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    Xenon as a transdermal enhancer for niacinamide in Strat-MTM membranes

    2022-09-10 13:18:16EvgenyPetrovAlexanderVerkhovskiy
    Medical Gas Research 2022年1期

    Evgeny Petrov,Alexander Verkhovskiy

    Laboratory of Biochemistry of Transport Systems,Faculty of Innovative Technologies,National Research Tomsk State University,Tomsk,Russian Federation

    Abstract Xenon is confirmed to diffuse readily through membranes and has properties of transdermal enhancer.In this study,the ability of xenon to regulate the transdermal diffusion of niacinamide was investigated using a model of an artificial skin analogue of Strat-MTM membranes in Franz cells.Based on the data obtained,we found that in the simplified biophysical model of Strat-MTM membranes xenon exerts its enhancer effect based on the heterogeneous nucleation of xenon at the interfaces in the microporous structures of Strat-MTM membranes.

    Key words:enhancer;Franz cell;gas nucleation;niacinamide;permeation;skin;Strat-M;transdermal drug delivery system;xenon

    INTRODUCTION

    Xenon is an inert gas with a number of interesting biologically active properties.Detailed studies have shown that xenon atoms are localized in hydrophobic “pockets” of protein molecules–small cavities with predominantly short hydrophobic residues,such as leucine,isoleucine,valine and alanine,1and also accumulated in the hydrophobic region of cell membranes.2-4In both cases,xenon acts as a modifier of the activity and functional state of transmembrane molecular complexes.More recently,it has been suggested that xenon can reduce the biological function of proteins by forming nanobubbles at or near hydrophobic sites on the protein surface.5,6

    Studies have been focused on the biologically active properties of xenon usedin vivo,7-10in vitro,11-15andin silico,16,17through which detailed data on the anesthetic and analgesic properties of xenon are obtained.However,the experimentalin vivoapproach,where xenon can affect biomolecules by contact with the skin,is completely overlooked.This approach seems quite reasonable,given the good solubility of xenon in hydrophobic media.In addition,it is technically not difficult to provide a high concentration of xenon on the skin area.

    How can xenon affect the barrier function of the epidermis and its integrity? How can xenon affect the physiology of deeper skin layers? These questions remain unanswered,and we have not found any mention of it in the scientific literature.It should be taken into account that the physiology and pathophysiology of the skin is very complex,and what the expected bioeffects of xenon are,is difficult to predict.In this regard,at this stage of research on biological properties of xenon in relation to “simple” barrier properties of the skin,we consider it appropriate to use the model of artificial skin analogues,namely,membrane Strat-MTMpatches.18This approach has successfully proven itself in studies of transdermal diffusion and permeability of a number of compounds.19-25Niacinamide,a widely used cosmetic ingredient,was chosen as the permeant.It stabilizes the barrier function of the epidermis,stimulates ceramide synthesis,accelerates differentiation of keratinocytes,smooths wrinkles,and reduces photoinduced and age-related pigmentation in the skin.26-28In addition,the laboratory has a well-established protocol for chromatographic analysis of niacinamide.

    MATERIALS AND METHODS

    Chromatography for niacinamide

    All experiments were performed on a Thermo ScientificTMUltiMateTM3000 UHPLC system (Thermo Fisher Scientific,Waltham,MA,USA) with a ultraviolet detector.The column used was a Zorbax Eclipse Plus Phenyl-Hexyl stationary phase(Agilent Technologies,Inc.,Santa Clara,CA,USA),150 ×4.6 mm,3.5 μm.

    Buffer solution was prepared by dissolving 3.2 g of ammonium dihydrophosphate (JSC VEKTON,St.Petersburg,Russia) and 250 μL of concentrated phosphoric acid in 1 L of water.The mobile phase was prepared by mixing 980 mL of buffer solution and 20 mL of acetonitrile (PanReac AppliChem GmbH,Darmstadt,Germany).Flow rate was 1.0 mL/min with isocratic elution.The column temperature was set to 30°C.The detection wavelength was set to 210 nm.Injected volume was 20 μL.Standard solution and calibration solutions were prepared by dissolving a dry sample (niacinamide;DSM Nutritional Products Ltd.,Basel,Switzerland) of the standard in deionized water.

    Chromatography for xenon

    A Chromatec-Crystall 5000.1 gas chromatograph (Chromatec,Yoshkar-Ola,Russia) with a thermal conductivity detector was used for the analysis.Sample with xenon (Akela-N Ltd.,Moscow,Russia) was placed into the vial,previously weighed together with the lid and the membrane cover.Second weighing was done to determine the mass of the sample in the vial.The vial with the sample was placed in a thermostat (75°C).Two needles with capillaries were inserted into the membrane cover.The first needle was connected to a six-way chromatograph splitter and the gas exiting the vial was blown and accumulated in a calibrated loop (1 mL) of the splitter.The second needle was connected to a vessel containing saturated aqueous NaCl solution (ρ=1.17 g/mL,t=20°C),then tap was opened and the solution pumped the air from the vial and xenon released from the sample entered into the chromatograph loop.After that by turning the valve the gas mixture (xenon + air) was injected into the chromatograph for separation and quantification of xenon.

    To separate xenon from air a 4 m long packed chromatographic column with NaX sorbent (fraction 60/80;Chromlab,Lyubertsy,Russia) was used.The sequence of the gases leaving the column was following:helium,hydrogen,neon,oxygen +argon,nitrogen,methane,carbon monoxide,krypton,xenon.Helium used as a carrier gas.Column thermostat temperature was set to 80°C.Rate of carrier gas was set to 30 mL/min.The concentrations of the components of the gas mixture were calculated by the method of absolute calibration using samples with known xenon concentration using software package Chromatec Analytic 2.5 (Chromatec).

    Preparation of Strat-MTM membranes

    Due to high xenon solubility in oils (20 times better than in water),29,30it was decided to use the neutral emollient Cetiol?CC (BASF Personal Care and Nutrition GmbH,Monheim,Germany) as xenon solvent that will serve as an efficient source of xenon.Strat-MTMmembranes (Merck Millipore,Burlington,MA,USA) were mounted and incubated in three Franz cells (PermeGear,Inc.,Hellertown,PA,USA) for 45 minutes at 37°C with a phosphate-buffered saline (PBS)-filled acceptor chamber before the experiment.Xenon-containing niacinamide (1×) solution was prepared ex-temporo.Gas was mixed with 10 mL of the prepared niacinamide solution(5%) in PBS by vigorous shaking it in a 20 mL syringe.The concentration of xenon in PBS was 0.86 ± 0.1 mg/g (n=3).Niacinamide solution with half xenon content (0.5×) was obtained by preparing 20 mL of niacinamide solution (5%)in PBS from which 10 mL was taken,saturated with xenon,and mixed with the remaining 10 mL of niacinamide xenonfree solution.1 mL of the solution was placed in the donor chamber of each Franz cell.The sampling volume was 0.4 mL for xenon and 0.4 mL for niacinamide measurements.Samples were collected every hour (up to 8 hours).

    Light microscopy

    An Amszoom trinocular light microscope (AmScope,Irvine,CA,USA) was used to observe the xenon nucleation on Strat-MTMmembranes.

    Statistical analysis

    Samples with xenon and niacinamide were collected during 8 hours from three separate Franz cells every hour for further use in chromatography analysis.Permeability parameters were derived from the total amount of xenon and niacinamide

    diffused through a membrane surface area (mg/cm2) unit per time unit.Results are presented as mean ± standard deviation(SD) (n≥ 3).Statistical analysis of the data was performed with one-way analysis of variance followed by Scheffe post hoc test using the Microcal Origin software package (version 8.1;OriginLab Corporation,Northhampton,MA,USA).

    RESULTS

    Transmembrane diffusion of xenon

    The resulting concentration of xenon in Cetiol?CC was 16.01± 1.07 mg/g (n=4).It was shown that xenon diffuses effectively through the membranes (Figure 1),and the diffusion rate is comparable with the case when the membrane was not used and the interface was the boundary between Cetiol?CC in the donor chamber and PBS in the acceptor chamber.

    Figure 1:Cumulative xenon flux in the absence of a barrier and through Strat-MTM membranes.

    Transmembrane diffusion of niacinamide in the presence of xenon

    In a transdermal diffusion study of a 5% solution of niacinamide,it was shown that xenon works as an enhancer–it increases the permeation rate of niacinamide across Strat-MTMmembranes (Figure 2A and B).However,the enhancer effect is stronger at lower concentrations of xenon,and only during the first 4 hours from the onset of experiment (Figure 2C).

    Figure 2:Dose-dependent effect of xenon on transdermal diffusion of niacinamide across Strat-MTM membranes.

    Nucleation of xenon on Strat-MTM membranes

    The proposed mechanism of xenon acting as an enhancer is different from the previously described.31A possible mechanism of xenon influence on transdermal diffusion of niacinamide is the formation of xenon microbubbles on hydrophobic groups(heterogeneous nucleation).The polyolefin layer of the Strat-MTMmembrane contains a combination of lipids (ceramides,cholesterol,free fatty acids and other components) in a specific ratio similar to that found in the human epidermis.19These groups may serve as centers for xenon nucleation.We tested the principle possibility of xenon nucleation on Strat-MTMmembranes under conditions of maximum PBS saturation with xenon (1×) (Figure 3).Placing the Strat-MTMmembrane strips in xenon solution,we observed nucleation,in which the bubbles became most distinguishable after half an hour from the moment of immersion.

    Figure 3:Nucleation of xenon on Strat-MTM membranes.

    DISCUSSION

    To understand the enhancer effect of xenon on niacinamide diffusion,we propose a simplified model (Figure 4) of the three-layer Strat-MTMmembrane as a single pore with the narrowest part in the upper region,which mimics the stratum corneum.Then the pore has an intermediate diameter (representing dermis layer) and the widest part as the lower region of the membrane (representing hypodermis).It is possible that xenon forms microbubbles on the interphase zones of the walls of such a pore.In this case,we can assume partial shielding of the pore surface by “sticking” xenon microbubbles,which fill its roughness.This phenomenon can facilitate the diffusion of niacinamide molecules from the high concentration zone (the donor chamber of Franz cells) to the low in acceptor chamber through the Strat-MTMmembrane.

    Figure 4:The proposed mechanism of xenon as an enhancer in Strat-MTM membranes.

    A similar explanation is given in microfluidics research as a superhydrophobic slippage phenomenon,when air microbubbles modify the surface from Wenzel state to Cassie state.32For our case this explanation of the xenon enhancing effect is challenged by the fact that there is no fluid flow along the interfaces of micropores but passive diffusion of niacinamide molecules along the concentration gradient.Moreover,the interaction of niacinamide molecules with the inner surface of Strat-MTMmembrane micropores to the diffusion process must be taken into account.The intensity of xenon nucleation process inside the pore depends mainly on its concentration.It is quite possible that at maximum concentration of xenon its microbubbles during nucleation may grow in size that becomes comparable with the diameter of the pore in the middle and lower parts of the membrane.Apparently,the amount of dissolved xenon in this zone reaches the level when the formation of such microbubbles becomes possible.In this case,some micropores are blocked by xenon microbubbles and excluded from net transmembrane diffusion of niacinamide.

    In our experiments xenon at both used concentrations operates as an enhancer.But,in the case of maximum saturation of PBS with xenon (1×),there may be partial overlapping of large bubbles with already larger diameter pores,leading to a decrease in the total lumen for transmembrane diffusion of niacinamide.In this case,the enhancer effect is less pronounced.Nevertheless,it is possible that overlapping of large pores in the membrane due to xenon nucleation also occurs in 0.5× case at late stages (more than 4 hours from the onset of experiment),and this explains the absence of significant differences in the xenon enhancing effect (Figure 2C) for 0.5× and 1× cases,suggesting that it is weakening at the later stages of experiment.

    There are some deficiencies and limitations in this study.In particular,the donor chamber of the Franz cell can not be considered as an infinite xenon source due to its rapid diffusion into the acceptor part.Therefore,we had to limit the duration of our experiments to 8 hours maximum.The light microscopy allowed us to visualize the nucleation of xenon in the form of large bubbles on the dermal surface of the Strat-MTMmembrane,but not the forming microbubbles in the layers of the membrane,what would be the direct proof of our hypothesis.It should also be noted that Strat-MTMmembranes are a simplified analogues of the skin.They possess no metabolic activity,and have different chemical composition.Direct extrapolation of observed enhancing activity of xenon on native skin preparations should be done with caution.

    The obtained data suggest that xenon can be considered as a promising transdermal enhancer with a new mechanism of action.However,the optimal concentration of xenon,at which its properties as an enhancer are manifested to the maximum extent,remains unknown.The question whether xenon will show its ability to act as an enhancer in case of using other permeants,as well as the scenario of utilizing native skin preparations,heat separated epidermis,etc.,remains unanswered and needs further research.

    Author contributions

    Conception of the work,experiment design,literature search:AV.Data acquisition,experiment design,data analysis,literature search,manuscript preparation:EP.Both the authors read and approved the final version of the manuscript for publication.

    Conflicts of interest

    Xenon Diffusion is in the patent pending process.

    Financial support

    This work was supported by the Xenon Skincare International,Inc.(East Stroudsburg,PA,USA),represented by Dr.Mikhail Artamonov.Neither the experimental design nor the results of this work were affected by the funder.

    Copyright license agreement

    The Copyright License Agreement has been signed by all authors before publication.

    Data sharing statement

    Individual participant data that underlie the results reported in this article,after deidentification (text,tables,figures,and appendices).Study protocol and informed consent form will be available immediately following publication,without end date.Results will be disseminated through presentations at scientific meetings and/or by publication in a peer-reviewed journal.Anonymized trial data will be available indefinitely at www.figshare.com.

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    Checked twice by iThenticate.

    Peer review

    Externally peer reviewed.

    Open access statement

    This is an open access journal,and articles are distributed under the terms of the Creative Commons Attribution-NonCommercial-ShareAlike 4.0 License,which allows others to remix,tweak,and build upon the work non-commercially,as long as appropriate credit is given and the new creations are licensed under the identical terms.

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