The Effect Of Topical Dapsone In Comparison With Tacrolimus On Dncb Induced Atopic Dermatitis In Mice

To assess the effect of topical dapsone in the treatment of atopic dermatitis in comparison with tacrolimus. A case-control study was done on 80 male Albino mice (20-30g) recruited from local markets, were treated with 1-Chloro-2,4-dinitrobenzene (DNCB)-induced atopic dermatitis and compared with age and the sex-matched control group comprised of 20 healthy male Albino mice. The topical applications of Tacrolimus 0.1% ointment and Dapsone 5% gel were performed on atopic dermatitis area for seven days and fourteen days once daily starting from the fourth day of induction and Complete blood count, IL-4 and IL-13 were measured in skin tissue homogenate in addition to histopathological evaluation of atopic dermatitis skin lesion and assessment of observational severity score and compared with those of controls. The results revealed that the levels of IL-4 and IL-13, total WBC, observational severity score, and the score of all histopathological markers were increased signi(cid:976)i-cantly in the group of mice treated with 1-Chloro-2,4-dinitrobenzene (DNCB) for A.D. induction in comparison with controls. These markers were reduced signi(cid:976)icantly after the topical application of tacrolimus. They showed a compa-rable reduction but after a longer duration of topical treatment with dapsone after two weeks of treatment. Topical application of dapsone on induced A.D. mice showed a signi(cid:976)icant reduction in the levels of IL-4 and IL-13, total WBC, observational severity score, and histopathological markers score and these effects were compared to those of topical tacrolimus.

dapsone, tacrolimus, Atopic dermatitis, IL-4, IL-13, 1-Chloro-2, 4-dinitrobenzene (DNCB) A To assess the effect of topical dapsone in the treatment of atopic dermatitis in comparison with tacrolimus. A case-control study was done on 80 male Albino mice (20-30g) recruited from local markets, were treated with 1-Chloro-2,4dinitrobenzene (DNCB)-induced atopic dermatitis and compared with age and the sex-matched control group comprised of 20 healthy male Albino mice. The topical applications of Tacrolimus 0.1% ointment and Dapsone 5% gel were performed on atopic dermatitis area for seven days and fourteen days once daily starting from the fourth day of induction and Complete blood count, IL-4 and IL-13 were measured in skin tissue homogenate in addition to histopathological evaluation of atopic dermatitis skin lesion and assessment of observational severity score and compared with those of controls. The results revealed that the levels of IL-4 and IL-13, total WBC, observational severity score, and the score of all histopathological markers were increased signi icantly in the group of mice treated with 1-Chloro-2,4-dinitrobenzene (DNCB) for A.D. induction in comparison with controls. These markers were reduced signi icantly after the topical application of tacrolimus. They showed a comparable reduction but after a longer duration of topical treatment with dapsone after two weeks of treatment. Topical application of dapsone on induced A.D. mice showed a signi icant reduction in the levels of IL-4 and IL-13, total WBC, observational severity score, and histopathological markers score and these effects were compared to those of topical tacrolimus.

INTRODUCTION
Atopic dermatitis (A.D.) is a common, familial, chronic in lammatory skin disease characterized by intense pruritus, erythematous lesions, scaly skin lesions, and xerosis. The pathophysiology of atopic dermatitis based on skin barrier dysfunction combined with complex interactions of genetic, immunologic, psychologic, and environmental factors (Lyons et al., 2015). Atopic dermatitis is count as a primarily T cell-driven disorder in which in iltrating T cells, especially T helper 2 cells, are essential. Cytokines related to T helper 2, IL-4, and IL-13 are the signi icant parameters in this disease. Topical corticosteroids, calcineurin inhibitors (TCIs); tacrolimus and pimecrolimus are the mainstay of the treatment for moderate to severe atopic dermatitis, both in children and adults (Fuxench, 2017).
Tacrolimus ointment is an immunosuppressive medication which considered as newer formulation used for the treatment of acute lares and maintenance therapy of atopic dermatitis, by binding to the cytosolic immunophilin receptor (macrophilin-12) to form a complex that inhibits the activity of the enzyme calcineurin it will block T-cells activation (Gutfreund et al., 2013). Dapsone (4,40diamino-diphenyl sulfone) is an aniline derivative belonging to the group of synthetic sulfones with microbial activity. The use of dapsone to treat non-pathogen-caused diseases revealed alternate anti-in lammatory mechanisms that initially were elucidated by in lammatory animal models. Thus, dapsone has dual functions of both: antimicrobial/antiprotozoal effects and anti-in lammatory features (Wozel and Blasum, 2014).
This study was aimed to investigate the effect of topical dapsone in treatment of induced atopic dermatitis in mice through measure the levels of IL-4, IL-13 in skin tissue homogenate, CBC, histopathological markers, and assessment of observational severity score, and compare them with those topically treated with tacrolimus and non-treated induced atopic dermatitis group.

Study design
A case-control study was done on 80 male Albino mice (20-30g) recruited from local markets, were treated with 1-Chloro-2,4-dinitrobenzene (DNCB)induced atopic dermatitis (Hamad et al., 2017) and compared with age and the sex-matched control group comprised of 20 healthy male Albino mice. The study was started in June and inished in December 2019. The experimental animals were performed in compliance with the principles guide of ethical in laboratory animals approved by the University of Al-Naharain. The practical part of the study was conducted at Department of pharmacology, College of Medicine, Al-Nahrain University, Baghdad-Iraq. Eighty-four animals have continued the study successfully. Sixteen animals died during the study because of environmental conditions and induction. Albino mice were sub-categorized into three groups; Group I represent 20 induced atopic dermatitis mice without treatment, Group II represent 20 induced atopic dermatitis mice treated with tacrolimus 0.1% ointment topically once daily at 9:00 AM for 7 and 14 days. Group III represent 20 induced atopic dermatitis mice treated with Dapsone 5% gel topically once daily at 9:00 AM for 7 and 14 days.

Treatment protocols
The topical applications of treatments (Tacrolimus 0.1% ointment and Dapsone 5% gel) were applied on atopic dermatitis area of animal for 7 days and 14 days once daily at 9 AM morning starting from the fourth day of induction.  The following listed parameters are used to compare in results between experimental groups on day 7 and 14 of the treatment 1. Complete blood count.
2. IL-4 and IL-13 were measured in skin tissue homogenate for mice with an atopic dermatitis skin lesion and compared with those of controls.
3. Histopathological evaluation of atopic dermatitis skin lesion and compared with those of controls.
4. Assessment of observational severity score.        Animal sacri icing, dissection, histological analysis, skin tissue homogenate preparation, and assessment of observational severity score At the 7 th day of the treatment, we took half number of mice from each study groups and anaesthetized through a piece of cotton soaked with ether put with the mouse inside a closed jar for few minutes to be anaesthetized by inhalation, blood sample collected (1ml) in EDTA tube then sacri iced by cervical dislocation and the sharp blade cut atopic dermatitis skin area; this skin wound was dissection into two equal pieces one for the histological analysis and the second for the preparation of skin homogenate. The remaining mice from each group were subjected to the same procedure on the 14 th day of the treatment.

Histological analysis
Dorsal skin samples were collected from each ani-mal in study groups and ixed in 10% formaldehyde, paraf in-embedded and cut into 6 µm sections. Deparaf inized sections were stained with hematoxylin and eosin (H and E) to determine the in lammatory degree and histological changes associated with atopic dermatitis.

Assessment of histopathological changes in skin sections
Histopathologic follow-up procedures were used for the skin samples taken from each group on the 7 th and 14 th days of treatment. Histopathological changes of skin of each specimen were evaluated and scored by semiquantitative scoring systems for the evaluation of mouse model histopathology include Epidermal hypertrophy, hyperkeratosis, parakeratosis, erosion, in lammation, oedema, ulcer (each 0-4) were examined by a pathologist (Watan-

Skin tissue homogenate preparation
The second piece of skin obtained were washed with normal saline, and rinsed with chilled phosphate buffer saline (1X PBS), put with ilter paper and weighed. Each 100 mg of skin wound tissue was homogenized with 1 ml of (1X PBS) with the aid of tissue homogenizer for 1 minute at 4 • C and must be stored overnight at 20 • C. Two freeze-thaw cycles must be performed to break the cell membranes; the homogenates were centrifuged for ten minutes at 2000 RPM at 2-8 • C. The supernatant was obtained and stored at -20 • C to the assay of IL-4 and IL-13 levels in the tissue.

Quantitative measurement of IL-4 and IL-13 (principle of the assay)
ELISA Kit for the estimation of IL-4 and IL-13 was obtained from Mybiosource/USA. The kit was based on sandwich enzyme-linked immune-sorbent assay technology. Anti-IL-4 and Anti-IL-13 antibodies were pre-coated onto 96-well plates. And the biotin conjugated anti-IL-4 and anti-IL-13 antibodies were used as detection antibodies. The standards, test samples and biotin conjugated detection antibodies were added to the wells subsequently and washed with wash buffer. HRP-Streptavidin was added, and unbound conjugates were washed away with wash buffer. TMB substrates were used to visualize HRP enzymatic reaction. TMB was catalyzed by HRP to produce a blue colour product that changed into yellow after adding the acidic stop solution. The density of yellow is proportional to the IL-4 and IL-13 amount of sample captured in plate. Read the O.D. absorbance at 450nm in a microplate reader. Then the concentration of IL-4 and IL-13 can be calculated by comparing the optical density of the samples to that of the standard curve in the corresponding microtiter plate (Voller et al., 1978). The concentration of IL-4 and IL-13 in each sample was expressed in pg/ml for comparison of results with those of controls concentration.

Assessment of observational severity score
The severity of AD on the dorsal area was evaluated for each group on the 7th and 14th days of treatment. The evolution of erythema, dryness, erosion and edema will scored as 0 (none), 1 (mild), 2 (moderate), and 3 (severe) (Suto et al., 1999).

Statistical analysis
The data of the study were stored in Microsoft Excel spreadsheet and analyzed on the computer using the SPSS software 20 and Microsoft excel program (2010). Numeric variables were expressed as mean ± S.D., and all statistical comparisons were made using independent t-test, and ANOVA test with P ≤0.05 was considered statistically signi icant. Categorical variables were expressed as numbers and analyzed by cross-tabulation to assess the frequency and percentage of each variable among studied groups. The correlation was done between all parameters using Pearson correlation test (Norman, 2010), eta (η) test between numerical and categorical variables (given that values ranged from 0-0.5 considered as weak correlation while values above 0.5 considered as strong correlation) and Chisquare to test the relationships between categorical variables.

General characteristics of the study groups
Some demographic characteristics of the studied groups were summarized in Table 1 that showed non-signi icant differences in age and weight among all studied groups. Table 2 revealed that the levels of IL-4 and IL-13 were increased signi icantly (p<0.05) in the group of mice with an induced A.D. in comparison with controls after the irst and second week of sampling. It was demonstrated that the values of complete blood count showed a signi icant increase in the total WBC count, basophils, eosinophils, lymphocytes and platelets after one and two weeks of atopic dermatitis induction when compared with control. The only exception was the monocytes that showed a signi icant high count in the irst week of induction in comparison with controls at the same time while a non-signi icant difference was obtained in the second week of application. Table 3 and Figure 1 obviated the effect of A.D. induction on the histopathological score after one and two weeks. It revealed that observational severity score, Epidermal thickness, Hyperkeratosis, Parakeratosis, Erosion, In lammation and Edema score showed signi icantly higher scores than controls after one and two weeks of A.D. induction. Table 4 elucidate clearly that the levels of IL-4 and IL-13 in mice received tacrolimus topically were signi icantly lower than the corresponding levels in A.D. induced nontreated group after one and two weeks of treatment. Furthermore, total WBC, neutrophils, basophils and eosinophils count showed a signi icant reduction after two weeks of topical application of tacrolimus. In contrast, platelets count decreased signi icantly after one week of treatment with topical tacrolimus which reduced further after the second week of treatment. Table 5 and Figure 2 showed that observational severity score, epidermal thickness, hyperkeratosis, parakeratosis, in lammation and oedema score were signi icantly reduced in tacrolimus treated group in comparison with those non-treated A.D. induced group after one week of treatment. Additionally, observational severity score, epidermal thickness, hyperkeratosis, parakeratosis, erosion, in lammation and oedema score showed signi icant reduction after two weeks of treatment with tacrolimus.

Results postulated in the
Data postulated in the Table 6 illustrated that the levels of all studied variables after the application of dapsone topically were non-signi icantly differ from those of corresponding non-treated induced A.D. group except the signi icant decrease in the count of WBC and neutrophils after one week of treatment. On the other hand, levels of IL-4 and IL-13 in addition to the count of WBCs, neutrophils, Monocytes, Eosinophils and RBC were signi icantly decreased in comparison with a non-treated A.D. induced group after two weeks of treatment. Table 7 and Figure 3 showed that the Parakeratosis and In lammation scores of topically dapsone treated group after one week of treatment were signi icantly lower than that of non-treated A.D. induced group whereas all studied histopathological scores including epidermal thickness, hyperkeratosis, parakeratosis, erosion, in lammation and oedema score in addition to the observational severity score were signi icantly lower than those of mice group with induced A.D. that did not receive treatment.

The in luence of sampling time on the studied variables:
All data presented in Tables 8 and 9 revealed that there was a non-signi icant difference between the levels of all studied variables that including IL-4, IL-13, CBC, observational severity score and A.D. histopathological scores obtained after one or two weeks of treatment, i.e. levels obtained after two weeks of induction or treatment were non-signi icantly differ from those obtained after the irst week.

Comparison between all studied groups by ANOVA test
Following the data postulated in the Table 10, the levels of IL-4 were signi icantly differenced among all studied groups, whereas IL-13 showed a nonsigni icant change among these groups in the irst week of sampling. CBC values showed that WBC and RBC counts were signi icantly changed among the studied group during the irst week of A.D. induction and treatment. Additionally, Observational severity score and histopathological scores including, Epidermal thickness, Hyperkeratosis, Erosion, and In lammation score were signi icantly changed in the irst week.
Furthermore, after two weeks of treatment with different topical application, more signi icant differences were obtained including signi icant differences in the levels of both studied cytokines  in addition to the CBC values that showed signi icant differences in WBCs, Basophils, Eosinophils, RBCs and platelets counts with signi icant changes in observational severity and all histopathological scores (Table 11). Table 12 revealed that the levels of IL-4 and IL-13 were correlated positively and signi icantly with each other. Moreover, levels of IL-4 showed a signi icant positive correlation with the weight of mice and correlated signi icantly and negatively with the age of mice subjected to the present study.

Correlations
Results of the present study revealed that the atopic dermatitis induction by DNCB cause signi icant elevations in the levels of IL-4 and IL-13 in skin homogenate in comparison with controls and also cause a signi icant increase in total WBC count, basophils, eosinophils, lymphocytes and platelets after one week. Many previous kinds of research used DNCB as an inducer for atopic dermatitis that causes an elevation in the levels of IL-4 and IL-13 (Kitamura et al., 2018) which is consistent with the results obtained in this study. The ability of DNCB to induce atopic dermatitis originate mainly from its role in increase type-2 helper T cell reactivity, IL-4 and IL-13 that result in the in lammatory response that elevate the levels of IgE and affect the histological scores of the affected skin which appear clearly via the histopathological investigations, which explained the high signi icant increase in observational severity scores (Kim et al., 2018). It was noticed that the levels of studied markers were reduced slightly after the application of DNCB by two weeks in comparison with the same markers after one week from the application which may be contributed to the healing process that occurs after more than ten days which is agreed with the results illustrated in recent work published in 2020 (Lee et al., 2020).
In a consistent with a majority of the articles that dealt with the use of tacrolimus in A.D. treatment (Crissinger and Nguyen, 2014), our recent work obviates the effect of tacrolimus on atopic dermatitis tissue markers, histological and observational severity scores and also on the CBC of the affected mice.
Levels of IL-4 and IL-13 were decreased signi icantly in topically tacrolimus treated group in comparison with those suffered from atopic dermatitis induced by DNCB which occur after one week of treatment and persist to the second week with the slight non-signi icant difference between these two sampling time. The assumed mechanism of action of tacrolimus was discussed in several types of research, and they postulated that the primary mechanism of action of tacrolimus is its immunosuppression activity (Sengoku et al., 2000) which then subjected to more profound studies to elucidate this mechanism precisely. Tacrolimus known to can bind speci ic receptors on T cells leading to an increase in intracellular calcium which, in turn, lead to series of reactions inhibiting the transcription of several genes for several cytokines such as IL-4 (Russell, 2002). Furtherly, more recent study postulated that tacrolimus bind to the F.K. binding protein-12 (FKBP12) to inhibit calcineurin, a protein phosphatase responsible for the dephosphorylation of the nuclear factor of activated T-cells (NF-AT) (Crissinger and Nguyen, 2014). Without dephosphorylation, NF-AT cannot be translocated into the nucleus, and thus the pro-duction of in lammatory interleukins is inhibited. Adjunctive mechanisms of action have been proposed for tacrolimus including binding at cell surface steroid receptors, inhibition of mast cell mediator release, and downregulation of chemoattractant IL-8 receptors, intracellular adhesion molecule-1, E-selectin, and Langerhans cells IgE receptors (Ohtsuki et al., 2018).
The proposed mechanisms for tacrolimus activity explain its anti-in lammatory and anti-chemotactic role that may provide an acceptable explanation about the other variables and histological scores that reduced after treatment with it for one and two weeks such as the reduction in the counts of total WBCs, neutrophils, eosinophils and basophils in agreement with the previous review (Kandikattu and Mishra, 2018). Additionally, the results illustrated in the current study showed a signi icant reduction in the count of platelets inconsistency with previous results (Arai et al., 2016).
The second treatment group that examined throughout the current study was topical dapsone which is an aniline derivative belonging to the group of synthetic sulfones with microbial activity. Shortly after that, the use of dapsone to treat non-pathogen-caused diseases revealed alternate anti-in lammatory mechanisms that initially were elucidated by in lammatory animal models. Thus, dapsone has dual functions of both: antimicrobial/antiprotozoal effects and antiin lammatory features similarly to non-steroidal anti-in lammatory drugs (Kridin, 2018). that is the cause of our study on topical dapsone to con irm its role in treating atopic dermatitis regarding a case report and brief assay which describe its use in A.D. (Lee et al., 2005).
Results illustrated in the present work obviate the possible role of topical dapsone in the treatment of atopic dermatitis as it showed a signi icant effect on the levels of IL-4, IL-13, CBC, histopathological scores, and observational severity scores that appear more clearly after two weeks of treatment with dapsone topically. No obvious explanation found about the effect of IL-4 and IL-13 levels. Still, the assumed effect of dapsone on Th2 cells may be the cause of the signi icant decrease in these cytokines levels in agreement with previous work (Wozel and Blasum, 2014).
The postulated decrease in the counts of total WBCs, Monocytes, eosinophils, neutrophils, and RBCs may be considered as a possible mechanism of an anti-in lammatory which also considered as a side effect for dapsone which can be used in future as a promising topical application for the treatment of A.D. which is inconsistent with previous works of literature that consider this activity as an adverse effect (Halim and Ogbeide, 2002). In eosinophil-mediated in lammation dapsone may act by several mechanisms, its anti-in lammatory actions involve several effects on neutrophils such as; reduced chemotactic attraction, inhibition of neutrophil myeloperoxidase, reduced secretion of reactive oxygen species, and reduced generation of 5-lipoxygenase and other lysosomal enzymes. Additionally, dapsone has a signi icant effect on eosinophil function. It has been shown to inhibit eosinophil peroxidase, which is a cytotoxic granule protein of eosinophils that induces mast cell degranulation (Bokotas et al., 2014). The inhibitory effect of dapsone on eosinophil peroxidase as a previous explanation of the therapeutic ef icacy of dapsone in eosinophil-mediated diseases showed that the dapsone inhibitory effect reduces the effect of eosinophil peroxidase on mast cells which lead to decreasing the release of the in lammatory mediators, this inhibitory effect might be due to the inhibition of lipoxygenase and ROS production (Smith and Cox, 2008).
These effects of dapsone may be the explanation of the reduction in the histopathological and observational severity scores recorded in the current study which require a further focusing on elucidating the obscure about the use of topical dapsone in atopic dermatitis treatment.
Results demonstrated in this study revealed that there were non-signi icant differences between the levels of all studied variables in the irst week and those in the second, which may indicate that our work needs longer time to obviate the differences with the application of treatment.
Results obtained in the current work showed that IL-4, CBC and RBC were the only variables that signi icantly varied among the studied group in addition to observational severity and histopathological scores of epidermal thickness, Hyperkeratosis, Erosion and In lammation which is consistent with the above-discussed results. Moreover, the majority of studied variables showed signi icant differences among all studied groups after two weeks of treatment that owned to the longer duration of topical application that causes a different rate of response in mice subjected to the current research. Results demonstrated in the present study showed clearly that the elevation of IL-4 was accompanied by an increase in IL-13 which is inconsistent with the previously mentioned source of them from Th2 cells that activated in atopic dermatitis (Bao and Reinhardt, 2015).

CONCLUSIONS
Levels of the majority of studied variables were increased in response to induction of atopic dermatitis with topical DNCB which then reduced generally after topical application of tacrolimus. Topical application of dapsone showed an antiin lammatory effect that may be used in future as a promising treatment for A.D.