible relationship between the cytotoxic and prooxidant effect of P5PA-4I NPs, their correlation was tested by plotting the data of cell viability (%) vs. DCFH positive cells (%) obtained in P5PA-4I NPs-treated HTLA-230 and HTLA-ER cells.The dispersion graphs were reported in Figure 26.Also in this case, when 4I was administered as a nano-formulation (P5PA-4I NPs), already at 24 h, it caused an increase in H2O2 levels in HTLA-ER cells not only higher than that caused by the pristine 4I, but also higher than that caused by ETO, at all concentrations tested, and in particular at low concentrations (0.5-5 µM).

Correlation between H2O2 Production and Cytotoxicity of P5PA-4I NPs
To validate the hypothesis of a possible relationship between the cytotoxic and prooxidant effect of P5PA-4I NPs, their correlation was tested by plotting the data of cell viability (%) vs. DCFH positive cells (%) obtained in P5PA-4I NPs-treated HTLA-230 and HTLA-ER cells.The dispersion graphs were reported in Figure 26.According to results reported in Figure 26, a correlation from discrete to good was shown both in HTLA-230 and HTLA-ER cells.Particularly, a discrete correlation was observed in HTLA-230, regardless of the time of exposure.A better correlation was observed in HTLA-ER cells and mainly for 24 h treatment, thus suggesting that, despite the high antioxidant defence in ETO resistant cells, the cytotoxic effects induced by P5PA-4I NPs were dependent on H2O2 production.On the contrary, the reduced correlation between peroxide production and cytotoxicity of P5PA-4I NPs at 48 and 72 h exposure suggested an adaptive cell response to H2O2 and the implication of other factors responsible for cancer cell death.Furthermore, these data were also confirmed by the results obtained with According to results reported in Figure 26, a correlation from discrete to good was shown both in HTLA-230 and HTLA-ER cells.Particularly, a discrete correlation was observed in HTLA-230, regardless of the time of exposure.A better correlation was observed in HTLA-ER cells and mainly for 24 h treatment, thus suggesting that, despite the high antioxidant defence in ETO resistant cells, the cytotoxic effects induced by P5PA-4I NPs were dependent on H 2 O 2 production.On the contrary, the reduced correlation between peroxide production and cytotoxicity of P5PA-4I NPs at 48 and 72 h exposure suggested an adaptive cell response to H 2 O 2 and the implication of other factors responsible for cancer cell death.Furthermore, these data were also confirmed by the results obtained with P5PA NPs, which were ineffective in reducing cell viability and enhancing H 2 O 2 levels (Figure S15).

Chemicals and Instruments
All reagents and solvents were purchased from Merck (formerly Sigma-Aldrich, Darmstadt, Germany) and were purified by standard procedures.2-2 -azobisisobutirronitrile (AIBN) was crystallized from methanol.Organic solutions were dried over anhydrous magnesium sulphate and were evaporated using a rotatory evaporator operating at a reduced pressure of about 10-20 mmHg.Copolymer P5 was prepared and characterized according to procedures and instruments previously reported [30], while imidazo-pyrazoles 4G and 4I were synthesized according to Brullo et al. [19].Attenuated total reflection-Fourier transform infrared (ATR-FTIR) spectra of the present paper were recorded on a Spectrum Two FT-IR Spectrometer (PerkinElmer, Inc., Waltham, MA, USA).Dynamic Light Scattering (DLS) and Z-potential determinations were performed on the same instrument and with the same modalities previously described [32].

Preparation of P5PA and P5PA-4I Nanoparticles (NPs)
PA/polystyrene-based (P5PA) and 4I-loaded PA/polystyrene-based (P5PA-4I) NPs were synthesized using the single emulsification technique like that described in the literature [39].Briefly, PA alone (119.1 mg; 0.4645 mmol), or 86.9 mg (0.1859 mmol) of 4I and PA (115.1 mg; 0.4489 mmol) were dissolved in 12 mL dichloromethane (DCM) to form the oily (O) phase.Secondly, P5 (238.2 mg; 0.047 mmol in the first case and 216.0 mg; 0.042 mmol in the second case) was dispersed in 5 mL ultrapure deionized water, to constitute the water (W) continuous phase, and magnetically stirred for 3 min at room temperature (RT).Next, the aqueous solution of P5 was added to the DCM solution containing 4I and PA or PA alone, and a VWR ® USC-300D, Ultrasonic Cleaning Bath (VWR International S.r.l., Milano, Italy) was used for 30 min to emulsify the system, thus obtaining an oil-in-water (O/W) emulsion.The obtained O/W emulsion was further sonicated at 40 • C for the time necessary to completely evaporate the DCM.The aqueous dispersion of the obtained NPs was washed with DCM 3 times to remove free drugs.Finally, the NPs were freeze-dried for 4 days, and the obtained P5PA NPs (337.5) and P5PA-4I NPs (402.0 mg) were stored in a dryer on P 2 O 5 at RT until further use.The morphologies of P5, P5PA and of P5PA-4I NPs were here investigated by optical microscopy (OM) analysis.In the performed experiments, powdery samples or aqueous dispersions were observed with a Nikon TMS-F inverted phase contrast microscope equipped with 4 × brightfield objective, 10 × phase contrast objective, LWD 20 × phase contrast objective, LWD 40 × phase contrast objective (Nikon Instruments, Inc., New York, NY, USA).Sequential images were acquired with 4 ×, 10 ×, 20 × and 40 × phase contrast objectives.The video was captured with a 20 × phase contrast objective.The camera for image capture was a Moticam 10+ (10 MP) (MoticEurope S.L.U., Cabrera de Mar, Barcelona, Spain).

Dynamic Light Scattering (DLS) Analysis
The hydrodynamic size (diameter) (Z-AVE, nm) and polydispersity index (PDI) of P5PA and P5PA-4I particles were determined using Dynamic Light Scattering (DLS) analysis.Z-Ave and PDI measurements were performed in water mQ as medium at max concentration of P5 of 3 mg/mL (pH = 7.4), in batch mode using a low volume quartz cuvette (pathlength, 10 mm).The analysis was performed by a photon correlation spectroscopy (PCS) assembly, equipped with a 50 mW He-Ne laser (532 nm) and thermo-regulated at the physiological temperature of 37 • C. The scattering angle was fixed at 90 • .Results were the combination of three 10 min runs for a total accumulation correlation function (ACF) time of 30 min.The hydrodynamic particle size result was volume-weighted and reported as the mean of three measurements ± SD.PDI value was reported as the mean of three measurements ± SD made by the instrument on the sample.The ζ-p was measured at 37 • C in mQ water as a medium, and an applied voltage of 100 V was used.The samples were loaded into pre-rinsed folded capillary cells, and twelve measurements were performed.

Cytofluorimetric Analyses
In the performed experiments the aqueous dispersions of P5, P5PA and P5PA-4I NPs prepared for the previous experiments were diluted 1:8 in type I deionized water 0.22 µM filtered (syringe filters, PVDF, 0.22 µm pour size, S.p.A, Milan, Italy cat#EPSPV2230) and filtered using disposable 40 µM mesh cell strainers (Euroclone S.p.A, Milan, Italy, cat#ET6040).Aliquots of the suspensions were loaded for flow cytometry analysis.Appropriate controls were run in parallel: unstained precision size standard beads 1 µm diameter (Polysciences Europe GmbH, Hirschberg an der Bergstrasse, Germany, cat# 64030-15) and deionized type I water 0.22 µM filtered.Data were acquired on a Guava easyCyte 6 flow cytometer (Merck Millipore, Burlington, MA, USA) and processed using the GuavaSoft 3.1.1software (Merck Millipore).Table 11 collects the experimental set up and the concentration of particles (Ps) expressed as number of particles per mL.

Chemometric Assisted ATR-FTIR Spectroscopy
FTIR spectra of 4I, P5PA NPs, P5PA-4I NPs, P5, and PA were recorded directly on the solid samples in attenuated total reflection (ATR) mode using a Spectrum Two FT-IR Spectrometer (PerkinElmer, Inc., Waltham, MA, USA).Acquisitions were made in triplicate from 4000 to 600 cm −1 , with 1 cm −1 spectral resolution, co-adding 32 interferograms, with a measurement accuracy in the frequency data at each measured point of 0.01 cm −1 , due to the internal laser reference of the instrument.The "find peaks" command of the instrument software was used to obtain the frequency of each band.The matrix of spectral data was subjected to by means of CAT statistical software (Chemometric Agile Tool, free down-loadable online, at: http://www.gruppochemiometria.it/index.php/software/19-download-the-r-based-chemometric-software; accessed on 18 July 2023).In particular, we arranged the FTIR data of the spectra acquired for all the samples in a matrix 3401 × 5 (n = 17,005) of measurable variables.For each sample, the variables consisted of the values of absorbance (%) associated with the wavenumbers (3401) in the range 4000-600 cm −1 .

Content of 4I in P5PA-4I, Drug Loading (DL%) and Entrapment Efficiency (EE%)
To construct the 4I calibration curve a stock solution of 4I (0.5 mg/mL) was prepared dissolving 4I in methanol (MeOH).The obtained colourless solution was added with 500 µL of Schiff fuchsin-sulphite reagent (Merck Italy, Milan, Italy) and left at room temperature up to reach a strong magenta coloration.Upon proper dilutions with MeOH, standard solutions at 4I concentrations of 0.025, 0.0375, 0.050, 0.075, 0.100 and 0.125 mg/mL were prepared.The obtained 4I solutions were analysed using a Fiber Optic UV-Vis Spectrometer System Ocean Optics USB 2000 (Ocean Optics, Inc., Dunedin, FL, USA) in 3 mL quartz cuvettes, thus detecting the related absorbance (Abs) at room temperature and at L abs = 543.88nm, using a sample of pure MeOH treated with the Schiff reagent, as blank.Determinations were made in triplicate and results were reported as mean of three independent experiments ± SD.The 4I concentrations were plotted vs. the Abs values, and the 4I calibration curve (Figure 17) was obtained by least-squares linear regression analysis using Microsoft Excel software.Equation (2) of the developed linear calibration model was the following.y = 9.3246x + 0.0531 In Equation ( 2), y was the Abs values measured at L abs = 543.88nm and x the 4I standard concentrations analysed.In Equation ( 2), the slope represents the coefficient of extinction (ε) of the Schiff base adduct between 4I and the Schiff reagent.
To estimate the 4I contained in P5PA-4I NPs, 50.0 mg of P5PA-4I NPs were dispersed in 10 mL of MeOH and vigorously stirred for ten minutes to promote the release of 4I.After centrifugation, the clear solution was added with 500 µL of Schiff fuchsin-sulphite reagent (Merck Italy, Milan, Italy) and left at room temperature up to reach a magenta coloration.The coloured solution was diluted 1:10 and the content of 4I was quantified at L max = 543.88nm by UV-Vis analysis, using a Fiber Optic UV-Vis Spectrometer System Ocean Optics USB 2000 (Ocean Optics, Inc., Dunedin, FL, USA) in 3 mL quartz cuvettes.The solutions were analysed against a methanol solution not containing 4I and treated with the Schiff reagent as blank.Determinations were made in triplicate and results were reported as mean of three independent experiments ± standard deviation (SD).
The values of DL% and EE% also indicted as drug loading capacity (DLC%) of P5PA-4I NPs were calculated from the following Equations ( 3) and (4) [63,64].Potentiometric titrations were performed on P5PA and P5PA-4I NPs at room temperature.Samples of each compound were exactly weighed (60.6 mg of P5PA and 60.8 mg of P5PA-4I) and suspended Milli-Q water (m-Q), qb to cover the pH-meter electrode.The solutions showed pH = 7.45 (P5PA) and pH = 7.50 (P5PA-4I).Then, they were treated under magnetic stirring with a standard 0.1 N NaOH aqueous solution (3.0 mL, pH = 10.19 for P5PA and 2.0 mL to pH = 9.20 for R4HG-4I), and potentiometrically titrated under stirring by adding aliquots of 0.2-0.7 mL of HCl 0.1 N for a total volume of 10.0 mL.Additional titrations were carried out after 1, 5, 10, 15, 20, 30, 35 and 40 days to assess the chemical stability of our materials in aqueous dispersion upon time at room temperature.
Titrations were performed in triplicate and measurements were reported as mean ± SD.The titration curves shown in the Discussion Section are those obtained by plotting the data obtained by carrying out the representative experiment described here.

Evaluation of 4I In Vitro Release Behaviors
The in vitro release of 4I from P5PA-4I and of 4I from a 4I suspension in PBS was determined by the dialysis method.About 200 mg of nanocomposite (P5PA-4I), whose content of 4I determined by the value of DL% (20.87%) was about 42 mg, and 42 mg of 4I were weighted.The samples were immersed separately in 10 mL of PBS medium (pH = 7.4) in dialysis bags with 3.5 K MWCO (Cellu Sep H1, Orange Scientific, Brainel'Alleud, Belgium) and subsequently dialyzed against 50 mL of release medium (PBS) at 37 • C and 100 rpm.At fixed interval points (0, 1, 2, 4, 24, 28, 48 and 72 h), aliquots of 1 mL of the release medium were taken out and 1 mL fresh PBS were replenished.Each aliquot was diluted 1:10 with MeOH, added with 500 µL of Schiff reagents and left to react up to a magenta coloration appeared.The amount of 4I in the aliquots was detected by measuring their absorbance at 543.88 nm using the UV-VIS spectrophotometer previously described and the 4I standard calibration curve previously constructed.A PBS solution not containing 4I and treated with the Schiff reagent was used as blank.Determinations were made in triplicate and results were expressed as mean of three independent experiments ± SD.The obtained concentrations were used to compute the cumulative drug release percentage, according to Equation (5).
In Equation ( 5), CDR (%) is the cumulative drug release, Dt was the cumulative 4I concentration at time t, and Di was the initial concentration of 4I in the dialysis bags (4.2 mg/mL for both P5PA-4I and for the 4I suspension).

Cell Treatments
To determine the biological actions of 4I or 4G, time-and dose-dependent experiments were carried out, by treating both cell populations for 24, 48 and 72 h, with increasing concentrations (0.5-100 µM) of the compounds.In another series of the experiments, NB cells were treated for 24, 48 and 72 h with increasing concentration (0.5-50 µM) of 4I or with the appropriate amounts of P5PA or P5PA-4I to provide cells the same concentrations of 4I and P5PA as described in Table 12.The stock solutions of these compounds were prepared in 40,000-fold diluted DMSO, and pilot experiments demonstrated that the final DMSO concentrations did not change any of the cell responses analysed.

Cell Viability
Cell viability was determined by using the CellTiter 96 ® AQueous One Solution Cell Proliferation Assay (Promega, Madison, WI, USA) as previously described [35,36].

Statistical Analyses
All biological data are expressed as means ± SEM of at least three independent experiments in which six different wells were analysed every time for each experimental condition.Concerning the experiments reported in Sections 2.1 and 2.2, statistical significance of differences was determined by one-way analysis of variances (ANOVA); p < 0.05 was considered statistically significant.Concerning experiments discussed in Sections 2.10 and 2.11, differential findings among the experimental groups were determined by a two-way ANOVA analysis of variance, with Bonferroni post tests, using GraphPad Prism 5 (GraphPad Software v5.0, San Diego, CA, USA).Asterisks or other indicators (see figures captions) indicate the following p-value ranges: * = p < 0.05, ** = p < 0.01, *** = p < 0.001.
The statistical significance of the slope of the 4I-calibration curve was investigated through the analysis of variance (ANOVA), performing the Fischer test.Statistical significance was established at the p-value < 0.05.

Conclusions
The aim of this study has been to identify a new potential approach for treating chemo-resistant NB and to this end we have industrialized an imidazo-pyrazole enriched drug delivery system by a nanotechnological approach, and we have tested its activity on ETO-sensitive (HTLA-230) and ETO-resistant (HTLA-ER) NB cells.As described in the manuscript, we have used PA as a nano-emulsion stabilizer and P5 as an encapsulating agent and solubilizer, thus achieving P5PA-4I solid NPs.No additives or additional surfactants, except for PA were used to prepare NPs, thus avoiding undesirable and detrimental interactions of other chemicals with 4I or P5, as well as unpleasant side effects in a possible future use in vivo.The characterization of NPs has shown that they have low positive Z-potentials (+6.97 and +8.53 mV) able to assure low haemolytic toxicity.In addition, the chemometric-assisted ATR-FTIR analyses, the release experiments, the NH 3 + groups determinations and the buffer capacity calculations fully support the physicochemical suitability of P5PA-4I NPs as an efficient new drug delivery system.Although further experiments are needed to optimize the nano-formulation here reported, including cytotoxicity investigations on normal cells, the embedment of 4I in P5PA NPs can represent a promising nanotechnological strategy to strongly enhance the cytotoxic action of 4I as well as of other imidazo-pyrazole derivatives.Collectively, the empty PAP5 NPs, deprived of intrinsic cytotoxic effects, could represent a safer and biocompatible platform for the design of novel delivery systems capable of increasing the cytotoxic action of entrapped traditional or novel anticancer drugs.

Figure 13 .
Figure 13.Representative flow cytometry histogram plots showing the Forward Scatter High (FSC-H Log) (a) and the Side Scatter High (SSC-H Log) (b) distributions of P5, P5PA and P5PA-4I NPs compared to the those of standard beads.Overall, 33,602 events per group were acquired.The colours of the histogram plots are the same of those used in Figures 10-12 and in Figures S2-S3.

Figure 13 .
Figure 13.Representative flow cytometry histogram plots showing the Forward Scatter High (FSC-H Log) (a) and the Side Scatter High (SSC-H Log) (b) distributions of P5, P5PA and P5PA-4I NPs compared to the those of standard beads.Overall, 33,602 events per group were acquired.The colours of the histogram plots are the same of those used in Figures 10-12 and in Figures S2 and S3.
Figure 13.Representative flow cytometry histogram plots showing the Forward Scatter High (FSC-H Log) (a) and the Side Scatter High (SSC-H Log) (b) distributions of P5, P5PA and P5PA-4I NPs compared to the those of standard beads.Overall, 33,602 events per group were acquired.The colours of the histogram plots are the same of those used in Figures 10-12 and in Figures S2 and S3.

2. 6 .
Chemometric Assisted ATR-FTIR Analyses ATR-FTIR analyses were carried out on 4I, PA, P5, P5PA NPs and P5PA-4I NPs to have qualitative indication of the chemical structure and composition of P5PA and of P5PA-4I NPs.Figures 14 and 15 show comparisons of the obtained spectra.

2. 8 .
Potentiometric Titrations of P5PA and of P5PA-4I NPs Upon titrations of both P5PA and P5PA-4I NPs dispersed in water as described in the Experimental Section, by plotting the measured pH values vs. the aliquots of HCl 0.1 N added, the titration curves of the samples were obtained as shown in Figure 17a.The first derivative (FD) curves of the titration lines shown in Figure 17b were obtained by computing the values of dpH/dV and plotting them against the corresponding volumes of HCl 0.1 N. The maxima of the FD lines represent the different titration end points.For comparison purposes, P5 alone was titrated in the same conditions as P5PA and P5PA-4I NPs and the titration curve, as well as the related FD are available in Figure S6 in the Supplementary Materials file.Int.J. Mol.Sci.2023, 24, x FOR PEER REVIEW 21 of 39

Figure 19 .
Figure 19.Score plot of PC1 (explaining the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance).Numbers associated with names indicate the number of days after first titration.Overlapped samples indicated very similar titration data and chemical stability.

Figure 19 .
Figure 19.Score plot of PC1 (explaining the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance).Numbers associated with names indicate the number of days after first titration.Overlapped samples indicated very similar titration data and chemical stability.
have been indicated with the name in red, while the samples of the training set have been represented with empty circles.Int.J. Mol.Sci.2023, 24, x FOR PEER REVIEW 25 of 39where the new samples titrated after standing in dispersion for 20 days, have been indicated with the name in red, while the samples of the training set have been represented with empty circles.

Figure 20 .
Figure 20.Projection of the external data set of new samples P5PA_20 and P5PA4I_20 (red labels) in the score plot of PC1 (explaining the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance) of the training set of the first ten samples (empty circles).

Figure 20 .
Figure 20.Projection of the external data set of new samples P5PA_20 and P5PA4I_20 (red labels) in the score plot of PC1 (explaining the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance) of the training set of the first ten samples (empty circles).
Int. J. Mol.Sci.2023, 24, x FOR PEER REVIEW 25 of 39where the new samples titrated after standing in dispersion for 20 days, have been indicated with the name in red, while the samples of the training set have been represented with empty circles.

Figure 20 .
Figure 20.Projection of the external data set of new samples P5PA_20 and P5PA4I_20 (red labels) in the score plot of PC1 (explaining the 97.6% of variance) vs. PC2 (explaining the 1.3% of variance) of the training set of the first ten samples (empty circles).

Figure 21 .
Figure 21.Cumulative release curves of 4I from P5PA-4I NPs and from an aqueous suspension of 4I, having the same initial 4I concentration (4.2 mg/mL).

Table 1 .
Therapeutics for NB treatment.

Table 3 .
Experimental data concerning the preparation of P5PA and P5PA-4I NPs.

Table 5
reports the FSC and SSC statistics (mean and median) calculated and provided by the instrument software for the R2 gated contour plot of SSC-HLog vs. FSC-HLog (panel d in FiguresS2, S3and 10-12).

Table 5 .
FSC and SSC statistics (mean and median) calculated and provided by the instrument software for the R2 gated contour plot Side Scatter High (SSC-HLog) vs. Forward Scatter High (FSC-HLog) of all samples.

Table 7 .
Equivalents of PA and basic nitrogen atoms of P5PA, P5PA-4I and P5 by potentiometric titration.
* Between the first and the second end point; ** between the second and the third end point; N.E.D. = not existing data.

Table 9 .
Values of the coefficients of determination obtained for all the kinetic models used.

Table 11 .
Experimental set up for the cytofluorimetric analyses.

Table 12 .
Concentrations of 4I used in the screening experiments expressed both in µM and in µg/mL.Concentrations of P5PA4I and P5PA NPs administered to NB cells in both cytotoxicity and ROS production experiments.MW = 467.5;** computed according to the drug loading (DL%) of 20.87%; *** computed according to the concentrations of P5PA-4I NPs; values in bold are the thresholds concentrations accepted by NCI for a new compound to be considered active against a cancer. *