Patent Application: US-23216799-A

Abstract:
nanoparticle coacervates of nucleic acids and polycations serve as effective vaccines when administered orally . they can induce immunity to a variety of disease causing agents and raise a protective response to allergens .

Description:
the disclosures of prior u . s . patent applications ser . nos . 08 / 265 , 966 , and 08 / 657 , 913 are expressly incorporated herein . our novel approach of using dna nanospheres for oral administration has demonstrated the general utility of oral dna - based immunization . the induced response may be either or both humoral or cellular . it may be used for inducing any type of immune response desired . this may be against bacterial , viral , fungal , parastic , or tumor - associated antigens . any type of expression construction can be used to obtain expression in the vaccinated mammal of the antigen gene . typically the gene will be operably linked to a promoter which is active in the recipient cells . viral promoters , such as cmv are particularly useful for this purpose , although any known promoter can be used . the gene or oligonucleotide encoding the antigen can be in the form of rna , dna , cdna . the antigen can be any known in the art , including but not limited to an allergen , particularly a food allergen , or a bacterial , viral , fungal , parastic , or tumor - associated antigen . the crucial aspect of the invention is the administration of the vaccines by the oral route . thus the formulation may be any which is safe and healthy for oral ingestion . preferably the formulation contains no toxic substances . if in a liquid form , sterility may be desired . the form of the vaccine may be as a tablet , capsule , liquid , elixir , powder , granules , etc . it may be admixed with food or drink . it may self - adminstered for added convenience rather than requiring the expense of a health professional for administration as is often required for injections and other inocculations . it is preferred that the nanospheres be less than 5 microns . more preferred are nanospheres of less than 3 microns , and even more proffered are nanospheres which are less than 2 , 1 , 0 . 5 , and 0 . 1 microns . while size can be effected by the conditions of coacervation and the size of the component polyanion and polycation , nanospheres of the desired size can also be size selected using a technique which separates the nanospheres on the basis of size . the particles can be size - fractionated , e . g ., by sucrose gradient ultracentrifugation . particles with size less than 150 nanometers can access the interstitial space by traversing through the fenestrations that line most blood vessels walls . the polymeric polycation from which the coacervate is formed can be any which is biologically degradable , and safe for oral ingestion . this includes , but is not limited to gelatin and chitosan . polyamino acids , synthetic or naturally occurring , can also be used , such as polylysine , poly - lysine - poly - arginine , polyarginine , protamine , spermine , spermidine , etc . polysaccharides may also be used . targeting ligands , if desired , can be directly bound to the surface of the nanosphere or can be indirectly attached using a “ bridge ” or “ spacer ”. because of the amino groups provided by the lysine groups of the gelatin , the surface of the nanospheres can be easily derivatized for the direct coupling of targeting moieties . for example , carbo - diimides can be used as a derivatizing agent . alternatively , spacers ( linking molecules and derivatizing moieties on targeting ligands ) such as avidin - biotin can be used to indirectly couple targeting ligands to the nanospheres . biotinylated antibodies and / or other biotinylated ligands can be coupled to the avidin - coated nanosphere surface efficiently because of the high affinity of biotin ( k a ˜ 10 15 m − 1 ) for avidin ( hazuda , et al ., 1990 , processing of precursor interleukin 1 beta and inflammatory disease , j . biol . chem ., 265 : 6318 - 22 ; wilchek , et al ., 1990 , introduction to avidin - biotin technology , methods in enzymology , 184 : 5 - 13 ). orientation - selective attachment of iggs can be achieved by biotinylating the antibody at the oligosaccharide groups found on the f c portion ( o &# 39 ; shannessy , et al ., 1984 , a novel procedure for labeling immunoglobulins by conjugation to oligosaccharides moieties , immunol . lett ., 8 : 273 - 277 ). this design helps to preserve the total number of available binding sites and renders the attached antibodies less immunogenic to f c receptor - bearing cells such as macrophages . spacers other than the avidin - biotin bridge can also be used , as are known in the art . for example , staphylococcal protein a can be coated on the nanospheres for binding the f c portions of immunoglobulin molecules to the nanosphetes . cross - linking of linking molecules or targeting ligands to the nanosphere is used to promote the stability of the nanosphere as well as to covalently affix the linking molecule or targeting ligand to the nanosphere . the degree of cross - linking directly affects the rate of nucleic acids released from the nanospheres . cross - linking can be accomplished using glutaraldehyde , carbodiimides such as edc ( 1 - ethyl - 3 -( 3 - dimethylaminopropyl )- carbodiimide , dcc ( n , n ′- dicyclohexylcarbodiimide ), carboxyls ( peptide bond ) linkage , bis ( sulfosuccinimidyl ) suberate , dimethylsuberimidate , etc . targeting ligands according to the present invention are any molecules which bind to specific types of cells in the body . these may be any type of molecule for which a cellular receptor exists . preferably the cellular receptors are expressed on specific cell types only . examples of targeting ligands which may be used are hormones , antibodies , cell - adhesion molecules , saccharides , drugs , and neurotransmitters . the nanospheres of the present invention have good loading properties . typically , following the method of the present invention , nanospheres having at least 5 % ( w / w ) nucleic acids can be achieved . preferably the loading is greater than 10 or 15 % nucleic acids . often nanospheres of greater than 20 or 30 %, but less than 40 or 50 % nucleic acids can be achieved . typically loading efficiencies of nucleic acids into nanospheres of greater than 95 % can be achieved . the method of the present invention involves the coacervation of polymeric cations and nucleic acids . because this process depends on the interaction of the positively charged polymeric cations and the negatively charged nucleic acids it can be considered as a complex coacervation process . however , sodium sulfate ( or ethanol ) induces the coacervation reaction by inducing a phase transition , and therefore it could also be considered as a simple coacervation reaction . nucleic acids are present in the coacervation mixture at a concentration of between 1 ng / ml to 500 μg / ml . desirably the nucleic acids are at least about 2 - 3 kb in length . sodium sulfate is present at between 7 and 43 mm . gelatin or other polymeric cation is present at between about 2 and 7 % in the coacervation mixture . nanosphere delivery vehicles synthesized by the complex coacervation of dna with either gelatin or chitosan have several potential attractive features : 1 ) ligands may be conjugated to the nanosphere for targeting or stimulating receptor - mediated endocytosis ; 2 ) lysosomolytic agents can be incorporated to reduce degradation of the dna in the endosomal and lysosomal compartments ; 3 ) other bioactive agents or multiple plasmids can be co - encapsulated ; 4 ) bioavailability of the dna can be improved because of protection from serum nuclease degradation by the matrix ; 5 ) the nanosphere can be lyophilized for storage . an attractive nanosphere delivery system requires a delicate balance among factors such as the simplicity of preparation , cost effectiveness , nucleic acids loading level , controlled release ability , storage stability , and immunogenicity of the components . the gene delivery system described here may offer advantages compared to other particulate delivery systems , including the liposomal system . the problems of instability , low loading level , and controlled release ability are better resolved with the polymeric nanosphere systems . gelatin has received increasing biologic use ranging from surgical tissue adhesive ( weinschelbaum , et al ., 1992 , surgical treatment of acute type a dissecting aneurysm with preservation of the native aortic valve and use of biologic glue . follow - up to 6 years , j . thorac . cardiovasc . surg ., 130 : 369 - 74 ) to quantitative immunohistochemical assays ( izumi , et al ., 1990 , novel gelatin particle agglutination test for serodiagnosis of leprosy in the field , j . clinical microbiol ., 28 : 525 - 9 ) and as drug delivery vehicle ( tabata , et al ., 1991 , effects of recombinant alpha - interferon - gelatin conjugate on in vivo murine tumor cell growth , cancer res ., 51 : 5532 - 8 ), due to its biocompatibility and enzymatic degradability in vivo . compared to other synthetic polymeric systems , such as the extensively studied polylactic / polyglycolic copolymers , the mild conditions of nanosphere formulation are appealing . unlike the solvent evaporation and hot - melt techniques used to formulate synthetic polymeric nanospheres , complex coacervation requires neither contact with organic solvents nor heat . it is also particularly suitable for encapsulating bio - macromolecules such as nucleic acids not only through passive solvent capturing but also by direct charge - charge interactions . unlike viral vectors , which cannot deliver genes larger than 10 kb , the nanosphere delivery system of the present invention does not have such size limitations . nucleic acid molecules of greater than about 2 kb can be used , and nucleic acid molecules even greater than 10 kb may be used . typically the nucleic acid will be greater than 300 bases , and typically greater than 0 . 5 , 1 , 2 , 5 , or 10 kb . typically the nucleic acid molecule will be less than 200 , 100 , or 50 kb . the above disclosure generally describes the present invention . a more complete understanding can be obtained by reference to the following specific examples which are provided herein for purposes of illustration only , and are not intended to limit the scope of the invention . we have evaluated the modulation of peanut allergen ( as a model allergen )- induced hypersensitivity using an oral chitosan / dna - based immunization approach . the model for this study is the hypersensitivity responses to peanut allergens in an inbred strain of mice ( c3h ), in which several quantitative parameters of hypersensitivity have been established , and a significant induction of the immune response has . been demonstrated following gene immunization . this system demonstrates that antigens can be delivered to the systemic circulation of the animal by oral administration of a dna . materials : approximately 6 - 7 weeks old inbred strains of c3h and akr / j mice were purchased from charles river laboratories , massachusetts . plasmid encoding the peanut allergen arah2 ( parah2 ) was grown in a large scale by peg method . high molecular weight chitosan ( c390 , mw ˜ 390 , 000 ) and low molecular weight chitosan ( pcl113 , mw ˜ 60 , 000 - 100 , 000 ) were used as the polycation to complex with the dna . gene expression construct : pcr3arah2 : burks et al ( 33 - 34 ) have identified two major protein fractions in peanuts , ara h1 ( 63 . 5 kd ) and ara h2 ( 17 kd ), and over 95 % of peanut allergic patients are sensitive to these proteins . we have generated an ara h2 gene construct , pcr3arah2 in an expression vector ( pcr3 ). a pcr - amplified ara h2 coding region gene segment with the addition of a kozak consensus translation codon was ligated into pcr3 expression vector containing cmv promoter sequence . nanosphere preparation : briefly , dna - chitosan nanospheres were prepared as described previously . briefly , a 0 . 02 % solution of chitosan ( ph 5 . 7 in naac - hoac buffer ) is vortexed with a 50 ug / ml dna solution in 50 mm sodium sulfate at 55 ° c . for 15 - 20 seconds . for the low molecular weight chitosan the concentration was changed to 0 . 04 % in deionized water ( ph adjusted to 5 . 7 ) and the salt concentration was 5 mm sodium sulfate . oral delivery : all nanospheres were prepared fresh before administration and kept at room temperature . un - anesthetized mice were fed different formulations of nanospheres and “ naked ” dna at a dose of 50 ug dna per mice . feeding ( intra - gastric delivery ) was performed using a 1 ml syringe fitted with an animal feeding needle ( fisher scientific , usa ). the feeding volume was 1 ml for each mice . experimental . protocols : the study was divided into two experiments : the first to examine the immune response at different time points after vaccination and the second to study the protection efficacy of the immunization protocol . in the first study the experimental groups were as follows : group 1 : single dose of high molecular weight chitosan - parah2 nanospheres , group 2 : one dose of high molecular weight chitosan - parah2 nanospheres followed by a booster shot after 2 weeks , group 3 : single dose of low molecular weight chitosan - parah2 nanospheres , group 4 : one dose of low molecular weight chitosan - parah2 nanospheres followed by a booster shot after 2 weeks , group 5 : naked dna ( parah2 ), group 6 : single dose of low molecular weight chitosan - pegfp ( plasmid encoding the firefly green fluorescence protein , clontech inc , usa ) nanospheres and group 7 : naive mice fed with phosphate buffered saline ( pbs ). in the second experiment the study groups were : group 1 : one dose of high molecular weight chitosan - parah2 nanospheres followed by a booster shot after 2 weeks , group 2 : one dose of low molecular weight chitosan - parah2 nanospheres followed by a booster shot after 2 weeks , group 3 : single dose of low molecular weight chitosan - parah2 nanospheres , group 4 : naive mice fed with pbs . sample collections and measurements : for the first study serum and fecal extracts were collected at different time points after the first immunization . briefly , for serum collection , 1 φul of blood was collected from the tail vein of each mice , clotted at room temperature for one hour and then centrifuged at 1000 rpm for 25 min . the resulting supernatant ( serum ) was stored at − 80 ° c . till antibody measurements were performed . for fecal extracts , one or two drops of fresh fecal pellets were collected , weighed and dissolved in pbs ( 100 mg / ml ). the debris were centrifuged at 14 , 000 rpm for 25 min and the supernatant was stored at − 80 ° c . for measurements . anti - arah2 specific igg or iga levels in serum and fecal extract were measured using an antigen specific elisa ( enzyme linked immuno - sorbent assay ). microtiter plates were coated overnight with 10 ug / ml ( 100 ul ) of purified arah2 protein in sodium carbonate - bicarbonate buffer . plates were blocked for 2 hrs in room temperature with 4 % bovine serum albumin , 2 % normal goat serum in pbs and then incubated with serial dilutions of serum or fecal extract for 18 hrs following the incubation , biotinylated anti - igg or anti - iga added to the wells for 1 hr at 37 ° c . the plates were then incubated with hrp conjugated streptavidin for 30 min at room temperature and developed with o - phenyladeneline ( opd ). absorbances were read at 490 nm using a microplate reader ( bio - rad lab ., usa ). igg titers were measured by coating the plates with different concentrations of mouse igg followed by the biotinylated antibody and subsequent steps . iga data was expressed as o . d . values . challenge and protection study : two weeks following the booster dose i . e ., four weeks after the first immunization all mice were sensitized orally and intra - peritoneally with crude peanut extracts . sensitization was performed 3 more times one week apart . following sensitization , mice were challenged intra - peritoneally with 1 mg of purified arah2 protein and anaphylactic response was observed and graded as described below . peanut - induced hypersensitivity in c3h mice : an inbred strain of mice , c3h , has been shown to exhibit immediate hypersensitivity following sensitization with ova together with ctx as an adjuvant ( 17 ). to examine the effect of oral sensitization of c3h mice with peanut allergen extracts ( pn ), we have performed studies using . various sensitization protocols , and developed quantitative parameters for measuring pn - induced hypersensitivity ( 16 ). symptoms of anaphylaxis became apparent in mice 5 to 10 min , peaked at 30 to 50 min , after ag challenge . the severity of symptoms was determined by observing mouse behavior post - challenge , and was scored by their responses to stimuli such as mild prodding . anaphylaxis was classified by the following scoring system : 0 , no sign of reaction ; 1 , scratching and rubbing around the nose and head ; 2 , decreased activity with an increasing respiratory rate , pilar erecti and / or puffing around the eyes ; 3 , labored respirations , cyanosis around the mouth and tail ; 4 , slight or no activity after prodding or tremors , convulsion ; 5 , death . this scoring system was established based on our previous experiments and a modified scoring system used previously ( 35 ). results in fig1 shows that there were positive antibody responses in groups immunized by the dna nanospheres . most importantly , the hypersensitivity study shows that significantly improved response in terms of symptoms of anaphylaxis in mice immunized by the dna nanospheres ( fig2 ). chitosan ( mw ˜ 390 , 000 ) was purchased from vansen inc ., wa , usa . to generate an expression gene construct containing a major peanut allergen gene , arah2 , a pcr - amplified arah2 coding region gene segment ( kindly provided by dr . g . bannon , university of arkansas ) with the addition of a kozak consensus translation codon was ligated into pcr3 expression vector containing cmv promoter / enhancer sequences . the resultant expression construct was designated as pcmv arah2 . plasmid encoding β - galactosidase ( p43lacz ) was a gift from dr . barry byrne , university of florida . 4 - 5 weeks old male akr / j mice were obtained from jackson laboratories massachusetts , usa . nanoparticles were made with chitosan and dna as described before 24 . briefly , 10 μg of plasmid was added to 100 μl of sodium sulfate and heated to 55 ° c . chitosan ( 0 . 02 %) was also heated to the same temperature and 100 μl of chitosan was added to the dna - sodium sulfate solution while vortexing at high speed for 20 sec . particles were examined immediately under light microscope and stored at room temperature the particles were characterized by size and zeta - potential using a zetasizer 3000 , malvern instruments inc ., massachusettes , usa . the number distribution of particle size as analyzed by the zetasizer and the zeta - potential ( ph 5 . 7 ) as measured in an aqueous dip cell was used for quality control of the nanoparticles . these particles were further characterized by transmission and scanning electron micrography . for tem freshly prepared particles were placed on a glow discharged carbon grid , allowed to sit for a few minutes and then air - dried . the grid rotary shadowed at 7 degrees with plantinum . a zeiss transmission electron microscope was used to visualize the particles . for sem , cells were grown on coverslips and incubated with nanospheres for 10 min . following incubation they were fixed , dehydrated in graded ethanol , critical point dried for several cycles and sputter coated with platinum . the particles on cell surface were than visualized through a scanning electron microscope . akr / j mice were fed with either chitosan - dna nanoparticles containing the lacz gene ( p43lacz ) or with naked plasmid dna ( p43lacz ) using animal feeding needles . five days later the animals were sacrificed and their stomachs and small intestines were surgically removed . the whole tissues were stained with 4 - chloro - 5 - bromo - 3 - indolyl - β - galactoside ( x - gal ) according to standard protocols . following overnight staining in a humidified chamber , the tissues were photographed at pathology photography , johns hopkins hospital . the pictures were scanned into a computer and adjusted equally for brightness and contrast using adobe photoshop . the tissues were then frozen in oct and cut into thin sections . the sections were counter stained with nuclear fast red and visualized under a light microscope equipped with a digital camera . pictures were adjusted equally for brightness and contrast in adobe photoshop . akr / j mice were divided into different experimental groups and immunized orally with various formulations using animal feeding needles ( fisher scientific inc ., usa ) attached to a one ml syringe . each mouse was fed with a ˜ 50 μg dna dose in a volume of 500 - 900 μl ( depending upon the formulations ). the anaphylactic protection experiments were repeated with different experimental and control groups . blood and fecal extract were collected from immunized and control mice to measured secreted iga levels in fecal extract , serum igg2a , increase in serum ige pre vs . post immunization and release of plasma histamine following ag challenge . blood was collected at 4 weeks ( before sensitization ) and 7 weeks ( immediately after sensitization but before challenge ) through tail vein bleeding from different groups of mice . after 30 min to 1 hr at room temperature the blood was centrifuged at 4 ° c . for 25 - 30 min and serum ( supematant ) was collected and stored at − 80 ° c . until further measurements . fecal pellets were also collected from the same groups of mice at 3 and 4 weeks after immunization and frozen at − 80 ° c . for further measurements . all mice were sensitized three times , one week apart , with crude peanut extract . each sensitization was performed over two consecutive days ; first day by oral administration of 1 mg crude peanut extract with 10 μg cholera toxin per mouse and the second day by i . p . administration of 0 . 5 μg extract per mouse with aluminum hydroxide as adjuvant . in both cases the administration volume was 200 μl per mouse . elisa was performed on serum collected pre and spot sensitization to determine ige and igg2a levels and on fecal extracts to measure secretory iga . briefly , plates were coated with has - dnp standards or arah2 protein ( 10 μg / ml ) at 4 ° c . overnight . blocking was performed for 2 hrs at 37 ° c . with 1 % bsa - pbst . serum samples were pooled for each group , was added in duplicate ( 1 : 5 dilution for ige and 1 : 20 for igg2a ), and incubated overnight at 4 ° c . biotinylated anti - mouse iga , ige and igg2a were added followed by the addition of streptavadin - hrp and tmb substrate . the plates were read at 450 nm in a microplate manager ( bio rad , usa ). for histamine measurements immunized and control mice were challenged with purified arah2 and after 12 - 15 min blood was collected from the optic artery and the plasma was assayed for histamine levels using a competive elisa based histamine kit ( immunotech inc ., usa ). first , non - immunized ( sensitized ) mice were challenged i . p . with 200 μg of arah2 protein . anaphylactic reactions were graded at different time points according to previously reported contentions . briefly the following grading protocol was observed . anaphylaxis was classified by the following scoring system : 0 , no sign of reaction ; 1 scratching and rubbing around the nose and head ; 2 , decreased activity with an increasing respiratory rate , pilar erecti and / or puffing around the eyes ; 3 , labored respiration , cyanosis around the mouth and tail ; 4 , slight or no activity after prodding or tremors , convulsion ; 5 , death . anaphylactic vascular leakage was measured using evan &# 39 ; s blue assay . briefly 200 μl of evan &# 39 ; s blue dye was injected into the tail vein of mice and immediately followed by an i . p challenge of 200 μg arah2 . mice were monitored for 45 min and sacrificed to record effect of anaphylactic vascular leakage as judged by blue color in the extremities . mice that develop anaphylaxis have blue extremities due to vascular leakage while immunized mice that are protected from anaphylaxis are expected to have no / reduced blue color . photograph was taken using a nikon camera and developed as ektachrome slides . the slide was scanned in , enlarged and adjusted for brightness and contrast using adobe photoshop . the nanoparticles were synthesized by complexing high molecular weight (˜ 390 , 000 ) chitosan with pdna . uniform particles were obtained by adding 0 . 02 % chitosan , ph 5 . 7 ( at 55 ° c .) into pdna ( 50 μg / ml in 50 mm sodium sulfate ) under high speed vortexing . transmission and scanning electron microscopy shown that freshly prepared particles are approximately 150 - 300 nm in size and fairly spherical ( fig3 a ). we have also demonstrated previously 41 that the plasmid is partially protected from dnase degradation in this formulation and its gel migration properties are unchanged by the complexation process ( results not shown ). dynamic light scattering ( malvern zetasizer 3000 ) measurements shown an unimodal number average particle size distribution between 100 - 200nm ( fig3 b ). the zeta - potential is approximately + 10 mv at ph 5 . 7 and close to neutral at ph 7 . this suggests that the particles are likely to be positively charged at gastric and early duodenal ph but neutral thereafter at more physiological or alkaline ph . to examine the expression and the distribution of transduced genes following oral dna delivery , akr / j mice were fed with either chitosan - dna nanoparticles containing the lacz gene ( p43lacz ) or with naked plasmid dna ( p43lacz ). fig4 a shows the tissue expression of bacterial β - galacotosidase ( lacz ) in the stomach and small intestine five days after the oral administration . the stained sections represent , on average , 10 % of the whole small intestine . while naive and naked dna fed mice show some background staining , mice fed with the nanoparticles clearly exhibited a higher level of gene expression in both the stomach and the small intestine . fig4 b shows frozen sections of the whole tissue ( shown in 4 a ) counter - stained with nuclear fast red . historically it appears that only epithelial cells in both the stomach and small intestine are strongly stained with x - gal . no staining of hematopoietic cells was observed although immunohistochemistry may not be sensitive enough to identify few transfected immune cells . to investigate the potential utility of oral nanoparticle - mediated gene immunization to modulate mucosal immune response , a murine model of peanut allergen - induced hypersensitivity was used . it has been demonstrated previously 42 , that susceptible strains of mice develop anaphylactic reactions with features similar to those observed in allergic patients . the induction of anaphylaxis was achieved by a combined oral and intraperitoneal ( i . p .) sensitization with crude peanut extract and adjuvants [ cholera toxin ( ctx ) and alum , respectively ], followed by i . p . challenge with recombinant arah2 . the hypersensitivity responses include the induction of specific ige abs , histamine , vascular permeability , and active systemic anaphylaxis . using this model , we first examined whether oral delivery of nanoparticles containing pcmv arah2 was able to induce significant immune response . four weeks after the first immunization , significant differences in the levels of secreted and serum antibodies were observed between nanoparticle - immunized and control ( pbs fed or naive ) or naked dna ( pcmv arah2 ) immunized mice ( fig5 a , b , c ). mice immunized with pcmv arah2 - nanoparticles showed increased levels of secretory iga in fecal extracts , indicating induction of mucosal immune response . in addition , a significant induction of serum anti - arah2 igg2a was observed in nanoparticle - treated animals , indicating a th1 type t cell response . of significance is the finding that mice receiving pcmv arah2 alone ( naked dna ) without chitosan show no detectable levels of either fecal iga or serum igg2a response at any time points . since allergic reactions are primarily characterized by an increase in ag specific serum ige levels , we also measured the levels of anti - arah2 serum ige pre and post sensitization in the immunized and control mice . the increase in serum ige ( post minus pre ) was significantly less pronounced in the nanoparticle - immunized groups compared to that in the control or naked dna immunized animals . fig6 shows the anaphylactic response ( in two separate sets of experiments ) immediately following i . p . challenge with arah2 protein in immunized and control mice one week after the third sensitization with pn . mice receiving sensitization alone without prior immunization or treated with naked dna ( pcmv arah2 ) showed physical signs of anaphylaxis within 10 - 20 min of challenge . the symptoms included slight or no activity after prodding , spasmodic labored breathing with retractions and sometimes death . the severity was ranked 3 to 5 in the scoring system . in contrast , significantly less severe ( score 0 - 2 ) and delayed anaphylactic responses were seen in chitosan - pcmv arah2 - immunized animals following challenge . all animals recovered in about two hours . in the second set of experiments , when challenged after three sensitization one mouse from each immunized and control groups had sudden death that did not appear to be anaphylactic . this phenomenon was not observed in the first set of challenge experiments . the anaphylactic responses of the remaining mice were similar to the first set of experiments and significant delay and decrease were observed in the nanoparticle - immunized animals as described above . histamine release from degranulated mast cells and an increase in vascular permeability are two of the important parameters that characterize anaphylaxis . to examine whether the delayed and less severe pn - induced anaphylactic response seen . in nanoparticle - immunized mice was associated with modulation of histamine release , plasma histamine levels of pn - sensitized , immunized and control mice were assayed 10 - 15 min following arah2 challenge . fig7 a shows that the histamine level . in the single - dose immunized group was significantly lower than the control group . the nanoparticle - booster group , which showed partial protection , however did not exhibit any significant reduction in histamine level . to determine changes in the level of vascular permeability upon challenge , evan &# 39 ; s blue dye was injected through the tail vein of mice from different experimental groups prior to pn challenge . fig7 b shows leakage of evan &# 39 ; s blue from peripheral vasculature ( skin and feet ). mice and chitosan - dna immunized groups show significantly less leakage ( i . e . blue color in the footpad and skin ) compared to mice from the control and naked dna immunized groups . this study demonstrates that chitosan - pdna nanoparticles delivered through the oral route can modify the immune system in mice and protect against food allergen induced hypersensitivity . one of the primary attractions of such an oral vaccine is its potential to generate mucosal as well as systemic immunity . the mucosal immune system is not only geared to protect antigenic entry to the systemic immune system but also be unresponsive to food antigens . peanut allergy is a “ mucosal disease ” in which the usually unreactive immune system becomes hypersensitive to the ingested protein and generates strong , abnormal anaphylactic reactions . to protect the host against food allergen - induced anaphylaxis , it is therefor ideal to pre - modify the mucosal immune system . furthermore , the high patient compliancy in oral administration , especially in children , gives such a delivery system a significant advantage . it has been reported that oral delivery of dna encapsulated in poly - lactide - co - glycolide ( plg ) microspheres can generate immune responses against rotavirus infections . oral gene delivery for correcting lactose intolerance in a rat model has also been achieved using an adeno - associated - viral vector 45 . chitosan is an attractive oral gene carrier because of its reported adhesive and transport properties in the gut . furthermore , chiosan , when complexed with pdna , can form stable nanoparticles that can be endocytosed by cells in the gastro - intestinal tract . chitosan being a mucoadhesive polymer , the dna - nanoparticles might adhere to the gastrointestinal epithelia , transported across the mucosal boundary by m - cells and transect epithelial and / or immune cells in the gut associated lymphoid tissue either directly or through “ antigen transfer ”, as suggested by the β - galactosidase expression following chitosan - p43lacz delivery . in vitro studies have also shown that chitosan can enhance trans and pericellular transport of drugs across intestinal epithelial monolayers . the anaphlaxis response in nanoparticle - immunized mice indicates that significant protection can be achieved against allergen challenge by oral delivery of a single dose of plasmid dna in particle formulation . unfortunately , the results of a single booster administration were inconclusive indicating that further studies are necessary to investigate the effect of multiple doses and kinetics for an optimal vaccination protocol . the level of plasma histamine in the booster group following challenge would not have suggested anaphylactic protection . the fact that same degree of protection was still observed suggests that the pathogenesis of allergic anaphylaxis in this murine model may be multifactorial . while the above examples utilize an ige response to demonstrate principle , this is but one example of a useful response elicited against an antigen . any type of immune response may be modified by oral vaccination using the nanospheres as taught herein . 1 . siraganian , r p . 1993 . mechanism of ige - 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