Effect of Water-Based Microencapsulation on Protection against EDIM Rotavirus Challenge in Mice

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J Virol, May 1998, p. 3859-3862, Vol. 72, No. 5
0022-538X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Effect of Water-Based Microencapsulation on Protection against EDIM Rotavirus Challenge in Mice

Charlotte A. Moser,¹^,^* Tully J. Speaker,² and Paul A. Offit¹^,³^,⁴

Section of Infectious Diseases, The Children's Hospital of Philadelphia,¹ University of Pennsylvania School of Medicine,³ and Wistar Institute of Anatomy and Biology,⁴ Philadelphia, Pennsylvania 19104, and Temple University School of Pharmacy, Philadelphia, Pennsylvania 19140²

Received 20 October 1997/Accepted 9 February 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

We determined the capacity of microcapsules formed by the combination of sodium alginate, an aqueous anionic polymer, andspermine hydrochloride, an aqueous cationic amine, to enhanceprotection against rotavirus challenge in mice. Adult BALB/c micewere orally inoculated with either free or microencapsulated rotavirus(simian rotavirus strain RRV) and challenged 6 or 16 weeks laterwith murine rotavirus strain EDIM. Virus-specific humoral immuneresponses were determined at the time of challenge and 4 daysafter challenge by intestinal fragment culture. We found thatspermine-alginate microcapsules enhanced protection against challenge16 weeks after immunization but not 6 weeks after immunization.Quantities of virus-specific immunoglobulin A produced by smallintestinal lamina propria lymphocytes were correlated with thedegree of protection against challenge afforded by spermine-alginatemicrocapsules. Possible mechanisms by which microcapsules enhanceprotection against rotavirus challenge are discussed.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Development of new vaccines or improvement of existing vaccines may depend on adjuvants that target antigens to specific tissues,eliminate the need for booster dosing, contain multiple antigens,or protect antigens from acids and proteases produced at mucosalsurfaces. One of the most widely studied adjuvant systems is microencapsulation(3, 12, 19, 22). This technique involves capturing antigensin particles typically 1 to 10 µm in size that can be deliveredby various routes.

We developed a water-based system of microencapsulation using anionic polymers (e.g., alginate, chondroitin sulfate, or carboxymethylcellulose) and cationic amines (e.g., spermine or decylamine)that react in a salt exchange to form precipitated microcapsules(18). We found that water-based microcapsules captured infectiousvirus (18), resisted breakdown by gastric acid (18), and enhancedvirus-specific humoral immune responses after oral or intramuscularinoculation (1, 7, 13, 14, 18).

In these studies, we extended our previous findings to include a study of the capacity of water-based microcapsules to enhanceprotection against rotavirus challenge in mice. To evaluate therelationship between humoral immunity and protection against challenge,we used an intestinal fragment culture assay to measure quantitiesof virus-specific and total antibodies produced by small intestinallamina propria lymphocytes (LPL) both at the time of challengeand 4 days after challenge.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Mice. Adult, 6- to 8-week-old, female BALB/c mice or pregnant Swiss-Webster mice were obtained from Taconic Breeding Laboratories(Germantown, N.Y.) and housed in separate isolation units.

Viruses. Rhesus rotavirus strain RRV (P5[3]G3), originally obtained from N. Schmidt (Berkeley, Calif.), was grown and titrated by plaqueassay in fetal green monkey kidney cells (MA-104) as previouslydescribed (17). Murine strain EDIM (P[18]G3), originally obtainedfrom R. Ward (Children's Hospital Research Foundation, Cincinnati,Ohio), was propagated in 7-day-old Swiss-Webster mice. Small intestineswere removed 3 to 4 days after oral inoculation, and 10% (wt/vol)suspensions were prepared in BHK cell medium (11; Wistar Institute,Philadelphia, Pa.). Suspensions were homogenized (PowerGen 125tissue homogenizer; Fisher Scientific, Pittsburgh, Pa.) and storedat $-$ 70°C.

Determination of SD₅₀. Groups of five adult, female BALB/c mice were orally inoculated with one of the following dilutions of EDIM prepared as anintestinal homogenate: 1:10, 1:10², 1:10³, 1:10⁴, 1:10⁵, or 1:10⁶. An average of three fecal pellets were collected from each animaldaily during the 6 days following inoculation. Samples were storedin 0.5 ml of Earle's balanced salt solution (Gibco Life Technologies,Grand Island, N.Y.) at $-$ 20°C and later tested for rotavirus antigenby enzyme-linked immunosorbent assay (ELISA). The 50% sheddingdose (SD₅₀) was calculated to be 1:60,250 by the method of Reedand Muench (20).

Microencapsulation. Five-milliliter aliquots of RRV were suspended in sodium alginate and precipitated in spermine hydrochloride to form spermine-alginate(SA) microcapsules as previously described (18). Microcapsuleswere washed and diluted in distilled water. Aliquots representingapproximately 2% of the entire preparation were disrupted in 2%sodium chloride, and the quantities of rotavirus released weredetermined by plaque assay as previously described (18). Approximately14% of the initial quantity of RRV to be microencapsulated wascaptured within SA microcapsules. Unencapsulated rotavirus wasdiluted in distilled water to correspond to the quantities ofmicroencapsulated rotavirus used to immunize mice.

Inoculation of mice. Groups of 20 mice were orally inoculated with either 2.2 × 10⁷ or 6.0 × 10⁶ PFU of RRV per mouse in SA microcapsules, equivalent quantitiesof unencapsulated RRV, or distilled water. All preparations wereinoculated in a volume of 100 µl by proximal esophogeal intubation.

Challenge of mice. At 6 or 16 weeks after inoculation, five mice per group were challenged orally with 1.2 × 10⁵ SD₅₀s of EDIM virus per mouse in a volume of 200 µl. On eachof the 6 days following challenge, an average of three fecal pelletswere collected from each mouse and placed in 0.5 ml of Earle'sbalanced salts solution. Samples were stored at $-$ 20°C prior todetermination of rotavirus antigen content by ELISA.

ELISA to detect rotavirus in feces. To determine the quantities of rotavirus antigen in feces, 96-well, high-binding, flat-bottom plates (Costar, Cambridge, Mass.)were coated with a 1:2,000 dilution in sodium carbonate buffer(1.5 mM sodium carbonate and 3.5 mM sodium bicarbonate) of serumobtained from cows hyperimmunized with bovine rotavirus strainWC3 (obtained from H Fred Clark, Philadelphia, Pa.). Plates werecovered and incubated overnight at 4°C in a humidified chamber.On the day of the assay, plates were washed (MultiReagent PlateWasher; Dynatech, Chantilly, Va.) four times with wash buffer(1.73 M NaCl, 0.03 M KH₂PO₄, 0.13 M Na₂HPO₄, 0.25% Tween 20; Sigma,St. Louis, Mo.) and two times with distilled H₂O (dH₂O). Individualwells were blocked with 200 µl of blocking buffer (0.5% gelatin[Sigma] containing 0.05% Tween 20) and incubated at room temperaturefor 1 h. Known concentrations of purified rotavirus were testedin duplicate during each assay to establish a standard curve fromwhich to determine quantities of rotavirus antigen in feces. Plateswere washed four times with wash buffer and twice with dH₂O, afterwhich 50 µl of undiluted sample, purified rotavirus, or blockingbuffer was added to each well. A negative control well containingonly blocking buffer was assayed to correspond to each individualsample. Plates were incubated for 1 h and then washed four timesin wash buffer and twice with dH₂O. One hundred microliters ofa 1:2,000 dilution of rabbit antiserum to bovine rotavirus strainWC3 (obtained from H Fred Clark) was added to each well. Plateswere incubated for 1 h at room temperature. After washing, 100µl of a 1:2,000 dilution of alkaline phosphatase-conjugated goatanti-rabbit immunoglobulin G (IgG; Cappel, Durham, N.C.) in blockingbuffer was added to each well. After 1 h at room temperature,plates were washed and 100 µl of developing solution (1 M diethanolamineand p-nitrophenyl phosphate solution; Kirkegaard & Perry Laboratories,Gaithersburg, Md.) was added to each well. One hour later, opticaldensities (OD) were read at a wavelength of 405 nm (Dynatech MR4000;Dynatech). Samples were considered to be positive if the OD inexperimental wells were at least 0.1 U and twofold greater thanthose of the corresponding control wells. Standard curves of purifiedrotavirus were determined by exponential fit (correlation coefficient,>0.90), and quantities of antigen in each sample were calculatedby using the net OD. Averages were calculated for each group oneach day. P values, obtained by Student t tests, of $<=$ 0.05 wereconsidered to be statistically significant.

Intestinal fragment cultures. At 6 or 16 weeks after inoculation of mice, fragment cultures of small intestines were established both at the time of challengeand 4 days after challenge as previously described (6). Briefly,intestines were removed from each animal, cut open longitudinally,and placed in Hanks balanced salt solution (HBSS; GIBCO) on icefor 2 h. Intestinal fragments were then washed twice in HBSS,once in HBSS containing 0.05% EDTA (to remove the intestinal epitheliallayer), and twice with HBSS. Sixteen 1- to 2-mm fragments wereisolated from each group and placed in individual wells of a 24-wellplate (Becton-Dickson, Lincoln Park, N.J.) containing 1 ml ofGALT medium (Kennett's HY medium [JRH, Lenexa, Kans.], 10% fetalbovine serum [GIBCO], 10 mM HEPES, 4 mM L-glutamine, 100-µg/mlstreptomycin, 50-µg/ml gentamicin, 0.025-µg/ml amphotericin B[all additives other than fetal bovine serum were obtained fromJRH]). Samples were placed in a 95% O₂-5% CO₂ environment at 37°Cfor 5 days. Supernatants were collected and stored at 4°C priorto determination of virus-specific and total antibodies.

Use of intestinal fragment cultures eliminated concerns associated with collection of intestinal contents, such as variabledilution of antibodies by osmotic catharsis, entrapment of antibodiesin the intestinal mucin layer, breakdown of antibodies duringcollection or storage, and complexing of antibodies with antigenfollowing challenge. In addition, intestinal fragment culturesallowed the preservation of antigen-presenting cells and antibody-secretingcells in a native microenvironment. Previous studies (15) havedemonstrated the fragment culture technique to be more sensitivethan intestinal lavage. Specifically, antibodies produced by LPLwere not always detected at the surface by lavage; however, thereverse was never observed.

ELISA to determine virus-specific and total antibodies in intestinal fragment cultures. Quantities of virus-specific and total IgG and IgA were determined as previously described (6). Samples were consideredto be positive if OD values in experimental wells were at least0.1 U and twofold greater than those in the corresponding controlwells. Quantities of antibodies were determined by comparisonwith standard curves constructed for either IgA, IgG, or IgM byusing purified murine antibodies (IgA-kappa chain, IgG1-kappachain, or IgM-kappa chain [Sigma]). Standard curves were establishedduring each assay, subjected to exponential fit, and used onlyif the correlation coefficient was greater than 0.90. The lowerlimit of detection was 1 ng/ml for all antibody isotypes. Standarderrors were calculated based on relative percentages of virus-specificand total antibodies among samples in each group.

Statistical analysis. Correlations between reduction of shedding and production of antibody were determined according to Spearman's rank correlationcoefficient, r_s, using Pearson's equation and a two-tailed probability.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

SA microcapsules enhanced protection against rotavirus challenge 16, but not 6, weeks after immunization. Mice orally inoculated 16 weeks previously with 2.2 × 10⁷ PFU of RRV in SA microcapsules shed less rotavirus antigen than didanimals inoculated with the same dose of unencapsulated virus(Table 1). However, protection against shedding in mice immunized6 weeks previously with microencapsulated RRV was either similarto or greater than that observed in animals that received identicaldoses of free virus (Table 1).

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TABLE 1. Average quantities of rotavirus antigen detected in feces at various intervals after challenge in mice immunized 6 or 16 weeks previously with either RRV or RRV in SA^a

Enhanced protection by SA microcapsules was associated with production of virus-specific IgA by small intestinal LPL. Mice inoculated 16 weeks previously with RRV in SA microcapsules developed quantities of virus-specific IgA 4 days after challengethat were approximately 10-fold greater than those found afterchallenge in animals inoculated with unencapsulated RRV (P $<=$ 0.0001;Table 2). Conversely, animals inoculated 6 weeks previously withRRV in SA microcapsules produced less virus-specific IgA 4 daysafter challenge than did mice inoculated with unencapsulated virus(Table 2), although these differences were not statisticallysignificant (P = 0.11).

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TABLE 2. Percentages and quantities of virus-specific and total antibodies detected by fragment culture at the time of and 4 days after challenge in mice immunized previously with RRV or RRV in SA^a

Lesser quantities of virus-specific IgG detected after challenge were also associated with reduced protection against challengein animals immunized 6 weeks previously with microencapsulatedcompared with unencapsulated virus (Tables 1 and 2). However,the presence of virus-specific IgG was not clearly associatedwith enhanced protection against challenge afforded by microencapsulation16 weeks after immunization (Tables 1 and 2). Virus-specificIgM was not detected either at the time of challenge or within4 days of challenge in any group (data not shown).

Virus-specific IgA produced on day 0 was not significantly correlated with reduced shedding (P $<=$ 0.2); however, virus-specificIgA produced on day 4 was correlated with reduced shedding (P $<=$ 0.001).

Immunization of mice with simian strain RRV induced protection against challenge with murine strain EDIM, and protection was not necessarily associated with production of virus-specific IgA by small intestinal LPL. Mice orally inoculated 6 or 16 weeks previously with unencapsulated RRV shed less EDIM in the days immediately following challengethan did unimmunized animals (Table 1). Protection against challengewas not necessarily associated with production of virus-specificIgA, IgG, or IgM at the time of challenge or within 4 days afterchallenge (Table 2).

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Microencapsulation of 2.2 × 10⁷ PFU of RRV in SA microcapsules enhanced protective immune responses 16 weeks after immunization(Table 1). While protection was not associated with virus-specificIgA or IgG at the time of challenge (Table 2), enhanced effectorB-cell responses derived from memory B cells in the days immediatelyfollowing challenge were observed. Specifically, 4 days afterchallenge, virus-specific IgA production was 10-fold greater inmice immunized with RRV in SA microcapsules than in those immunizedwith unencapsulated RRV (Table 2).

There are a number of possible mechanisms by which microencapsulation in SA enhanced protection against challenge. First,microcapsules may protect virus from the acids and proteases encounteredin the digestive tract. However, both RRV and RRV encapsulatedin SA microcapsules are completely inactivated by exposure tosimulated gastric acid (pH 1.2) at room temperature for 1 h (datanot shown). It is possible that although the microcapsules areresistant to breakdown by acid in vitro, influx of protons throughpores in the microcapsule wall allows inactivation of the viruswithin microcapsules. In addition, intramuscular immunizationof mice with rotavirus in SA microcapsules enhanced rotavirus-specificIgG responses (13). Second, microencapsulation of rotavirusin SA microcapsules may select for antigen-presenting cells differentfrom and perhaps more efficient than those involved followinginfection with unencapsulated virus. We found that fluorescentlylabelled SA microcapsules are taken up by dendritic cells in Peyer'spatches to a greater extent than macrophages or B cells afteroral inoculation of mice (10); dendritic cells have been foundto be more efficient at processing and presenting antigens thanother professional antigen-presenting cells in a number of systems(4, 8, 9). Conversely, oral inoculation of mice withEDIM resulted in the detection of rotavirus-specific proteinsprimarily in Peyer's patch macrophages rather than either dendriticcells or B cells (2). Therefore, one possibility is that bydelivering the virus within microcapsules, dendritic cells ratherthan macrophages have the opportunity to process and present theantigen, thereby leading to an alteration in the generation ofthe immune response. However, the relative capacity of macrophagesand dendritic cells to present rotavirus antigens remains to bedetermined. Third, SA microcapsules may delay, prolong, or otherwisealter rotavirus processing and presentation by antigen-presentingcells. Several pieces of evidence support this hypothesis. First,we previously found that virus-specific IgM was produced by LPL60, but not 21, days after oral inoculation of suckling mice withinactivated rotavirus in SA microcapsules (7). In addition,microencapsulation of RRV in SA microcapsules ablated protectiveimmune responses 6 weeks after immunization (Table 1), suggestingthat animals that received microencapsulated virus had not beenexposed to enough virus to generate a protective response equivalentto that of those that received unencapsulated virus.

Determination of the immunologic mechanisms by which microencapsulation enhances protection against rotavirus challenge depends,in part, upon understanding protective immune responses whichoccur after immunization with free virus. Immunization of micewith simian rotavirus strain RRV induced a reduction in virusshedding (partial protection) following challenge with murinerotavirus strain EDIM. At a dose of 2.2 × 10⁷ PFU of RRV per mouse, protection was associated with productionof virus-specific IgA both at the time of challenge and 4 daysafter challenge. However, at a lower dose of RRV (6.0 × 10⁶ PFU of RRV per mouse), protection against challenge detected16 weeks after immunization occurred in the absence of productionof virus-specific IgA or virus-specific IgG at the time of challengeor within 4 days of challenge (Table 2). Therefore, mechanismsother than virus-specific humoral immune responses play a rolein protection against challenge.

The immunologic basis of protection against rotavirus challenge in the absence of production of virus-specific IgA or IgGis unclear. Reduction of virus shedding, which occurred within2 days of challenge, is probably not mediated by virus-specificcytotoxic T lymphocytes (CTLs). First, following immunizationwith RRV, virus-specific CTLs are not detected at the intestinalmucosal surface (among intraepithelial lymphocytes) beyond 6 daysafter infection (16). Second, generation of CTLs from CTL precursorsis unlikely to occur within 2 days (5, 16). Therefore, anothereffector mechanism, possibly secretion of antiviral cytokinesby memory T cells, may be associated with early reduction of sheddingafter challenge.

While the mechanisms responsible for enhanced protection against rotavirus challenge after immunization with microencapsulatedvirus are not completely understood, these findings may impactvaccine design. Although it remains to be determined whether microencapsulationprovides a commercially feasible approach to enhancing vaccine-specificprotective immune responses, a delay in protective immune responsesby microencapsulation may allow the use of unique combinationvaccines that decrease the need for booster doses. Potential applicationsof microcapsules that alter the kinetics of virus-specific immuneresponses will be a subject of future study. In addition, a broaderrange of doses, increased time intervals, and, perhaps, less stringentchallenge doses may help us to gain a better understanding ofthe boundaries of the protection afforded by microencapsulation.

	ACKNOWLEDGMENTS

We thank Tashveen Kaur, David Lim, Jeannette Ouyang, and Daniel Sloane for technical assistance, as well as Kurt Brown, JeffBrubaker, John Cebra, H. Fred Clark, Susan Coffin, and Jenny Krissfor helpful discussions and comments.

This work was supported in part by grant RO1 AI-26251 from the National Institutes of Health to P.A.O.

	FOOTNOTES

^* Corresponding author. Mailing address: Section of Infectious Diseases, The Children's Hospital of Philadelphia, Abramson ResearchCenter, Rm. 1205A, 34th St. and Civic Center Blvd., Philadelphia,PA 19104. Phone: (215) 590-5152 or (215) 590-2186. Fax: (215)590-2025. E-mail: Moser{at}email.chop.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Brown, K. A., C. A. Moser, T. J. Speaker, C. A. Khoury, and P. A. Offit. 1995. Enhancement by microencapsulation of rotavirus-specific intestinal immune responses in mice assessed by enzyme-linked immunospot assay and intestinal fragment culture. J. Infect. Dis. 171:1334-1338[Medline].

2. Brown, K. A., and P. A. Offit. Rotavirus-specific proteins are detected in murine macrophages in both intestinal and extraintestinal lymphoid tissues. Microb. Pathog., in press.

3. Eldridge, J. H., R. M. Gilley, J. K. Staas, Z. Moldoveanu, J. A. Meulbroek, and T. R. Tice. 1989. Biodegradable microspheres: vaccine delivery system for oral immunization. Curr. Top. Microbiol. Immunol. 146:59-66[Medline].

4. Guery, J. C., and L. Adorini. 1995. Dendritic cells are the most efficient in presenting endogenous naturally processed self-epitopes to class II-restricted T cells. J. Immunol. 154:536-544[Abstract].

5. Issekutz, T. B. 1984. Kinetics of cytotoxic lymphocytes in efferent lymph from single lymph nodes following immunization with vaccinia virus. Clin. Exp. Immunol. 56:515-523[Medline].

6. Khoury, C. A., K. Brown, J. Kim, and P. A. Offit. 1994. Rotavirus-specific intestinal immune response in mice assessed by enzyme-linked immunospot assay and intestinal fragment culture. Clin. Diagn. Lab. Immunol. 1:722-728[Abstract/Free Full Text].

7. Khoury, C. A., C. A. Moser, T. J. Speaker, and P. A. Offit. 1995. Oral inoculation of mice with low doses of microencapsulated, noninfectious rotavirus induces virus-specific antibodies in gut-associated lymphoid tissue. J. Infect. Dis. 172:870-874[Medline].

8. Liu, L. M., and G. G. MacPherson. 1991. Lymph-borne (veiled) dendritic cells can acquire and present intestinally administered antigens. Immunology 73:281-286[Medline].

9. Liu, L. M., and G. G. MacPherson. 1993. Antigen acquisition by dendritic cells: intestinal dendritic cells acquire antigen administered orally and can prime naive T cells in vivo. J. Exp. Med. 177:1299-1307[Abstract/Free Full Text].

10. Lomotan, E. A., K. A. Brown, T. J. Speaker, and P. A. Offit. Aqueous-based microcapsules are detected primarily in gut-associated dendritic cells after oral inoculation of mice. Vaccine, in press.

11. MacPherson, I., and M. Stoker. 1982. Polyoma transformation of hamster cell clones: an investigation of genetic factors affecting cell competence. Virology 16:147-151.

12. Morris, W., M. C. Steinhoff, and P. K. Russell. 1994. Potential of polymer microencapsulation technology for vaccine innovation. Vaccine 12:5-11[Medline].

13. Moser, C. A., T. J. Speaker, J. A. Berlin, and P. A. Offit. 1996. Aqueous-based microencapsulation enhances virus-specific humoral immune responses in mice after parenteral inoculation. Vaccine 14:1235-1238[Medline].

14. Moser, C. A., T. J. Speaker, and P. A. Offit. 1997. Effect of microencapsulation on immunogenicity of a bovine herpes virus glycoprotein and inactivated influenza virus in mice. Vaccine 15:1767-1772[Medline].

15. Moser, C. A., S. Cookinham, S. E. Coffin, H. F. Clark, and P. A. Offit. 1998. Relative importance of rotavirus-specific effector and memory B cells in protection against challenge. J. Virol. 72:1108-1114[Abstract/Free Full Text].

16. Offit, P. A., S. L. Cunningham, and K. I. Dudzik. 1991. Memory and distribution of virus-specific cytotoxic T lymphocytes (CTLs) and CTL precursors after rotavirus infection. J. Virol. 65:1318-1324[Abstract/Free Full Text].

17. Offit, P. A., H F. Clark, W. G. Stroop, E. M. Twist, and S. A. Plotkin. 1983. The cultivation of human rotavirus strain "Wa" to high titer in cell culture and characterization of the viral structural polypeptides. J. Virol. Methods 7:29-40[Medline].

18. Offit, P. A., C. A. Khoury, C. A. Moser, H F. Clark, J. E. Kim, and T. J. Speaker. 1994. Enhancement of rotavirus immunogenicity by microencapsulation. Virology 203:134-143[Medline].

19. O'Hagan, D. T. 1994. Microparticles as oral vaccines, p. 175-205. In D. T. O'Hagan (ed.), Novel delivery systems for oral vaccines. CRC Press, Inc., Boca Raton, Fla.

20. Reed, L. J., and H. Muench. 1938. A simple method of estimating fifty per cent endpoints. Am. J. Hyg. 27:493-497.

21. Sah, H. K., R. Toddywala, and Y. W. Chien. 1994. The influence of biodegradable microcapsule formulations on the controlled release of a protein. J. Control. Release 30:201-211.

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1.	Brown, K. A., C. A. Moser, T. J. Speaker, C. A. Khoury, and P. A. Offit. 1995. Enhancement by microencapsulation of rotavirus-specific intestinal immune responses in mice assessed by enzyme-linked immunospot assay and intestinal fragment culture. J. Infect. Dis. 171:1334-1338[Medline].
2.	Brown, K. A., and P. A. Offit. Rotavirus-specific proteins are detected in murine macrophages in both intestinal and extraintestinal lymphoid tissues. Microb. Pathog., in press.
3.	Eldridge, J. H., R. M. Gilley, J. K. Staas, Z. Moldoveanu, J. A. Meulbroek, and T. R. Tice. 1989. Biodegradable microspheres: vaccine delivery system for oral immunization. Curr. Top. Microbiol. Immunol. 146:59-66[Medline].
4.	Guery, J. C., and L. Adorini. 1995. Dendritic cells are the most efficient in presenting endogenous naturally processed self-epitopes to class II-restricted T cells. J. Immunol. 154:536-544[Abstract].
5.	Issekutz, T. B. 1984. Kinetics of cytotoxic lymphocytes in efferent lymph from single lymph nodes following immunization with vaccinia virus. Clin. Exp. Immunol. 56:515-523[Medline].
6.	Khoury, C. A., K. Brown, J. Kim, and P. A. Offit. 1994. Rotavirus-specific intestinal immune response in mice assessed by enzyme-linked immunospot assay and intestinal fragment culture. Clin. Diagn. Lab. Immunol. 1:722-728[Abstract/Free Full Text].
7.	Khoury, C. A., C. A. Moser, T. J. Speaker, and P. A. Offit. 1995. Oral inoculation of mice with low doses of microencapsulated, noninfectious rotavirus induces virus-specific antibodies in gut-associated lymphoid tissue. J. Infect. Dis. 172:870-874[Medline].
8.	Liu, L. M., and G. G. MacPherson. 1991. Lymph-borne (veiled) dendritic cells can acquire and present intestinally administered antigens. Immunology 73:281-286[Medline].
9.	Liu, L. M., and G. G. MacPherson. 1993. Antigen acquisition by dendritic cells: intestinal dendritic cells acquire antigen administered orally and can prime naive T cells in vivo. J. Exp. Med. 177:1299-1307[Abstract/Free Full Text].
10.	Lomotan, E. A., K. A. Brown, T. J. Speaker, and P. A. Offit. Aqueous-based microcapsules are detected primarily in gut-associated dendritic cells after oral inoculation of mice. Vaccine, in press.
11.	MacPherson, I., and M. Stoker. 1982. Polyoma transformation of hamster cell clones: an investigation of genetic factors affecting cell competence. Virology 16:147-151.
12.	Morris, W., M. C. Steinhoff, and P. K. Russell. 1994. Potential of polymer microencapsulation technology for vaccine innovation. Vaccine 12:5-11[Medline].
13.	Moser, C. A., T. J. Speaker, J. A. Berlin, and P. A. Offit. 1996. Aqueous-based microencapsulation enhances virus-specific humoral immune responses in mice after parenteral inoculation. Vaccine 14:1235-1238[Medline].
14.	Moser, C. A., T. J. Speaker, and P. A. Offit. 1997. Effect of microencapsulation on immunogenicity of a bovine herpes virus glycoprotein and inactivated influenza virus in mice. Vaccine 15:1767-1772[Medline].
15.	Moser, C. A., S. Cookinham, S. E. Coffin, H. F. Clark, and P. A. Offit. 1998. Relative importance of rotavirus-specific effector and memory B cells in protection against challenge. J. Virol. 72:1108-1114[Abstract/Free Full Text].
16.	Offit, P. A., S. L. Cunningham, and K. I. Dudzik. 1991. Memory and distribution of virus-specific cytotoxic T lymphocytes (CTLs) and CTL precursors after rotavirus infection. J. Virol. 65:1318-1324[Abstract/Free Full Text].
17.	Offit, P. A., H F. Clark, W. G. Stroop, E. M. Twist, and S. A. Plotkin. 1983. The cultivation of human rotavirus strain "Wa" to high titer in cell culture and characterization of the viral structural polypeptides. J. Virol. Methods 7:29-40[Medline].
18.	Offit, P. A., C. A. Khoury, C. A. Moser, H F. Clark, J. E. Kim, and T. J. Speaker. 1994. Enhancement of rotavirus immunogenicity by microencapsulation. Virology 203:134-143[Medline].
19.	O'Hagan, D. T. 1994. Microparticles as oral vaccines, p. 175-205. In D. T. O'Hagan (ed.), Novel delivery systems for oral vaccines. CRC Press, Inc., Boca Raton, Fla.
20.	Reed, L. J., and H. Muench. 1938. A simple method of estimating fifty per cent endpoints. Am. J. Hyg. 27:493-497.
21.	Sah, H. K., R. Toddywala, and Y. W. Chien. 1994. The influence of biodegradable microcapsule formulations on the controlled release of a protein. J. Control. Release 30:201-211.