The present work illustrates the convenience of using sublingual immunotherapy to boost the innate immune response in the lungs and confer protection against acute pneumococcal pneumonia in mouse.
Sublingual route has been widely used to deliver small molecules into the bloodstream and to modulate the immune response at different sites. It has been shown to effectively induce humoral and cellular responses at systemic and mucosal sites, namely the lungs and urogenital tract. Sublingual vaccination can promote protection against infections at the lower and upper respiratory tract; it can also promote tolerance to allergens and ameliorate asthma symptoms. Modulation of lung’s immune response by sublingual immunotherapy (SLIT) is safer than direct administration of formulations by intranasal route because it does not require delivery of potentially harmful molecules directly into the airways. In contrast to intranasal delivery, side effects involving brain toxicity or facial paralysis are not promoted by SLIT. The immune mechanisms underlying SLIT remain elusive and its use for the treatment of acute lung infections has not yet been explored. Thus, development of appropriate animal models of SLIT is needed to further explore its potential advantages.
This work shows how to perform sublingual administration of therapeutic agents in mice to evaluate their ability to protect against acute pneumococcal pneumonia. Technical aspects of mouse handling during sublingual inoculation, precise identification of sublingual mucosa, draining lymph nodes and isolation of tissues, bronchoalveolar lavage and lungs are illustrated. Protocols for single cell suspension preparation for FACS analysis are described in detail. Other downstream applications for the analysis of the immune response are discussed. Technical aspects of the preparation of Streptococcus pneumoniae inoculum and intranasal challenge of mice are also explained.
SLIT is a simple technique that allows screening of candidate molecules to modulate lungs’ immune response. Parameters affecting the success of SLIT are related to molecular size, susceptibility to degradation and stability of highly concentrated formulations.
The overall goal of this work is to illustrate the benefits of sublingual immunotherapy for the treatment of acute respiratory infections (ARI) and present the advantages of this delivery route compared to other routes of administration, namely intranasal.
ARI cause millions of deaths every year especially in children under five. Streptococcus pneumoniae remains as one of the major etiological agents of bacterial pneumonia in infants and the elderly1,2. To present, the main available treatment relies on the use of antibiotics but resistant strains are continuously arising3,4.
SLIT induces broad responses at systemic and also mucosal level, particularly at the respiratory tract5. It has proven effectiveness against influenza infection, promoting long term protection with production of humoral and cellular responses6,7. Besides, it has been shown that prophylactic treatment with bacterial lysates delivered by sublingual route reduced exacerbations of chronic obstructive bronchitis in the elderly8 and prevented recurrent respiratory infections in children9. SLIT has been widely used for the treatment of allergies and asthma. Clinical studies had not only demonstrated its efficacy to modulate the immune response in the respiratory tract but also its safety10. Despite the growing interest of pharmaceutical companies and researchers in SLIT, the mechanisms involved in the induction of mucosal immune responses after sublingual delivery of compounds remain obscure. Recently, attention has been focused on the mechanisms promoting tolerance associated with allergen desensitization. It has been proposed that resident and recruited cells at the sublingual mucosa, like dendritic cells and macrophages, can promote tolerance after SLIT11-13. Dendritic cells of the oral mucosa can promote IFN-gamma and IL-10 producing T helper cells11 as well as recirculate to the distal genital mucosa and promote CD8+ T cells14. However, little is known about the impact of SLIT on innate cells or its capacity to improve pathogen clearance during acute respiratory infections.
The natural control of pneumococcal infection in the lungs greatly depends on the efficient and swift activation of local innate defences. We previously showed that enhancement of lungs’ innate immunity by a single intranasal dose of flagellin (FliC), a TLR5 and NLRC4 agonist, protects 75-100% of mice challenged with a lethal dose of a clinical isolate of Streptococcus pneumoniae serotype 1. This protection was shown to be dependent on local recruitment of GR1+ cells (likely polymorphonuclear neutrophils, PMNs) and not dependent on antibodies, B or T cells15.
Flagellin is the structural component of the bacterial flagellum. In its monomeric form it is recognized by two Pathogen Recognition Receptors (PRRs), TLR5 that senses extracellular FliC16 and NLRC4/NAIP5 inflammasome that detects intracellular flagellin17,18. When FliC is sensed by the PRRs an important inflammatory response is triggered. We and others have demonstrated that instillation of purified FliC from Salmonella enterica serovar Typhimurium into the lungs drives swift production of chemokines and cytokines specially when recognized by the lungs’ epithelium that in turn orchestrate the recruitment of immune cells into the airways, mainly PMNs15,19-21. Although transient, the substantial neutrophil infiltration that takes place into the airways after nasal delivery of FliC could be a concern if moving towards clinical therapies for human use. Excessive inflammation could be detrimental for the lungs’ function. Moreover, it has been shown that intranasal delivery of immunostimulatory molecules may cause facial paralysis and/or brain toxicity22-24.
Sublingual immunotherapy offers a safer alternative to modulate the immune response in the respiratory tract compared to the intranasal route. It is non-invasive, painless, simple and has good patient compliance25. Furthermore, as mentioned before, it can induce protective responses in the respiratory mucosa without the risks associated to direct intranasal or intrapulmonary delivery of formulations. Sublingual route could be alternatively used to deliver molecules that have great effects onto the lung’s immune system but that have been proven to be toxic or to elicit great inflammation when administered intranasally. Besides these advantages, formulations for sublingual immunotherapy have lower cost of manufacture since non-sterile products can be delivered by this route and endotoxic shock is not a concern for SLIT. On the other hand, it is worth noticing that higher doses of the immunostimulatory compounds compared to those used by intranasal or parenteral routes are necessary to induce an immune response in the lungs; also highly concentrated solutions are needed when using the mouse model of SLIT since the anatomical site where the formulations are deposited is small.
Based on our previous published data, we developed a model of protection using sublingual immunotherapy with flagellin as model immunostimulant. We demonstrated that a single dose of flagellin induced 60% survival against invasive pneumococcal pneumonia caused by the serotype 1 strain while all mice in the control group died of infection within 5 days. Flow cytometry analysis showed that higher numbers of PMN are recruited into the airways of protected animals after sublingual treatment with flagellin suggesting that these cells might be involved in the mechanism of protection induced by sublingual immunotherapy.
This video shows in detail how to perform sublingual immunotherapy and also how to recover relevant tissue from the sublingual mucosa, draining lymph nodes as well as lungs and airways to perform further analysis. Additionally, it illustrates the general technique of cell preparation for FACS analysis and briefly shows how to prepare Streptococcus pneumoniae suspensions and how to perform intranasal infections in mouse to set up the acute infection model.
Sublingual administration af terapeutiske midler har vist sig som et nyttigt middel til at modulere immunresponset i luftvejene. Den største fordel af SLIT til behandling af luftvejssygdomme er, at det ikke indebærer direkte levering af forbindelser til lungerne eller næsebor, er sikrere end behandlinger baseret på intranasal administration 31.
Sublingual immunterapi kan anvendes til at modulere immunreaktionen på forskellige måder, enten til induktion af regulatoriske responser, der kan mildne symptomerne på allergisk inflammation og astma 32 eller at inducere forbigående aktivering af medfødte immunmekanismer til behandling af akutte lungeinfektioner, som vist her.
Den musemodel præsenteres i denne video er en bekvem metode til screening af forskellige forbindelser som terapeutiske midler til SLIT.
Dette dyr model tilbyder et nyttigt middel til at fastslå virkningenaf SLIT reaktion lungerne immunsystem såvel som i andre organer (f.eks., drænende lymfeknuder eller distale slimhinder), der ikke kan efterlignes ved anvendelse af in vitro-modeller. Selv om der er flere papirer, der beskriver resultater opnået ved hjælp af sublingual immunterapi, ikke er blevet fremsat detaljerede metoder til procedurerne i sublingual indgivelse til rådighed endnu. Derudover kan modellen anvendes til evaluering af sublinguale vacciner til formål at give systemisk samt lokal beskyttelse i luftvejene.
Som vist i den ledsagende video, sublingual indgivelse af forbindelser er en simpel procedure, der let kan udføres uden behov for omfattende træning. Typisk vil en person dygtige i håndtering af dyr kræver 1 time at udføre SLIT i en gruppe af 10 mus bruger injicerbar bedøvelsesmidler som beskrevet i denne protokol. Hvis der udføres pneumokok udfordring så godt, vil 90 ekstra minutter skal udarbejdebakteriesuspensionen og udfør intranasal udfordring af dyrene.
FACS protokoller præsenteres her tillader bekvem karakterisering af virkningen af SLIT på det lokale stedet for administration drænende lymfeknuder samt deres effekter på lungerne 'celle dynamik.
Separat analyse af bronkoalveolær indhold og lungeparenkym er vigtigt at skelne luftvejene immunsystem hjemmehørende og infiltrerende celletyper fra dem, der forbliver i vævet. Analyse af BAL indhold muliggør studiet af alveolær makrofag såvel omsætning som dynamikken i cellerne rekruttering til de alveolære rum induceret af forskellige behandlinger, f.eks., PMN'er, eosinofile, monocytter. BAL kan også anvendes til at vurdere tilstedeværelsen af udskilte cytokiner og chemokiner ved enzym-bundet immunosorbent assay (ELISA) eller detektion af secernerede IgA-antistoffer fremkaldt efter sublingual vaccination. Undersøgelse af lungerne 'vævvil tillade karakterisering af andre celletyper, klassisk dendritiske celler, T-celler og B-celler.
Fremstilling af BAL-prøver og lymfeknuder til FACS-analyse er enkel. Efter prøvetagning, normalt 60 minutter kræves for at fuldføre farvningsprotokol i 10-20 prøver. I modsætning hertil vil isolering af celler fra lungerne eller sublinguale væv kræver mere tid, eftersom nedbrydning af den ekstracellulære matrix er påkrævet. Absorption af det terapeutiske middel leveret af sublinguale rute kan løses ved sporing af fluorescens eller radioaktivt mærkede molekyler under anvendelse af in vivo billeddannelse.
Sublingual immunterapi er en attraktiv metode til effektivt at inducere immunresponser i luftvejene samt systemisk, som kan anvendes til at behandle eller forebygge respiratoriske tilstande. Belysning af de mekanismer, der bestemmer aktivering vs tolerance over for immunreaktion i luftvejene efter SLIT Is afgørende at tillade rationelt design af nye terapeutiske strategier, der kan anvendes alene eller i kombination med tilgængelige behandlinger mod forskellige luftvejssygdomme.
The authors have nothing to disclose.
We acknowledge Dr. Jean-Claude Sirard from the Center for Infection and Immunity of Lille, Institute Pasteur de Lille-France, for kindly providing the purified flagellin and Dr. Teresa Camou, Director of the National Reference Laboratory, Ministry of Health of Uruguay for kindly providing the pneumococcal strain.
The authors would like to express their acknowledgement to Mr. Diego Acosta and Mr. Ignacio Turel form BichoFeo Producciones-Uruguay for their commitment and hard work during the entire video production and edition.
This work was supported by the grants PR_FCE_2009_1_2783 and BE_POS_2010_1_2544 from the National Agency of Research and Innovation, ANII from Uruguay, the Program for Development of Basic Sciences, PEDECIBA of Uruguay and Sectoral Commission of Scientific research, CSIC-Universidad de la República, Uruguay.
Name of Material/ Equipment | Company | Catalog Number | Comments/Description |
Ketamine solution (50 mg/ml) | Pharma Service, Uruguay | N/A | |
Xilacine solution (2 %) | Portinco S.A., Uruguay | N/A | |
Sterile 1ml syringe | Modern, Uruguay | N/A | |
Sterile 27G needle | Modern, Uruguay | N/A | |
RPMI 1640 | General Electric Health Care | E15885 | |
Fetal Bovine Serum | ATCC | 302020 | |
Penicillin/Streptimycin Solution | SIGMA | P4333 | |
Sterile PBS without Ca2+/Mg2+ | PAA | H21002 | |
Type-I Collagenase | Life Technologies/Gibco | 17100017 | |
Deoxyribonuclease I (DNAse-I) | SIGMA | D4513 | |
Dispase | Life Technologies/Gibco | 17105041 | |
PerCP-Cy5.5 conjugated rat anti mouse IgG2b anti CD11b | BD | 550993 | Clone M1/70 |
APC conjugated hamster anti mouse IgG1 anti CD11c | BD | 550261 | Clone HL3 |
APC-Cy7 conjugated rat anti mouse IgG2a anti Ly6G | BD | 560600 | Clone 1A8 |
Sterile Saline Solution | Laboratorio Farmaco Uruguayo, Uruguay | N/A | |
Tryptic Soy Agar | BD Difco, France | 236950 | |
Defibrinated Sheep Blood | Biokey, Uruguay | N/A | |
Sterile Petri Dishes | Greiner | 633180 | |
p10 Pipette | Gilson | F144802 | |
P20 Pipette | Eppendorf | 3120000097 | |
p200 Pipette | Gilson | F123601 | |
p200 Pipette | Capp | C200 | |
p200 Pipette | Eppendorf | 3120000054 | |
p1000 Pipette | Eppendorf | 3120000062 | |
Sterile Filter Tips P10 | Greiner | 771288 | |
Sterile Filter Tips P200 | Greiner | 739288 | |
Sterile Filter Tips P1000 | Greiner | 750288 | |
Vortex | BIOSAN | V1-plus | |
Stainless steel fine tip forceps | SIGMA | Z168785/Z168777 | curved and straight |
Dressing tissue forceps | SIGMA | F4392 | length 8 inches |
Micro-dissecting forceps | SIGMA | F4017 | straight |
Micro-dissecting forceps | SIGMA | F4142 | Curved |
Mayo Scissors | SIGMA | Z265993 | |
Scalpel | SAKIRA MEDICAL | N/A | |
Sterile Biopsy Punch Ø 3mm | Stiefel Laboratories Ltd. | 2079D | 5mm diameter can also be used |
Sterile 1.5ml Tubes | Deltalab | 200400P | |
Sterile 15ml Tubes | Greiner | 188271 | |
Sterile 50ml Tubes | Greiner | 227261 | |
Sterile serological pipettes 5 ml | Greiner | 606160 | |
Sterile serological pipettes 10 ml | Greiner | 607160 | |
Sterile serological pipettes 25 ml | Greiner | 760180 | |
Biological safety cabinet, class II | Thermo Scientific | 1300 series, type A2 | |
Micro-Isolator Rack | RAIR IsoSystem | 76144W | Super Mouse 1800 AllerZone |
Refrigerated Microcentfifuge | Eppendorf | Legend Micro 21R | |
Microcentfifuge | Heraeus | Biofuge-pico | |
Centrifuge | Thermo Scientific | Sorval ST40R | |
CO2 Incubator | Thermo Scientific | Model 3111 | |
Sterile Thin-tip pasteur pipettes | Deltalab | D210022 | |
Sterile pasteur pipettes | Deltalab | 200007 | |
Sterile 24-well plate | Greiner | 662160 | |
Trypan Blue Solution | Life Technologies | T10282 | |
Automatic Cell Counter – Cuntess | Life Technologies | C10227 | |
Countess Cell Counting Chamber Slides | Life Technologies | C10312 | |
Flow Cytometry Tubes | BD | 343675 | |
Flow Cytometer – FACS Canto-II | BD | N/A | |
Real Time PCR Instrument – Rotor Gene Q or ABI 7900 | Qiagen / Applied Biosystems | N/A | |
Trizol Reagent | Life Technologies | 15596-026 | Molecular Biology Grade |
DNAse-I | Life Technologies | 18068-015 | Molecular Biology Grade |
DNAse-I Buffer 10X | Life Technologies | 18068015 | Molecular Biology Grade |
EDTA 25 mM | Life Technologies | 18068015 | Molecular Biology Grade |
Ultra-Pure Water | Life Technologies | 10977 | Molecular Biology Grade |
RNAse Out | Life Technologies | 100000840 | Molecular Biology Grade |
Rndom Hexamer Primers | Life Technologies | N8080127 | Molecular Biology Grade |
M-MLV-RT buffer | Life Technologies | 18057-018 | Molecular Biology Grade |
M-MLV-RT enzime | Life Technologies | 28025-021 | Molecular Biology Grade |
QuantiTect Syber Green PCR Kit | Qiagen | 204143 | Molecular Biology Grade |
Specific primers | Life Technologies | N/A | Molecular Biology Grade |