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. 2009 Mar 27;26(7):1635–1643. doi: 10.1007/s11095-009-9874-6

Immune Modulation by Adjuvants Combined with Diphtheria Toxoid Administered Topically in BALB/c Mice After Microneedle Array Pretreatment

Z Ding 1,3, E Van Riet 1, S Romeijn 1, G F A Kersten 2, W Jiskoot 1, J A Bouwstra 1,
PMCID: PMC2689355  PMID: 19326190

Abstract

Purpose

In this study, modulation of the immune response against diphtheria toxoid (DT) by various adjuvants in transcutaneous immunization (TCI) with microneedle array pretreatment was investigated.

Methods

TCI was performed on BALB/c mice with or without microneedle array pretreatment using DT as a model antigen co-administrated with lipopolysaccharide (LPS), Quil A, CpG oligo deoxynucleotide (CpG) or cholera toxin (CT) as adjuvant. The immunogenicity was evaluated by measuring serum IgG subtype titers and neutralizing antibody titers.

Results

TCI with microneedle array pretreatment resulted in a 1,000-fold increase of DT-specific serum IgG levels as compared to TCI. The immune response was further improved by co-administration of adjuvants, showing a progressive increase in serum IgG titers when adjuvanted with LPS, Quil A, CpG and CT. IgG titers of the CT-adjuvanted group reached levels comparable to those obtained after DT-alum subcutaneous injection. The IgG1/IgG2a ratio of DT-specific antibodies decreased in the following sequence: plain DT, Quil A, CT and CpG, suggesting that the immune response was skewed towards the Th1 direction.

Conclusions

The potency and the quality of the immune response against DT administered by microneedle array mediated TCI can be modulated by co-administration of adjuvants.

KEY WORDS: cholera toxin, CpG, diphtheria toxoid, microneedle array, transcutaneous immunization

INTRODUCTION

Currently, most vaccines are administrated by injection. Costs, risks and discomforts associated with the use and abuse of needles have boosted research on needle-free vaccinations (1). Around 10 years ago, Glenn, G.M et al. reported for the first time data on transcutaneous immunization (TCI) and showed that strong immune responses could be induced by topically applied cholera toxin (2). TCI is particularly attractive because of the high accessibility of the skin and the presence of antigen-presenting cells (APCs) in the epidermis and dermis, in particular the Langerhans cells (LCs) and the dermal dendritic cells (DCs) (3). However, the upper layer of the skin, the stratum corneum, acts as a barrier for diffusion of macromolecules and therefore is a major obstacle to dermal vaccine delivery. To overcome this barrier and achieve effective TCI, physical methods such as intradermal injection (4,5), thermal ablation (6), microdermabrasion (7) electroporation (8) and cavitational ultrasound (9) have been used. Physical disruption of the skin barrier increases the percutanous penetration of the antigen and makes the antigen more readily available for sampling by APCs (10). Moreover, disruption of the skin barrier may induce a chain of molecular events that lead to the secretion of pro-inflammatory cytokines and facilitate APC activation.

A relatively novel approach to disrupt the skin barrier in a controlled manner with little pain sensation is the use of microneedle arrays. It was proposed first by Gerstel and Place already in the 1970s (11). Ten years ago, when the technology for fabrication in micron dimensions became readily available, Prausnitz resumed the study using microneedle arrays in transdermal drug delivery (12). When used as a pretreatment, microneedle arrays enable antigens to diffuse along the transiently formed tiny conduits through the stratum corneum. Thereby antigens may be able to approach the LCs in the epidermis and the DCs in the dermis (13). Using ovalbumin-coated microneedle array, Matriano et al. evaluated the uniformity of skin piercing, and studied the dose of the vaccine used and the kinetics and magnitude of antibody titers induced in hairless guinea pigs (14). Widera et al. investigated the influence of important fabrication parameters, e.g. length and density of the microneedles, area and coating of the microneedle arrays, on vaccination efficiency of TCI (15). Hooper et al. reported that smallpox DNA vaccine-coated microneedle arrays applied topically in combination with electroporation protected mice against lethal challenge (16). Recently, Van Damme et al. tested the injectable microneedle array in human volunteers using influenza vaccine, resulting in a comparable seroprotection rate as compared to i.m. injection with 5 fold dose sparing (17). These interesting results show that TCI using microneedle array is promising. However, after more than 10 years of extensive research (18,19), there continues to be a need for further improvement of microneedle array mediated TCI, e.g. by using potent adjuvants or novel ways of applying the microneedle arrays.

Recently a new electric applicator was developed in our lab. It is designed to insert microneedle arrays into the skin with a predetermined velocity and thereby counteracts the elasticity of the skin. This applicator enables us to reproducibly pierce human and mouse skin in vivo with microneedles with a length of 300 μm or less (20). DT was recruited as a model antigen to evaluate the potential of microneedle array pretreatment in TCI. In a previous study the immunogenicity of topically applied DT was dramatically improved by microneedle array pretreatment as compared to untreated skin (21).

The objective of the present study was to determine the effect of adjuvants on the quantity and quality of the immune response against DT after TCI with microneedle array pretreatment (M-TCI). The Th1/Th2 balance of the immune response depends on several factors including the nature of the antigen and the adjuvant, the delivery route and the targeted APCs, as suggested by the ratio of IgG1/IgG2a antibody titers (22). The adjuvants included in this study, cholera toxin (CT), lipopolysaccharide (LPS), synthetic oligo deoxynucleotide containing a CpG motif (CpG), immunostimulatory fractions extracted from the bark of the tree Quillaja saponica (Quil A) and aluminum phosphate (alum), differ in their adjuvant mechanism and ability to modulate the immune response (see Table I) (22). Immune modulation by these adjuvants was evaluated in (M-)TCI and compared with conventional subcutaneous (s.c.) injection of DT or DT-alum, by measuring serum IgG (subtype) titers and neutralizing antibody titers.

Table I.

Properties of the Adjuvants Employed in the Current Study (Adapted from (22,47,48))

Adjuvant Type Cell-mediated immunity (Th1) Humoral immunity (Th2) Receptor
Cholera toxin Exotoxin +a +++ GM1 ganglioside
lpxL1 LPS Endotoxin ++ ++ TLR4
Quil A Saponin based +++ ++ Not identified
CpG Bacterial DNA ++++ + TLR9
Alum Inorganic salt + +++ Not identified

aHumoral and cellular immunity in arbitrary units represent the ability of adjuvants to enhance Th2 response or CTL or Th1, respectively, to foreign antigens

MATERIALS AND METHODS

Materials

Diphtheria toxin (batch 79/1), diphtheria toxoid (batch 98/40, protein content 12.6 mg/ml by BCA assay, 1 μg equal to approximately 0.3 Lf) and the lpxL1 LPS were provided by the Netherlands Vaccine Institute (NVI, Bilthoven, The Netherlands). Horseradish peroxidase-conjugated goat anti-mouse (HRP-GAM) IgG (γ-chain specific), IgG1 (γ1-chain specific) and IgG2a (γ2a-chain specific) were purchased from Southern Biotech (Birmingham, USA). Quil A and Adju-Phos® (alum) were obtained from Brenntag Biosector (Copenhagen, Denmark). CpG oligo deoxynucleotide 1826 (5′-tcc atg acg ttc ctg acg tt-3′, phosphorothioated) was synthesized by Isogen Biosolutions (IJsselstein, The Netherlands). Chromogen 3, 3′, 5, 5′-tetramethylbenzidine (TMB) and the substrate buffer were purchased from Biosource B.V. (Nivelles, Belgium). Cholera toxin was ordered from Sigma-Aldrich (Zwijndrecht, The Netherlands). Nimatek® (100 mg/ml Ketamine, Euovet Animal Health B.V., Bladel, The Netherlands), Rompun® (20 mg/ml Xylasine, Bayer B.V., Mijdrecht, The Netherlands) and the injection fluid (0.9% NaCl) were obtained from a local pharmacy. All other chemicals used were of analytical grade and all solutions were prepared with distilled water.

Animals

Female BALB/c mice (H2d), 8-week old at the start of the experiment were purchased from Charles River (Maastricht, The Netherlands), and maintained under standardized conditions in the animal facility of the Leiden/Amsterdam Center for Drug Research, Leiden University. The study was conducted in conformity with the Public Health Service Policy on use of laboratory animals and had been approved by the Research Ethical Committee of Leiden University (UDEC, nr. 07016).

Methods

Microneedle Array and Applicator

Assembled microneedle arrays were manufactured from commercially available 30G hypodermic needles (BD, Alphen a/d Rijn, The Netherlands) as described previously (13). The needles were assembled as a 300 μm-long, 4 × 4 array on a polymer back plate with a surface area of about 0.5 cm2. The electric applicator was developed and optimized as reported previously (21). The microneedles were pierced into mouse skin using a velocity of 3 m/s.

Immunization Study

The DT-alum formulations were prepared as previously described and the adsorption of DT to alum was between 70% and 80% (23). As control groups, 5 μg of DT (∼1.5 Lf) with and without alum in 100 μl solution/suspension was administered per mouse by s.c injection. The other vaccine-adjuvant formulations were freshly prepared by mixing DT and the adjuvants in buffer solution in appropriate amounts as indicated in Table II. One hundred micrograms DT and adjuvants per mouse were applied on intact skin (TCI) or on microneedle array pretreated skin (M-TCI) as previously described (21,24). A mutant of LPS, lpxL1 LPS, with reduced toxicity but retained adjuvanticity, was employed in this study (25). The dose of alum and lpxL1 LPS used in M-TCI were based on the w/w ratio of antigen/adjuvant used in injection control group and previous immunization study (25), respectively.

Table II.

Formulations Prepared for In Vivo (M-)TCI Study

DT dose (μg) Adjuvants Adjuvant dose (μg) Solvent (pH) Volume (μl)
for s.c. injection
5 AlPO4 150 0.9% saline (7.0) 100
5 0.9% saline (7.0) 100
(M)-TCI
100 PBSa (7.4) 70
100 lpxL1 LPS 25 PBS/Trisb (7.4) 70
100 Quil A 100 PBS (7.4) 70
100 CT 100 PBS (7.4) 70
100 CpG 100 PBS (7.4) 70
100 AlPO4 3,000 0.9% saline (7.0) 70

aPBS: 2.67 mM KCl, 1.47 mM KH2PO4, 137.93 mM NaCl, 8.06 mM Na2HPO4·7H2O, without Ca2 + and Mg2+

bPBS/Tris: PBS mixed with 1 mM Tris–HCl (v/v = 5:3).

During vaccination, mice were anaesthetized by intraperitoneal injection of 150 mg/kg ketamine and 10 mg/kg xylazine. For all groups receiving transcutaneous vaccination, the abdominal skin of the mice, shaved 24 h prior to vaccination, was first wiped with 70% ethanol. For M-TCI group, a skin fold was supported by styrofoam and pierced using the microneedle array and the electric applicator. Then 70 μl DT-adjuvant formulation was carefully spread to wet the entire skin area of application (microneedle array-pretreated or untreated, ∼2 cm2 area restricted by a metal ring). After 1 h of occlusive incubation, the skin area was extensively washed with lukewarm tap water and patted dry twice. All mice were immunized three times on day 1, 21 and 42 (at approximately the same skin region for all the TCI groups) and sacrificed on day 56. Blood was sampled from the tail vein one day before each immunization and the whole blood was collected from the femoral artery during sacrifice. Cell free sera were obtained using MiniCollect® tubes (Greiner bio-one, Alphen a/d Rijn, The Netherlands) by centrifugation after clot formation and stored at −80°C.

Serum Antibody Assay

Serum IgG, IgG1 and IgG2a titers were determined by sandwich ELISA as previously described (26). Briefly, ELISA plate (Microlon®, Greiner Bio-one, Alphen a/d Rijn, The Netherlands) wells were coated with DT at 4°C overnight. Two-fold serial dilutions of serum samples were applied in the plates and the containing DT-specific antibodies were detected by HRP-GAM IgG, IgG1 or IgG2a using TMB as substrate. Antibody titers are expressed as the reciprocal of the calculated sample dilution corresponding to half of the maximum absorbance at 450 nm of a complete s-shaped absorbance-log dilution curve. If samples were not diluted in the optimal range, additional measurements were performed to generate an s-shaped curve. Subsequently, the titers were calculated using a four-parameter fitting of the curve. Samples that did not reach the half-saturated absorbance value at the lowest (ten fold) dilution were considered as non-responders.

Neutralizing Antibody Assay

Immunity against diphtheria depends on the presence of circulating toxin-neutralizing antibodies. These antibodies were evaluated using Vero cell test, the WHO standard method to assess the success of diphtheria vaccination, which relies on the inhibition of a cytotoxic dose of diphtheria toxin (26). In brief, after complement inactivation, two-fold serial dilutions of serum samples were prepared with complete medium 199 (CM199, Gibco, Breda, The Netherlands) and applied to microtiter plates (CELLSTAR®, Greiner Bio-one, Alphen a/d Rijn, The Netherlands). Subsequently, 2.5 × 10−5 Lf diphtheria toxin was added to the wells. After 2 h incubation at 37°C for neutralization, Vero cells suspension in CM199 was added to each well. Covered with a plate sealer, Vero cells were incubated at 37°C in 5% CO2 for 6 days. The end point was taken as the highest serum dilution protecting the Vero cells.

Statistical Analysis

ELISA titers were logarithmically transformed for better normality before statistical analysis. Two way ANOVA with Bonferroni posttest, one way ANOVA with Tukey posttest, or Kruskal–Wallis nonparametric test with Dunns posttest were performed as indicated. Statistical analysis was carried out using Prism Graphpad and a p value less than 0.05 was considered to be significant.

RESULTS

During the immunization study, there was no adverse effect from the shaving, anesthesia, piercing, immunization, or washing procedure observed. Neither erythema nor induration was seen at the immunization site after exposure of antigen and adjuvants.

Immune Response Improved by Microneedle Array Pretreatment

The IgG titers of mice from all groups after prime, first boost and second boost (day 20, 41 and 56) are shown in Fig. 1a–e and an overview of the DT-IgG titers after the second boost is shown in Fig. 1f. It is clear that non-adjuvanted DT did not result in a substantial IgG response when applied on intact skin (TCI). Microneedle array pretreatment provided major improvement to the immunogenicity of DT. After prime, more mice responded with higher mean IgG titers in the M-TCI group than in the TCI group. After the first boost, all mice responded and the IgG titers were 100 fold higher in the M-TCI group (p < 0.01) and the difference of IgG titers was further increased to over 1,000 fold after the second boost (p < 0.001, Fig. 1a). Immunogenicity of DT was further improved by the co-administered adjuvants e.g. Quil A, CpG and CT in M-TCI. The improvement by the adjuvant in question is indicated by the space in between the black and the brown lines in Fig. 1b, c, d and e, respectively. DT-specific IgG titers in the CT M-TCI group after the second boost were the highest among all M-TCI groups and reached very close level to those from DT-alum injection group (p > 0.05). For the adjuvants in the absence of microneedle array pretreatment, their effects on the DT immunogenicity were more variable and less pronounced. Only CT moderately improved the IgG titers after the second boost (Fig. 1a, e, p < 0.05), while the presence of the other adjuvants did not augment the IgG titers significantly. Comparing the two injection control groups, alum speeded up IgG development and increased the IgG titers significantly (p < 0.001 after first boost). However, when DT-alum was applied in M-TCI, no adjuvanticity was observed as the IgG titers were lower than those of plain DT in M-TCI (data not shown).

Fig. 1.

Fig. 1.

DT-specific IgG titers to dermally delivered DT with (M-TCI) and without (TCI) microneedle array pretreatment of the skin: a Plain DT; b DT + LPS; c DT + Quil A; d DT + CpG; e DT + CT. Sera were collected after prime, first boost and second boost (day 20, 41 and 56) and antibodies were determined by ELISA. TCI with DT + LPS was not carried out. An overview of the DT-specific IgG titers after the second boost for the M-TCI and s.c. injection groups are shown in f. Data are shown as mean + SD (n = 8). Non-responders were given an arbitrary titer of 10 (*p < 0.05, **p < 0.01, ***p < 0.001, two way ANOVA with Bonferroni posttest).

Immune Modulation by Adjuvants in M-TCI

Focusing on the M-TCI, immune modulation functions of the adjuvants were investigated. The DT-specific IgG1 and IgG2a titers in the sera collected after prime, first boost and second boost (day 21, 42 and 56) were determined (Fig. 2). For all adjuvants, IgG1 showed similar titers as compared to the total IgG titers and each vaccination showed a booster effect. After the first boost, Quil A and CT enhanced the IgG1 titers significantly as compared to plain DT (p < 0.01 and 0.001, respectively). After the second boost, only CT significantly enhanced the IgG1 titers as compared to plain DT (p < 0.01). A clear effect of the adjuvants on the IgG2a titers was observed after the second boost, which increased in the following sequence: plain DT, LPS, Quil A, CT and CpG.

Fig. 2.

Fig. 2.

DT-specific IgG1 and IgG2a titers during M-TCI. Sera were collected after prime, first boost and second boost (day 20, 41 and 56) and antibodies were determined by ELISA. Data shown as mean + SD (n = 8). Non-responders were given an arbitrary titer of 10. (*p < 0.05, **p < 0.01, ***p < 0.001, two way ANOVA with Bonferroni posttest).

The IgG1/IgG2a ratio, which is considered a measure for the Th1/Th2 balance of the immune response (27), of individual mice from each group after the second boost was calculated and presented in Fig. 3. Plain DT and DT-alum induced an IgG1 biased response when delivered via s.c. injection. Applying plain DT by M-TCI induced the same IgG1/IgG2a ratio as by s.c. injection. With adjuvants, the ratio decreased in the following sequence: plain DT, Quil A, CT and CpG, suggesting that the Th2 biased immune response induced by plain DT was skewed towards the Th1 direction.

Fig. 3.

Fig. 3.

DT-specific IgG1/IgG2a ratios of individual mouse after M-TCI. Sera were collected on day 56, DT-specific IgG1 and IgG2a titers were measured by sandwich ELISA. IgG1/IgG2a ratios were calculated only using IgG2a responders. Data shown as mean + SD (n = 8, **p < 0.01 and ***p < 0.001, one-way ANOVA with Tukey posttest).

Protective Immunity of DT in M-TCI

The protective immunity of DT with the serial of immune modulators in M-TCI was evaluated using the Vero cells test (Fig. 4). Although for LPS, Quil A and CpG groups the neutralizing antibody titers were not significantly different from those for plain DT, improvement was seen for the CT group (p < 0.05). The mean titer was very close to that of the DT-alum injection group, and the difference was not significant (p > 0.05). As expected, the groups that had received formulations on untreated skin (TCI) did not show detectable neutralizing antibody titers.

Fig. 4.

Fig. 4.

Diphtheria toxin-neutralizing antibody titers after M-TCI. Serum samples were collected after the second boost (day 56) and determined by Vero cell test. Data are expressed as logarithm of the highest dilution that was still capable of protecting the Vero cells from the challenge of diphtheria toxin (filled circle the M-TCI groups, empty circle the injection groups, *p < 0.05, **p < 0.01, ***p < 0.001, Kruskal–Wallis nonparametric test with Dunns posttest).

DISCUSSION

This is the first study in which the immune modulatory activity of several known adjuvants was directly compared in TCI with microneedle array pretreatment, using DT as a model antigen. In this study, we first compared the immune responses of DT formulated with different adjuvants in TCI and M-TCI. Then we focused our study on the modulation capability of these adjuvants to the immune response in M-TCI.

Application of DT on intact skin did not induce a substantial immune response in the absence or presence of the tested adjuvants. The poor penetration of DT across the stratum corneum seems to be the limiting factor, since the antibody titers of DT in TCI was strongly increased by microneedle array pretreatment. The skin barrier disruption and increased DT diffusion across the stratum corneum provided remarkable improvement to the immune response via TCI, similar as the tape-stripping method, however, through a practically easier and more controllable approach (28). Co-administration of adjuvants in M-TCI was able to further augment the immunogenicity of DT and demonstrated marked differences between the immune stimulatory activities of the adjuvants. In the following section, the tested adjuvants are discussed individually concerning their mechanism of action and the role of delivery route in the augmentation and modulation of DT immune response.

CT is a molecule with five nontoxic B subunits (CTB) surrounding a single, toxic A fragment (CTA). Both the CTB-mediated specific binding to the GM1 ganglioside receptors and the ADP-ribosyltransferase activity of CTA have been reported to be of importance for the immune stimulatory properties of CT (29,30). Whereas CT is a well-documented Th2 immune modulator in conventional and mucosal vaccination (30), our results point to a more Th1 biased response against DT when co-administered with CT via M-TCI. The Th1 skewing of CT in TCI was also reported by Stickings et al. using mutant diphtheria toxin, CRM197, as model antigen (31) and by Skountzou et al. using influenza vaccine (32). This suggests that the Th1 skewing of CT is delivery-route dependent. Studies performed by Anjuere et al. using ovalbumin as prototype antigen clarified that CTB suppresses systemic Th1 responses when given by a mucosal route, but potentiates these responses when administered by TCI. This finding underscores the role of the epithelial microenvironment in the regulation of immune responses and reflects the DC heterogeneity between mucosal tissue and skin (33).

The signaling of CpG starts by engagement of Toll-like receptor 9 (TLR9), followed by induction of pro-inflammatory cytokine (e.g. IL-12, TNF-α and IFN-γ) expression, and results in a Th1 biased response (34). In our present study, CpG induced the highest IgG2a titers among all M-TCI groups and our results strongly support a skewing of the Th1/Th2 balance towards the Th1 direction, similar to the immune modulatory effect of CpG in mucosal and injection vaccination. Although at the site of application TLR9 is not constitutively expressed by the LCs, it is almost exclusively expressed by the keratinocytes in the upper and most differentiated layer of the epidermis. Their TLR9 expression and reactivity to CpG is reported to be greatly up-regulated by transforming growth factor (TGF-α), a growth and differentiation factor present after skin barrier disruption and during wound healing (35).

Quil A is composed of immune-stimulatory fractions extracted from the bark of the tree Quillaja saponica. The Quil A concentration (1.43 mg/ml) used in the applied formulation was well above its reported critical micelle concentration of 0.3 mg/ml (36). The average particle size of the DT-Quil A dispersion in PBS was about 56 nm with a PDI of 0.10, as measured by dynamic light scattering. Quil A is a potent Th1 biased adjuvant when given by i.m. injection (37). In M-TCI, it improved the IgG titers marginally as compared to the non-adjuvanted DT (p < 0.05 after the first boost; p > 0.05 after the second boost). The ratios of anti-DT IgG1/IgG2a titers were significantly lowered as compared to M-TCI of plain DT (p < 0.01), suggesting that it skewed the response towards the Th1 direction.

LPS, major outer membrane constituent of Gram-negative bacteria, stimulates APCs through TLR4, induces high levels of pro-inflammatory cytokines and usually leads to a strong Th1 response (38). The DT-lpxL1 LPS dispersion applied in our study had a bigger average particle size than Quil A, about 300 nm with a PDI of 0.45, indicating that relatively large complexes had been formed. In M-TCI, the effect of the lpxL1 LPS mutant on the anti-DT IgG, IgG1, IgG2a and the neutralizing antibody titers was not significant (p > 0.05). This may be due to the following factors: (a) LCs do not express TLR4 and do not respond to bacteria or LPS (39). TLR4 expression by mouse keratinocytes also seems limited. Besides few data available from mice, reports on TLR4 expression by human keratinocytes are conflicting (40,41); (b) Although little is known about the actual diffusion of these dispersions across the conduits induced by the microneedles, previous studies of our group showed that fluorescently labeled particles of ca. 200 nm did pass through the conduits created by the same microneedle arrays as used in the present study (20). However, as no quantitative information is available, it is possible that only a limited amount of the DT-lpxL1 LPS dispersion reached the DCs in the dermis; (c) the LPS mutant may work in a less efficient way as the original LPS in the epidermal/dermal microenvironment. Further studies are required to elucidate the exact mechanism. The different reactivity of skin immune system to CpG and LPS may be involved in a strategic control of host defense to the bacterial commensal skin flora (39).

Alum did not show any adjuvanticity in M-TCI. It induced lower IgG and IgG1 titers than those of non-adjuvanted DT group after each vaccination. Furthermore, alum in M-TCI did not induce detectable IgG2a titers and provided no protection in the Vero cell test after the second boost (data not shown). This may partially be due to the size of DT-alum particles, several microns in diameter, which prevents their diffusion through the conduits in sufficient amount to exert a ‘depot’ effect (42). The adjuvanticity of alum could also be dependent on the epithelial microenvironment; the danger signal it induces through injection, the uric acid production (43), may not be provoked in the dermis and epidermis.

Interestingly, when comparing IgG subtype titers and neutralizing antibody titers between CpG and Quil A groups (Figs. 1 and 4), the CpG group, with similar IgG titers, but much higher IgG2a titers than the other, induced similar to slightly lower neutralizing antibody titers, which indicates that IgG2a might not contribute to toxin-neutralization. This was confirmed by the comparison between CpG and CT groups, also showing that higher IgG2a titers did not result in higher neutralizing antibody titers. IgG1 seems to be the main neutralizing antibody for protection, as IgG1 titers significantly correlated with neutralizing titers. However, IgG1 titers could not be used to predict individual neutralizing antibody titers with great accuracy, which is in line with a diphtheria vaccination study done in human infants (44). Therefore, from an application perspective, CpG in M-TCI is more suitable for anti-viral immune responses such as influenza vaccination where IgG2a provides the main immune protection and a Th1 biased response is more desired (45).

In this study, a high dose of DT, 20 times of that used in the s.c. injection group, was applied in M-TCI. This dose is similar to the dose of DT used by Glenn et al. in previous studies (24,46). High doses were used as apparently only a fraction of DT applied actually enters epidermis/dermis. A limiting factor for diffusion of the antigen into the skin is that the mice used for this study can only be kept under anesthesia for about 1 h. This is not a limitation of the transcutaneous route, but a limitation of the animal model used. The high doses used until now also indicate that formulation improvement to increase the efficiency of the immune response is very important in transcutaneous vaccination. Conjugation and encapsulation of adjuvants into vaccine-containing particles and specific DC and LC targeting approaches could be attractive strategies to further improve the potency of vaccine formulations for M-TCI.

CONCLUSION

We have shown that the type of adjuvant used has a significant effect on the immune response and protective immunity against DT in M-TCI. The epithelial microenvironment and DC heterogeneity also play an important role in the regulation of the immune response. This delivery method is applicable to many other vaccines by formulating with proper adjuvants and holds a lot of promise for future use.

Acknowledgements

Henk Verpoorten from the Fine Mechanic Department (FMD) of Leiden University is acknowledged for manufacturing the assembled microneedle arrays. Dr. Rob J. Vandebriel from the National Institute of Public Health and the Environment (RIVM) of the Netherlands is acknowledged for helpful discussions. This work was financially supported, in part, by the Chinese Scholarship Council (CSC).

Open Access This article is distributed under the terms of the Creative Commons Attribution Noncommercial License which permits any noncommercial use, distribution, and reproduction in any medium, provided the original author(s) and source are credited.

Abbreviations

Alum

Adju-Phos®, colloidal aluminum phosphate

CM199

complete medium 199

CRM 197

cross-reacting material of diphtheria toxin

CT

cholera toxin

DT

diphtheria toxoid

HRP-GAM IgG

horseradish peroxidase conjugated goat anti-mouse IgG

M-TCI

TCI with microneedle array pretreatment

TCI

transcutaneous immunization

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